rabbit monoclonal antibody against egr 1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc rabbit monoclonal antibody against egr 1
    Luciferase activity in adult <t>Egr-1-luc</t> mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
    Rabbit Monoclonal Antibody Against Egr 1, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/rabbit monoclonal antibody against egr 1/product/Cell Signaling Technology Inc
    Average 93 stars, based on 1 article reviews
    Price from $9.99 to $1999.99
    rabbit monoclonal antibody against egr 1 - by Bioz Stars, 2023-03
    93/100 stars

    Images

    1) Product Images from "Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing"

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    Journal: BMC Developmental Biology

    doi: 10.1186/1471-213X-11-28

    Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
    Figure Legend Snippet: Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.

    Techniques Used: Luciferase, Activity Assay, Transgenic Assay, Injection

    Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test
    Figure Legend Snippet: Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test

    Techniques Used: Luciferase, Activity Assay, Injection, Standard Deviation

    Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm
    Figure Legend Snippet: Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm

    Techniques Used: Immunohistochemical staining, Luciferase, Expressing, Staining, Transgenic Assay

    Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).
    Figure Legend Snippet: Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Techniques Used: Luciferase, Activity Assay, Standard Deviation, MANN-WHITNEY

    Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in
    Figure Legend Snippet: Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in "Methods". Forty-eight hours after surgery mice were sacrificed, liver tissue fixed in PFA and stained for luciferase (luc). Tissue next to the site of surgery (rim upper left corner in both images) is shown and cells staining positive for luciferase ( A ) as well as Egr-1 ( B ) appear as clusters with brown-reddish staining (arrows; scale bar: 50 μm)

    Techniques Used: Immunohistochemical staining, Luciferase, Expressing, Staining

    mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).
    Figure Legend Snippet: mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Techniques Used: Luciferase, Quantitative RT-PCR, Western Blot, Standard Deviation, MANN-WHITNEY, Expressing

    In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).
    Figure Legend Snippet: In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).

    Techniques Used: In Vivo, Imaging, Luciferase, Standard Deviation, MANN-WHITNEY

    function egr 1 approaches  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc function egr 1 approaches
    ( A ) Time-dependent activation of <t>Egr-1</t> protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.
    Function Egr 1 Approaches, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Average 86 stars, based on 1 article reviews
    Price from $9.99 to $1999.99
    function egr 1 approaches - by Bioz Stars, 2023-03
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    Images

    1) Product Images from "Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability"

    Article Title: Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability

    Journal: PLoS ONE

    doi: 10.1371/journal.pone.0021707

    ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.
    Figure Legend Snippet: ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.

    Techniques Used: Activation Assay, Expressing, Staining

    ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.
    Figure Legend Snippet: ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.

    Techniques Used: Transfection, Dominant Negative Mutation, Construct, Western Blot, Expressing, Binding Assay, Sequencing

    transcription factor egr 1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc transcription factor egr 1
    ( A ) Time-dependent activation of <t>Egr-1</t> protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.
    Transcription Factor Egr 1, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/transcription factor egr 1/product/Cell Signaling Technology Inc
    Average 86 stars, based on 1 article reviews
    Price from $9.99 to $1999.99
    transcription factor egr 1 - by Bioz Stars, 2023-03
    86/100 stars

    Images

    1) Product Images from "Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability"

    Article Title: Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability

    Journal: PLoS ONE

    doi: 10.1371/journal.pone.0021707

    ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.
    Figure Legend Snippet: ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.

    Techniques Used: Activation Assay, Expressing, Staining

    ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.
    Figure Legend Snippet: ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.

    Techniques Used: Transfection, Dominant Negative Mutation, Construct, Western Blot, Expressing, Binding Assay, Sequencing

    rabbit monoclonal antibody against egr 1  (Cell Signaling Technology Inc)


    Bioz Verified Symbol Cell Signaling Technology Inc is a verified supplier
    Bioz Manufacturer Symbol Cell Signaling Technology Inc manufactures this product  
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    Cell Signaling Technology Inc rabbit monoclonal antibody against egr 1
    Luciferase activity in adult <t>Egr-1-luc</t> mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
    Rabbit Monoclonal Antibody Against Egr 1, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/rabbit monoclonal antibody against egr 1/product/Cell Signaling Technology Inc
    Average 93 stars, based on 1 article reviews
    Price from $9.99 to $1999.99
    rabbit monoclonal antibody against egr 1 - by Bioz Stars, 2023-03
    93/100 stars

    Images

    1) Product Images from "Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing"

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    Journal: BMC Developmental Biology

    doi: 10.1186/1471-213X-11-28

    Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
    Figure Legend Snippet: Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.

    Techniques Used: Luciferase, Activity Assay, Transgenic Assay, Injection

    Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test
    Figure Legend Snippet: Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test

    Techniques Used: Luciferase, Activity Assay, Injection, Standard Deviation

    Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm
    Figure Legend Snippet: Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm

    Techniques Used: Immunohistochemical staining, Luciferase, Expressing, Staining, Transgenic Assay

    Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).
    Figure Legend Snippet: Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Techniques Used: Luciferase, Activity Assay, Standard Deviation, MANN-WHITNEY

    Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in
    Figure Legend Snippet: Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in "Methods". Forty-eight hours after surgery mice were sacrificed, liver tissue fixed in PFA and stained for luciferase (luc). Tissue next to the site of surgery (rim upper left corner in both images) is shown and cells staining positive for luciferase ( A ) as well as Egr-1 ( B ) appear as clusters with brown-reddish staining (arrows; scale bar: 50 μm)

    Techniques Used: Immunohistochemical staining, Luciferase, Expressing, Staining

    mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).
    Figure Legend Snippet: mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Techniques Used: Luciferase, Quantitative RT-PCR, Western Blot, Standard Deviation, MANN-WHITNEY, Expressing

    In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).
    Figure Legend Snippet: In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).

    Techniques Used: In Vivo, Imaging, Luciferase, Standard Deviation, MANN-WHITNEY

    egr 1 rabbit monoclonal antibody  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc egr 1 rabbit monoclonal antibody
    Luciferase activity in adult <t>Egr-1-luc</t> mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
    Egr 1 Rabbit Monoclonal Antibody, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Images

    1) Product Images from "Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing"

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    Journal: BMC Developmental Biology

    doi: 10.1186/1471-213X-11-28

    Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
    Figure Legend Snippet: Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.

    Techniques Used: Luciferase, Activity Assay, Transgenic Assay, Injection

    Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test
    Figure Legend Snippet: Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test

    Techniques Used: Luciferase, Activity Assay, Injection, Standard Deviation

    Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm
    Figure Legend Snippet: Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm

    Techniques Used: Immunohistochemical staining, Luciferase, Expressing, Staining, Transgenic Assay

    Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).
    Figure Legend Snippet: Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Techniques Used: Luciferase, Activity Assay, Standard Deviation, MANN-WHITNEY

    Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in
    Figure Legend Snippet: Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in "Methods". Forty-eight hours after surgery mice were sacrificed, liver tissue fixed in PFA and stained for luciferase (luc). Tissue next to the site of surgery (rim upper left corner in both images) is shown and cells staining positive for luciferase ( A ) as well as Egr-1 ( B ) appear as clusters with brown-reddish staining (arrows; scale bar: 50 μm)

    Techniques Used: Immunohistochemical staining, Luciferase, Expressing, Staining

    mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).
    Figure Legend Snippet: mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Techniques Used: Luciferase, Quantitative RT-PCR, Western Blot, Standard Deviation, MANN-WHITNEY, Expressing

    In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).
    Figure Legend Snippet: In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).

    Techniques Used: In Vivo, Imaging, Luciferase, Standard Deviation, MANN-WHITNEY

    anti egr 1  (Cell Signaling Technology Inc)


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    Structured Review

    Cell Signaling Technology Inc anti egr 1
    Protocols of experimental grouping and reagent administering. (a) Protocol used to investigate role of ERK1/2 and <t>Egr-1</t> in extracellular-calcium-containing-H/R injury. (b) Protocol used to investigate role of PKC α /ERK1/2/Egr-1 in extracellular-calcium-containing-H/R injury. (c) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-free-H/R injury. (d) Protocol used to investigate role of cAMP/PKA in extracellular-calcium-free-H/R injury. CaCon, calcium-containing normoxia; CaH/R, calcium-containing H/R; 0CaCon, calcium-free normoxic control; 0CaH/R, calcium-free H/R.
    Anti Egr 1, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/anti egr 1/product/Cell Signaling Technology Inc
    Average 93 stars, based on 1 article reviews
    Price from $9.99 to $1999.99
    anti egr 1 - by Bioz Stars, 2023-03
    93/100 stars

    Images

    1) Product Images from "N -n-Butyl Haloperidol Iodide Ameliorates Cardiomyocytes Hypoxia/Reoxygenation Injury by Extracellular Calcium-Dependent and -Independent Mechanisms"

    Article Title: N -n-Butyl Haloperidol Iodide Ameliorates Cardiomyocytes Hypoxia/Reoxygenation Injury by Extracellular Calcium-Dependent and -Independent Mechanisms

    Journal: Oxidative Medicine and Cellular Longevity

    doi: 10.1155/2013/912310

    Protocols of experimental grouping and reagent administering. (a) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-containing-H/R injury. (b) Protocol used to investigate role of PKC α /ERK1/2/Egr-1 in extracellular-calcium-containing-H/R injury. (c) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-free-H/R injury. (d) Protocol used to investigate role of cAMP/PKA in extracellular-calcium-free-H/R injury. CaCon, calcium-containing normoxia; CaH/R, calcium-containing H/R; 0CaCon, calcium-free normoxic control; 0CaH/R, calcium-free H/R.
    Figure Legend Snippet: Protocols of experimental grouping and reagent administering. (a) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-containing-H/R injury. (b) Protocol used to investigate role of PKC α /ERK1/2/Egr-1 in extracellular-calcium-containing-H/R injury. (c) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-free-H/R injury. (d) Protocol used to investigate role of cAMP/PKA in extracellular-calcium-free-H/R injury. CaCon, calcium-containing normoxia; CaH/R, calcium-containing H/R; 0CaCon, calcium-free normoxic control; 0CaH/R, calcium-free H/R.

    Techniques Used:

    Effects of F 2 , Verapamil, and ERK1/2 inhibitors and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-ERK1/2 and total ERK1/2; (b) Egr-1 protein. Quantitative densitometric data were expressed as percentages of the level observed in the CaCon group. All values are expressed as mean ± SEM of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.
    Figure Legend Snippet: Effects of F 2 , Verapamil, and ERK1/2 inhibitors and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-ERK1/2 and total ERK1/2; (b) Egr-1 protein. Quantitative densitometric data were expressed as percentages of the level observed in the CaCon group. All values are expressed as mean ± SEM of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.

    Techniques Used: Expressing, Western Blot

    Effects of F 2 , Verapamil, and PKC α inhibitor and activator on p-PKC α , total PKC α , p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-PKC α and total PKC α protein levels; (b) p-ERK1/2 and total ERK1/2 protein levels; (c) Egr-1 protein levels. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.
    Figure Legend Snippet: Effects of F 2 , Verapamil, and PKC α inhibitor and activator on p-PKC α , total PKC α , p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-PKC α and total PKC α protein levels; (b) p-ERK1/2 and total ERK1/2 protein levels; (c) Egr-1 protein levels. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.

    Techniques Used: Expressing, Western Blot

    Effects of F 2 , ERK1/2 inhibitors, and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-free myocardial H/R by western-blot assay. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus 0CaCon group; # P < 0.05 versus 0CaH/R group; † P < 0.05 versus 0CaH/R+F 2 group.
    Figure Legend Snippet: Effects of F 2 , ERK1/2 inhibitors, and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-free myocardial H/R by western-blot assay. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus 0CaCon group; # P < 0.05 versus 0CaH/R group; † P < 0.05 versus 0CaH/R+F 2 group.

    Techniques Used: Expressing, Western Blot

    rabbit anti egr 1 antibody  (Cell Signaling Technology Inc)


    Bioz Verified Symbol Cell Signaling Technology Inc is a verified supplier
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    Cell Signaling Technology Inc rabbit anti egr 1 antibody
    (A) HMEC-1s and HUVECs were incubated with SW480-derived EVs (1 µg/mL) or untreated control. mRNA was isolated from untreated control cells or cells treated with EVs for 0, 0.5, 1, 2, and 4 h and analyzed using real time RT-PCR (n = 3). Values represent <t>Egr-1</t> mRNA/GAPDH mRNA normalized to untreated control cells. (B) HMEC-1s were treated with EVs (1 µg/mL) derived from HCT116 colorectal carcinoma, A549 lung adenocarcinoma, HT1080 fibrosarcoma, PC3 prostate carcinoma, SH-SY5Y neuroblastoma, and BEAS-2B normal bronchial epithelial cells for 0.5 h (n = 3). (C, D) In HMEC-1s, nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 0.5, 1, 2, and 4 h was analyzed under confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel C. Scale bars represent 30 µm. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over that of total cells (D). Data are represented as mean ± SD. * P <0.05; ** P <0.01; ** P <0.001; n.s., not significant.
    Rabbit Anti Egr 1 Antibody, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/rabbit anti egr 1 antibody/product/Cell Signaling Technology Inc
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    Images

    1) Product Images from "Egr-1 Activation by Cancer-Derived Extracellular Vesicles Promotes Endothelial Cell Migration via ERK1/2 and JNK Signaling Pathways"

    Article Title: Egr-1 Activation by Cancer-Derived Extracellular Vesicles Promotes Endothelial Cell Migration via ERK1/2 and JNK Signaling Pathways

    Journal: PLoS ONE

    doi: 10.1371/journal.pone.0115170

    (A) HMEC-1s and HUVECs were incubated with SW480-derived EVs (1 µg/mL) or untreated control. mRNA was isolated from untreated control cells or cells treated with EVs for 0, 0.5, 1, 2, and 4 h and analyzed using real time RT-PCR (n = 3). Values represent Egr-1 mRNA/GAPDH mRNA normalized to untreated control cells. (B) HMEC-1s were treated with EVs (1 µg/mL) derived from HCT116 colorectal carcinoma, A549 lung adenocarcinoma, HT1080 fibrosarcoma, PC3 prostate carcinoma, SH-SY5Y neuroblastoma, and BEAS-2B normal bronchial epithelial cells for 0.5 h (n = 3). (C, D) In HMEC-1s, nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 0.5, 1, 2, and 4 h was analyzed under confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel C. Scale bars represent 30 µm. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over that of total cells (D). Data are represented as mean ± SD. * P <0.05; ** P <0.01; ** P <0.001; n.s., not significant.
    Figure Legend Snippet: (A) HMEC-1s and HUVECs were incubated with SW480-derived EVs (1 µg/mL) or untreated control. mRNA was isolated from untreated control cells or cells treated with EVs for 0, 0.5, 1, 2, and 4 h and analyzed using real time RT-PCR (n = 3). Values represent Egr-1 mRNA/GAPDH mRNA normalized to untreated control cells. (B) HMEC-1s were treated with EVs (1 µg/mL) derived from HCT116 colorectal carcinoma, A549 lung adenocarcinoma, HT1080 fibrosarcoma, PC3 prostate carcinoma, SH-SY5Y neuroblastoma, and BEAS-2B normal bronchial epithelial cells for 0.5 h (n = 3). (C, D) In HMEC-1s, nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 0.5, 1, 2, and 4 h was analyzed under confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel C. Scale bars represent 30 µm. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over that of total cells (D). Data are represented as mean ± SD. * P <0.05; ** P <0.01; ** P <0.001; n.s., not significant.

    Techniques Used: Incubation, Derivative Assay, Isolation, Quantitative RT-PCR, Translocation Assay, Confocal Microscopy, Staining, Fluorescence

    (A) HMEC-1s were transfected with 50 nM of scrambled siRNA or Egr-1 siRNA-1, Egr-1 siRNA-2, or Egr-1 siRNA-3. mRNAs were isolated from the cells after 48 h and the level of Egr-1 mRNA was analyzed using real time RT-PCR (n = 3). (B) Nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 1 h was analyzed in scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) transfected HMEC-1s (n = 3). (C, D) Confluent HMEC-1s transfected with scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) were scratched and treated with SW480-derived EVs (1 µg/mL); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). The number of migrated cells in the denuded zone of each group is shown in panel D. Scale bars represent 100 µm. Data are represented as mean ± SD. * P <0.05; ** P <0.01; *** P <0.001; n.s., not significant.
    Figure Legend Snippet: (A) HMEC-1s were transfected with 50 nM of scrambled siRNA or Egr-1 siRNA-1, Egr-1 siRNA-2, or Egr-1 siRNA-3. mRNAs were isolated from the cells after 48 h and the level of Egr-1 mRNA was analyzed using real time RT-PCR (n = 3). (B) Nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 1 h was analyzed in scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) transfected HMEC-1s (n = 3). (C, D) Confluent HMEC-1s transfected with scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) were scratched and treated with SW480-derived EVs (1 µg/mL); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). The number of migrated cells in the denuded zone of each group is shown in panel D. Scale bars represent 100 µm. Data are represented as mean ± SD. * P <0.05; ** P <0.01; *** P <0.001; n.s., not significant.

    Techniques Used: Transfection, Isolation, Quantitative RT-PCR, Translocation Assay, Derivative Assay

    (A, B) HMEC-1s were pretreated with signaling inhibitors for 1 h and then stimulated for 1 h with SW480-derived EVs (1 µg/mL). Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel A. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over total cells (B). (C, D) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of signaling inhibitors; then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). Representative photographs of confocal microscopic imaging are shown in panel C and the number of migrated cells in the denuded zone of each group is shown in panel D. ERK1/2 inhibitor, PD98059 (20 µM); p38 MAPK inhibitor, SB203580 (10 µM); JNK inhibitor, SP600125 (20 µM); Akt inhibitor, BML-257 (20 µM). (E, F) C57BL/6 mice were subcutaneously injected with Matrigel containing SW480-derived EVs (20 µg) with PD98059 (20 µM) or SP600125 (20 µM). After 7 days, whole-mount staining of Matrigel with anti-CD31 antibody was conducted (n = 5). Representative confocal Z-stack photographs of whole mounts stained for CD31 (green) are shown in panel E. Fluorescence intensities of CD31 in the Z-stack plane of the Matrigel were measured as described in the (F). Scale bars in panels A, C, and E represent 30, 100, and 100 µm, respectively. Data are represented as mean ± SD. *** P <0.001.
    Figure Legend Snippet: (A, B) HMEC-1s were pretreated with signaling inhibitors for 1 h and then stimulated for 1 h with SW480-derived EVs (1 µg/mL). Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel A. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over total cells (B). (C, D) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of signaling inhibitors; then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). Representative photographs of confocal microscopic imaging are shown in panel C and the number of migrated cells in the denuded zone of each group is shown in panel D. ERK1/2 inhibitor, PD98059 (20 µM); p38 MAPK inhibitor, SB203580 (10 µM); JNK inhibitor, SP600125 (20 µM); Akt inhibitor, BML-257 (20 µM). (E, F) C57BL/6 mice were subcutaneously injected with Matrigel containing SW480-derived EVs (20 µg) with PD98059 (20 µM) or SP600125 (20 µM). After 7 days, whole-mount staining of Matrigel with anti-CD31 antibody was conducted (n = 5). Representative confocal Z-stack photographs of whole mounts stained for CD31 (green) are shown in panel E. Fluorescence intensities of CD31 in the Z-stack plane of the Matrigel were measured as described in the (F). Scale bars in panels A, C, and E represent 30, 100, and 100 µm, respectively. Data are represented as mean ± SD. *** P <0.001.

    Techniques Used: Derivative Assay, Translocation Assay, Confocal Microscopy, Staining, Fluorescence, Imaging, Injection

    (A) HMEC-1s were treated with DiI-labeled SW480-derived EVs (1 µg/mL) for 1 h in the presence or absence of MβCD (10 mM) (n = 3). SW480-derived EVs and nuclei were stained with DiI (red) and Hoechst (blue) respectively. Representative photographs are shown in panel A. Scale bars represent 10 µm. (B) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of MβCD (10 mM); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). (C, D) HMEC-1s were pretreated with MβCD (10 mM) for 1 h and then stimulated with SW480-derived EVs (1 µg/mL) for 1 h. Scale bars represent 30 µm. Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy and the percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus co-localized signals over that of total cells (n = 3). Data are represented as mean ± SD. *** P <0.001.
    Figure Legend Snippet: (A) HMEC-1s were treated with DiI-labeled SW480-derived EVs (1 µg/mL) for 1 h in the presence or absence of MβCD (10 mM) (n = 3). SW480-derived EVs and nuclei were stained with DiI (red) and Hoechst (blue) respectively. Representative photographs are shown in panel A. Scale bars represent 10 µm. (B) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of MβCD (10 mM); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). (C, D) HMEC-1s were pretreated with MβCD (10 mM) for 1 h and then stimulated with SW480-derived EVs (1 µg/mL) for 1 h. Scale bars represent 30 µm. Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy and the percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus co-localized signals over that of total cells (n = 3). Data are represented as mean ± SD. *** P <0.001.

    Techniques Used: Labeling, Derivative Assay, Staining, Translocation Assay, Confocal Microscopy

    egr 1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc egr 1
    Egr 1, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    rabbit monoclonal antibodies egr  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc rabbit monoclonal antibodies egr
    Growth-quiescent SMCs were treated with MMP inhibitor GM6001+ (25 µM) and TAPI-1 (10 µM) for 30 min before stimulation with IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) <t>Egr-1</t> mRNA levels in GM6001+ or GM6001- treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs treated with GM6001+ or GM6001-. ( C ) Egr-1 mRNA levels in TAPI-1 treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( D ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with TAPI-1. DMSO was used as a carrier. ( E ) Western blotting for ADAM17, ADAM10, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ADAM17 siRNA (0.1 µM) and treated with IL-1beta for 30 min.
    Rabbit Monoclonal Antibodies Egr, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    1) Product Images from "IL-1beta Signals through the EGF Receptor and Activates Egr-1 through MMP-ADAM"

    Article Title: IL-1beta Signals through the EGF Receptor and Activates Egr-1 through MMP-ADAM

    Journal: PLoS ONE

    doi: 10.1371/journal.pone.0039811

    Growth-quiescent SMCs were treated with MMP inhibitor GM6001+ (25 µM) and TAPI-1 (10 µM) for 30 min before stimulation with IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in GM6001+ or GM6001- treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs treated with GM6001+ or GM6001-. ( C ) Egr-1 mRNA levels in TAPI-1 treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( D ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with TAPI-1. DMSO was used as a carrier. ( E ) Western blotting for ADAM17, ADAM10, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ADAM17 siRNA (0.1 µM) and treated with IL-1beta for 30 min.
    Figure Legend Snippet: Growth-quiescent SMCs were treated with MMP inhibitor GM6001+ (25 µM) and TAPI-1 (10 µM) for 30 min before stimulation with IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in GM6001+ or GM6001- treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs treated with GM6001+ or GM6001-. ( C ) Egr-1 mRNA levels in TAPI-1 treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( D ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with TAPI-1. DMSO was used as a carrier. ( E ) Western blotting for ADAM17, ADAM10, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ADAM17 siRNA (0.1 µM) and treated with IL-1beta for 30 min.

    Techniques Used: Western Blot, Transfection

    Growth-quiescent SMCs were incubated with EGFR inhibitors AG1478 (5 µM) and PD153035 (5 µM) for 30 min, and exposed to IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in AG1478- and PD153035-treated SMCs incubated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with AG1478 or PD153035. ( C ) Western blotting for EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with EGFR siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( D ) Western blotting for ErbB4, EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ErbB4 siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( E ) Egr-1 mRNA levels in AG825 (10 µM for 30 min)-treated SMCs incubated with IL-1beta for 30 min by qPCR. Data were normalized to beta-actin. ( F ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs pretreated with AG825 (10 µM for 30 min) then stimulated with IL-1beta for another 30 min.
    Figure Legend Snippet: Growth-quiescent SMCs were incubated with EGFR inhibitors AG1478 (5 µM) and PD153035 (5 µM) for 30 min, and exposed to IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in AG1478- and PD153035-treated SMCs incubated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with AG1478 or PD153035. ( C ) Western blotting for EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with EGFR siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( D ) Western blotting for ErbB4, EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ErbB4 siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( E ) Egr-1 mRNA levels in AG825 (10 µM for 30 min)-treated SMCs incubated with IL-1beta for 30 min by qPCR. Data were normalized to beta-actin. ( F ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs pretreated with AG825 (10 µM for 30 min) then stimulated with IL-1beta for another 30 min.

    Techniques Used: Incubation, Western Blot, Transfection

    ( A ) Growth-quiescent SMCs were stimulated with IL-1beta (10 ng/ml) for the indicated times. Total protein extracts were resolved by SDS-PAGE and subjected to Western blot analysis using antibodies for Egr-1, EGFR phospho-Tyr 845 , total EGFR and beta-actin. Alternatively, Western blotting for EGFR phospho-Tyr 845 or EGFR of total extracts of SMCs treated with ( B ) AG1478 (5 µM), ( C ) GM6001+ or GM6001- (25 µM) ( D ) TAPI-1 (10 µM), PD153035 (5 µM) for 30 min followed by IL-1beta stimulation for 5 min.
    Figure Legend Snippet: ( A ) Growth-quiescent SMCs were stimulated with IL-1beta (10 ng/ml) for the indicated times. Total protein extracts were resolved by SDS-PAGE and subjected to Western blot analysis using antibodies for Egr-1, EGFR phospho-Tyr 845 , total EGFR and beta-actin. Alternatively, Western blotting for EGFR phospho-Tyr 845 or EGFR of total extracts of SMCs treated with ( B ) AG1478 (5 µM), ( C ) GM6001+ or GM6001- (25 µM) ( D ) TAPI-1 (10 µM), PD153035 (5 µM) for 30 min followed by IL-1beta stimulation for 5 min.

    Techniques Used: SDS Page, Western Blot

    ( A ) Western blotting for Egr-1, ADAM17, EGFR, IL-1RI or beta-actin using total extracts of growth-quiescent wild-type or ADAM17-deficient mEFs treated with IL-1beta for 30 or 60 min. ( B ) Interaction of 125 I-IL-1beta with ADAM17WT and ADAM17-deficient cells. Growth-quiescent ADAM17WT and ADAM17−/− mEFs (1.8×10 4 cells/well) were incubated with increasing amounts of 125 I-IL-1beta in 1% BSA/PBS for 1 h at 4°C. The cells were washed and lysed with 1M NaOH prior to assessment of counts in an automated gamma-counter.
    Figure Legend Snippet: ( A ) Western blotting for Egr-1, ADAM17, EGFR, IL-1RI or beta-actin using total extracts of growth-quiescent wild-type or ADAM17-deficient mEFs treated with IL-1beta for 30 or 60 min. ( B ) Interaction of 125 I-IL-1beta with ADAM17WT and ADAM17-deficient cells. Growth-quiescent ADAM17WT and ADAM17−/− mEFs (1.8×10 4 cells/well) were incubated with increasing amounts of 125 I-IL-1beta in 1% BSA/PBS for 1 h at 4°C. The cells were washed and lysed with 1M NaOH prior to assessment of counts in an automated gamma-counter.

    Techniques Used: Western Blot, Incubation

    egr 1 antibody  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc egr 1 antibody
    <t>EGR-1</t> deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.
    Egr 1 Antibody, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    1) Product Images from "Loss of EGR-1 uncouples compensatory responses of pancreatic β cells"

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    Journal: Theranostics

    doi: 10.7150/thno.40664

    EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.
    Figure Legend Snippet: EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.

    Techniques Used: Immunofluorescence, Staining, Isolation, Western Blot

    Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.
    Figure Legend Snippet: Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.

    Techniques Used: Binding Assay, Expressing, Isolation, Software, Real-time Polymerase Chain Reaction, Amplification

    The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.
    Figure Legend Snippet: The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.

    Techniques Used: Expressing

    egr 1 protein  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc egr 1 protein
    <t>EGR-1</t> deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.
    Egr 1 Protein, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    1) Product Images from "Loss of EGR-1 uncouples compensatory responses of pancreatic β cells"

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    Journal: Theranostics

    doi: 10.7150/thno.40664

    EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.
    Figure Legend Snippet: EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.

    Techniques Used: Immunofluorescence, Staining, Isolation, Western Blot

    Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.
    Figure Legend Snippet: Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.

    Techniques Used: Binding Assay, Expressing, Isolation, Software, Real-time Polymerase Chain Reaction, Amplification

    The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.
    Figure Legend Snippet: The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.

    Techniques Used: Expressing

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    Luciferase activity in adult <t>Egr-1-luc</t> mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
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    ( A ) Time-dependent activation of <t>Egr-1</t> protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.
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    ( A ) Time-dependent activation of <t>Egr-1</t> protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.
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    egr 1 rabbit monoclonal antibody  (Cell Signaling Technology Inc)
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    Luciferase activity in adult <t>Egr-1-luc</t> mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.
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    anti egr 1  (Cell Signaling Technology Inc)
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    Protocols of experimental grouping and reagent administering. (a) Protocol used to investigate role of ERK1/2 and <t>Egr-1</t> in extracellular-calcium-containing-H/R injury. (b) Protocol used to investigate role of PKC α /ERK1/2/Egr-1 in extracellular-calcium-containing-H/R injury. (c) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-free-H/R injury. (d) Protocol used to investigate role of cAMP/PKA in extracellular-calcium-free-H/R injury. CaCon, calcium-containing normoxia; CaH/R, calcium-containing H/R; 0CaCon, calcium-free normoxic control; 0CaH/R, calcium-free H/R.
    Anti Egr 1, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    rabbit anti egr 1 antibody  (Cell Signaling Technology Inc)
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    (A) HMEC-1s and HUVECs were incubated with SW480-derived EVs (1 µg/mL) or untreated control. mRNA was isolated from untreated control cells or cells treated with EVs for 0, 0.5, 1, 2, and 4 h and analyzed using real time RT-PCR (n = 3). Values represent <t>Egr-1</t> mRNA/GAPDH mRNA normalized to untreated control cells. (B) HMEC-1s were treated with EVs (1 µg/mL) derived from HCT116 colorectal carcinoma, A549 lung adenocarcinoma, HT1080 fibrosarcoma, PC3 prostate carcinoma, SH-SY5Y neuroblastoma, and BEAS-2B normal bronchial epithelial cells for 0.5 h (n = 3). (C, D) In HMEC-1s, nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 0.5, 1, 2, and 4 h was analyzed under confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel C. Scale bars represent 30 µm. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over that of total cells (D). Data are represented as mean ± SD. * P <0.05; ** P <0.01; ** P <0.001; n.s., not significant.
    Rabbit Anti Egr 1 Antibody, supplied by Cell Signaling Technology Inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    egr 1  (Cell Signaling Technology Inc)
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    (A) HMEC-1s and HUVECs were incubated with SW480-derived EVs (1 µg/mL) or untreated control. mRNA was isolated from untreated control cells or cells treated with EVs for 0, 0.5, 1, 2, and 4 h and analyzed using real time RT-PCR (n = 3). Values represent <t>Egr-1</t> mRNA/GAPDH mRNA normalized to untreated control cells. (B) HMEC-1s were treated with EVs (1 µg/mL) derived from HCT116 colorectal carcinoma, A549 lung adenocarcinoma, HT1080 fibrosarcoma, PC3 prostate carcinoma, SH-SY5Y neuroblastoma, and BEAS-2B normal bronchial epithelial cells for 0.5 h (n = 3). (C, D) In HMEC-1s, nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 0.5, 1, 2, and 4 h was analyzed under confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel C. Scale bars represent 30 µm. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over that of total cells (D). Data are represented as mean ± SD. * P <0.05; ** P <0.01; ** P <0.001; n.s., not significant.
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    rabbit monoclonal antibodies egr  (Cell Signaling Technology Inc)
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    Growth-quiescent SMCs were treated with MMP inhibitor GM6001+ (25 µM) and TAPI-1 (10 µM) for 30 min before stimulation with IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) <t>Egr-1</t> mRNA levels in GM6001+ or GM6001- treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs treated with GM6001+ or GM6001-. ( C ) Egr-1 mRNA levels in TAPI-1 treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( D ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with TAPI-1. DMSO was used as a carrier. ( E ) Western blotting for ADAM17, ADAM10, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ADAM17 siRNA (0.1 µM) and treated with IL-1beta for 30 min.
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    egr 1 antibody  (Cell Signaling Technology Inc)
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    <t>EGR-1</t> deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.
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    <t>EGR-1</t> deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.
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    Image Search Results


    Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.

    Article Snippet: Equal amounts of protein were separated on a 4-20% Tris-glycine gel (Serva) and immunoreactive bands were visualized using Super-Signal-Femto-West (Pierce) with a HRP conjugated rabbit polyclonal antibody against firefly luciferase (1:1000, Santa Cruz Biotechnology), a rabbit monoclonal antibody against Egr-1 (1:500, Cell Signaling) or β-actin (1:2000, Sigma), respectively.

    Techniques: Luciferase, Activity Assay, Transgenic Assay, Injection

    Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test

    Article Snippet: Equal amounts of protein were separated on a 4-20% Tris-glycine gel (Serva) and immunoreactive bands were visualized using Super-Signal-Femto-West (Pierce) with a HRP conjugated rabbit polyclonal antibody against firefly luciferase (1:1000, Santa Cruz Biotechnology), a rabbit monoclonal antibody against Egr-1 (1:500, Cell Signaling) or β-actin (1:2000, Sigma), respectively.

    Techniques: Luciferase, Activity Assay, Injection, Standard Deviation

    Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm

    Article Snippet: Equal amounts of protein were separated on a 4-20% Tris-glycine gel (Serva) and immunoreactive bands were visualized using Super-Signal-Femto-West (Pierce) with a HRP conjugated rabbit polyclonal antibody against firefly luciferase (1:1000, Santa Cruz Biotechnology), a rabbit monoclonal antibody against Egr-1 (1:500, Cell Signaling) or β-actin (1:2000, Sigma), respectively.

    Techniques: Immunohistochemical staining, Luciferase, Expressing, Staining, Transgenic Assay

    Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Article Snippet: Equal amounts of protein were separated on a 4-20% Tris-glycine gel (Serva) and immunoreactive bands were visualized using Super-Signal-Femto-West (Pierce) with a HRP conjugated rabbit polyclonal antibody against firefly luciferase (1:1000, Santa Cruz Biotechnology), a rabbit monoclonal antibody against Egr-1 (1:500, Cell Signaling) or β-actin (1:2000, Sigma), respectively.

    Techniques: Luciferase, Activity Assay, Standard Deviation, MANN-WHITNEY

    Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in "Methods". Forty-eight hours after surgery mice were sacrificed, liver tissue fixed in PFA and stained for luciferase (luc). Tissue next to the site of surgery (rim upper left corner in both images) is shown and cells staining positive for luciferase ( A ) as well as Egr-1 ( B ) appear as clusters with brown-reddish staining (arrows; scale bar: 50 μm)

    Article Snippet: Equal amounts of protein were separated on a 4-20% Tris-glycine gel (Serva) and immunoreactive bands were visualized using Super-Signal-Femto-West (Pierce) with a HRP conjugated rabbit polyclonal antibody against firefly luciferase (1:1000, Santa Cruz Biotechnology), a rabbit monoclonal antibody against Egr-1 (1:500, Cell Signaling) or β-actin (1:2000, Sigma), respectively.

    Techniques: Immunohistochemical staining, Luciferase, Expressing, Staining

    mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Article Snippet: Equal amounts of protein were separated on a 4-20% Tris-glycine gel (Serva) and immunoreactive bands were visualized using Super-Signal-Femto-West (Pierce) with a HRP conjugated rabbit polyclonal antibody against firefly luciferase (1:1000, Santa Cruz Biotechnology), a rabbit monoclonal antibody against Egr-1 (1:500, Cell Signaling) or β-actin (1:2000, Sigma), respectively.

    Techniques: Luciferase, Quantitative RT-PCR, Western Blot, Standard Deviation, MANN-WHITNEY, Expressing

    In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).

    Article Snippet: Equal amounts of protein were separated on a 4-20% Tris-glycine gel (Serva) and immunoreactive bands were visualized using Super-Signal-Femto-West (Pierce) with a HRP conjugated rabbit polyclonal antibody against firefly luciferase (1:1000, Santa Cruz Biotechnology), a rabbit monoclonal antibody against Egr-1 (1:500, Cell Signaling) or β-actin (1:2000, Sigma), respectively.

    Techniques: In Vivo, Imaging, Luciferase, Standard Deviation, MANN-WHITNEY

    ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.

    Journal: PLoS ONE

    Article Title: Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability

    doi: 10.1371/journal.pone.0021707

    Figure Lengend Snippet: ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.

    Article Snippet: Pharmacological blockade (cell signaling) and loss-of-function (Egr-1) approaches demonstrated the role of mitogen-activated protein kinases (MAPKs), PI3K/Akt and the downstream transcription factor Egr-1 respectively, in morphine-mediated induction of PDGF-BB.

    Techniques: Activation Assay, Expressing, Staining

    ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.

    Journal: PLoS ONE

    Article Title: Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability

    doi: 10.1371/journal.pone.0021707

    Figure Lengend Snippet: ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.

    Article Snippet: Pharmacological blockade (cell signaling) and loss-of-function (Egr-1) approaches demonstrated the role of mitogen-activated protein kinases (MAPKs), PI3K/Akt and the downstream transcription factor Egr-1 respectively, in morphine-mediated induction of PDGF-BB.

    Techniques: Transfection, Dominant Negative Mutation, Construct, Western Blot, Expressing, Binding Assay, Sequencing

    ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.

    Journal: PLoS ONE

    Article Title: Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability

    doi: 10.1371/journal.pone.0021707

    Figure Lengend Snippet: ( A ) Time-dependent activation of Egr-1 protein expression by morphine in HBMECs. ( B ) Representative image of Egr-1 staining in HBMECs treated with morphine. Scale bar = 5 µm. Pretreatment of HBMECs with the inhibitors specific for Erk1/2-U0126 20 µM,JNK-SP600125 20 µM ( C ) and p38-SB203580 20 µM ( D ) but not Akt-LY294002 10 µM ( C ) pathways abrogates morphine-mediated induction of Egr-1. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group; #p<0.05, ###p<0.001 vs morphine group.

    Article Snippet: Pharmacological blockade (cell signaling) and loss-of-function (Egr-1) approaches demonstrated the role of mitogen-activated protein kinases (MAPKs), PI3K/Akt and the downstream transcription factor Egr-1 respectively, in morphine-mediated induction of PDGF-BB.

    Techniques: Activation Assay, Expressing, Staining

    ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.

    Journal: PLoS ONE

    Article Title: Morphine Induces Expression of Platelet-Derived Growth Factor in Human Brain Microvascular Endothelial Cells: Implication for Vascular Permeability

    doi: 10.1371/journal.pone.0021707

    Figure Lengend Snippet: ( A ) Whole cell lysates of HBMECs transfected with either the wild type (WT) or dominant negative (DN) construct of Egr-1 were subject to western blot analysis using antibodies specific for PDGF-BB. Transfection of cells with the DN-Egr-1, but not the WT-Egr-1 inhibited morphine-mediated induction of PDGF-BB expression. ( B ) Schematic illustration of Egr-1 binding consensus sequence on the PDGF-B promoter region. ( C ) ChIP assay demonstrating morphine-mediated binding of Egr-1 to the PDGF-B promoter. All the data are presented as mean±SD of three individual experiments. ***p<0.001 vs control group.

    Article Snippet: Pharmacological blockade (cell signaling) and loss-of-function (Egr-1) approaches demonstrated the role of mitogen-activated protein kinases (MAPKs), PI3K/Akt and the downstream transcription factor Egr-1 respectively, in morphine-mediated induction of PDGF-BB.

    Techniques: Transfection, Dominant Negative Mutation, Construct, Western Blot, Expressing, Binding Assay, Sequencing

    Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Luciferase activity in adult Egr-1-luc mice . Transgenic Egr-1-luc mice (4 month old, male or female) were anaesthetized with isofluorane in oxygen and received 6 mg luciferin in 100 μl PBS by i.p. injection. Ten minutes after injection BLI measurement was carried out (1 min signal collection, setting 'high resolution'). A representative animal is shown. The reflected light picture is overlaid by a a liacolor coded BLI image visualized in 'blend mode', which allows allocating the BLI signal to the respective areas shown in the underlying reflected light picture.

    Article Snippet: Slides were incubated over night at 4°C with an anti-luciferase goat polyclonal horseradish peroxidase (HRP) conjugated antibody (Abcam, 1:50 in Tris-buffered saline (TBS)/0.3% BSA (TBS-B)) and an Egr-1 rabbit monoclonal antibody (clone: 15F7, # 4153, Cell Signaling, dilution 1:50 in TBS-B), respectively.

    Techniques: Luciferase, Activity Assay, Transgenic Assay, Injection

    Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Egr-1 promoter driven luciferase activity during postnatal development (day 7 - 21 after birth) . Luciferase activity in Egr-1-luc mice at indicated age was measured by BLI after i.p. injection of luciferin. The luciferase signal was collected for 10 sec from the ventral side of the mice (n = 6). A : A reflected light picture of representative animals at indicated age is overlaid by a color coded BLI image. B and C : Luciferase activity was quantified within regions of interest (ROIs) placed at the paw ( B ) or snout area ( C ) and expressed as photons per second per cm 2 to correct for size differences in ROI size at different ages. A background ROI of similar size was subtracted. Median values of six animals + standard deviation are shown. * p < 0.05, *** p < 0.001; indicated day vs. day 7, Wilcoxon test

    Article Snippet: Slides were incubated over night at 4°C with an anti-luciferase goat polyclonal horseradish peroxidase (HRP) conjugated antibody (Abcam, 1:50 in Tris-buffered saline (TBS)/0.3% BSA (TBS-B)) and an Egr-1 rabbit monoclonal antibody (clone: 15F7, # 4153, Cell Signaling, dilution 1:50 in TBS-B), respectively.

    Techniques: Luciferase, Activity Assay, Injection, Standard Deviation

    Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Immunohistochemical analyses of luciferase and Egr-1 expression during embryonic development . Egr-1-luc ( A , B , C and G ) and wildtype ( D , E and F ) C57BL/6 embryos on day E14 of development were stained for luciferase protein ( A-F ) or Egr-1 protein ( G ). In bone primordia of hindlimbs ( A ), sympathetic paravertebral ganglia ( B ) and masticatory apparatus ( C ) luciferase positive areas (arrows) are stained in lilac in transgenic embryos, in wildtype embryos no luciferase signal was detected ( D-F ). When staining for Egr-1 protein, a similar pattern of protein expression was found - exemplarily shown for the masticatory apparatus ( G ) - as for luciferase ( C ); scale bar: 50 μm

    Article Snippet: Slides were incubated over night at 4°C with an anti-luciferase goat polyclonal horseradish peroxidase (HRP) conjugated antibody (Abcam, 1:50 in Tris-buffered saline (TBS)/0.3% BSA (TBS-B)) and an Egr-1 rabbit monoclonal antibody (clone: 15F7, # 4153, Cell Signaling, dilution 1:50 in TBS-B), respectively.

    Techniques: Immunohistochemical staining, Luciferase, Expressing, Staining, Transgenic Assay

    Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Egr-1 promoter driven luciferase activity after partial liver hepatectomy . A : BLI of sham operated (left) or hepatectomized (right) Egr-1-luc mice at 48 h (top row) and 72 h (bottom row) after surgery. Representative animals from n = 3-6 are shown. Red arrows denote the site of initial surgery, arrowhead points at the edge of a liver lobe showing luciferase activity. B : Quantitative luciferase signals from ROIs placed over the liver area of sham operated or hepatectomized mice 48 h or 72 h after surgery. A representative background ROI of comparable size was subtracted to account for background activity. n = 3-6; mean values of six animals + standard deviation are shown. *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Article Snippet: Slides were incubated over night at 4°C with an anti-luciferase goat polyclonal horseradish peroxidase (HRP) conjugated antibody (Abcam, 1:50 in Tris-buffered saline (TBS)/0.3% BSA (TBS-B)) and an Egr-1 rabbit monoclonal antibody (clone: 15F7, # 4153, Cell Signaling, dilution 1:50 in TBS-B), respectively.

    Techniques: Luciferase, Activity Assay, Standard Deviation, MANN-WHITNEY

    Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: Immunohistochemical analyses of Egr-1 driven luciferase expression in regenerating liver . Egr-1-luc mice 4-8 weeks of age were subjected to one third liver hepatectomy as described in "Methods". Forty-eight hours after surgery mice were sacrificed, liver tissue fixed in PFA and stained for luciferase (luc). Tissue next to the site of surgery (rim upper left corner in both images) is shown and cells staining positive for luciferase ( A ) as well as Egr-1 ( B ) appear as clusters with brown-reddish staining (arrows; scale bar: 50 μm)

    Article Snippet: Slides were incubated over night at 4°C with an anti-luciferase goat polyclonal horseradish peroxidase (HRP) conjugated antibody (Abcam, 1:50 in Tris-buffered saline (TBS)/0.3% BSA (TBS-B)) and an Egr-1 rabbit monoclonal antibody (clone: 15F7, # 4153, Cell Signaling, dilution 1:50 in TBS-B), respectively.

    Techniques: Immunohistochemical staining, Luciferase, Expressing, Staining

    mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: mRNA and protein levels of Egr-1 and luciferase after partial hepatectomy . Egr-1-luc mice were subjected to one third hepatectomy or sham operation, sacrificed 12 h ( A ) or 48 h ( B ) after surgery and liver tissue subjected to mRNA analyses by qRT-PCR ( A ) or Western blot analyzing protein levels of Egr-1 and luciferase ( B ). A : mRNA levels of Egr-1 and luciferase, respectively (average relative mRNA levels relative to 18S rRNA levels); mRNA levels of luciferase in sham operated animals were below the detection limit. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney). B : Representative Western blots showing the protein levels of Egr-1, luciferase and β-actin for sham operated (left panel) or hepatectomized animals (right panel), respectively; data from two representative animals per treatment are shown. Numbers indicate relative luciferase and Egr-1 expression calculated from optical densities (OD) of luciferase, Egr-1 and ß-actin protein bands. n = 4, mean values + standard deviation are shown; *p < 0.05 sham vs. hepatectomy (U-test, Mann-Whitney).

    Article Snippet: Slides were incubated over night at 4°C with an anti-luciferase goat polyclonal horseradish peroxidase (HRP) conjugated antibody (Abcam, 1:50 in Tris-buffered saline (TBS)/0.3% BSA (TBS-B)) and an Egr-1 rabbit monoclonal antibody (clone: 15F7, # 4153, Cell Signaling, dilution 1:50 in TBS-B), respectively.

    Techniques: Luciferase, Quantitative RT-PCR, Western Blot, Standard Deviation, MANN-WHITNEY, Expressing

    In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).

    Journal: BMC Developmental Biology

    Article Title: Live in vivo imaging of Egr-1 promoter activity during neonatal development, liver regeneration and wound healing

    doi: 10.1186/1471-213X-11-28

    Figure Lengend Snippet: In vivo bioluminescence imaging of the ear wound . In Egr-1-luc mice between the ages of 4-8 weeks an ear wound was inflicted in one ear. Twenty-four hours after infliction animals were subjected to BLI. Luciferase signal was collected for 2 min from the wounded or the control ear, respectively. A : Color coded BLI image overlaid onto a reflected light image from the control ear (left) or wounded ear (right) immediately (top row) or 24 h (bottom row) after wound infliction. B : Quantitative luciferase signals from ROIs placed over the wound site or a similar sized ROI at the control ear. n = 3, mean values + standard deviation are shown; *p < 0.05 control vs. wound (U-test, Mann-Whitney).

    Article Snippet: Slides were incubated over night at 4°C with an anti-luciferase goat polyclonal horseradish peroxidase (HRP) conjugated antibody (Abcam, 1:50 in Tris-buffered saline (TBS)/0.3% BSA (TBS-B)) and an Egr-1 rabbit monoclonal antibody (clone: 15F7, # 4153, Cell Signaling, dilution 1:50 in TBS-B), respectively.

    Techniques: In Vivo, Imaging, Luciferase, Standard Deviation, MANN-WHITNEY

    Protocols of experimental grouping and reagent administering. (a) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-containing-H/R injury. (b) Protocol used to investigate role of PKC α /ERK1/2/Egr-1 in extracellular-calcium-containing-H/R injury. (c) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-free-H/R injury. (d) Protocol used to investigate role of cAMP/PKA in extracellular-calcium-free-H/R injury. CaCon, calcium-containing normoxia; CaH/R, calcium-containing H/R; 0CaCon, calcium-free normoxic control; 0CaH/R, calcium-free H/R.

    Journal: Oxidative Medicine and Cellular Longevity

    Article Title: N -n-Butyl Haloperidol Iodide Ameliorates Cardiomyocytes Hypoxia/Reoxygenation Injury by Extracellular Calcium-Dependent and -Independent Mechanisms

    doi: 10.1155/2013/912310

    Figure Lengend Snippet: Protocols of experimental grouping and reagent administering. (a) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-containing-H/R injury. (b) Protocol used to investigate role of PKC α /ERK1/2/Egr-1 in extracellular-calcium-containing-H/R injury. (c) Protocol used to investigate role of ERK1/2 and Egr-1 in extracellular-calcium-free-H/R injury. (d) Protocol used to investigate role of cAMP/PKA in extracellular-calcium-free-H/R injury. CaCon, calcium-containing normoxia; CaH/R, calcium-containing H/R; 0CaCon, calcium-free normoxic control; 0CaH/R, calcium-free H/R.

    Article Snippet: Anti-p-PKC α , anti-total PKC α , anti-PKA, and chemiluminescence luminol reagents were purchased from Santa Cruz Biotechnology (U.S.); anti-p-ERK1/2, anti-total ERK1/2, and anti-Egr-1 were purchased from Cell Signaling Technology (U.S.); anti- β -actin and horseradish peroxidase-conjugated secondary antibodies were purchased from Wuhan Boster Biotechnology Limited Company (China); all the other chemicals and reagents were purchased from local agencies.

    Techniques:

    Effects of F 2 , Verapamil, and ERK1/2 inhibitors and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-ERK1/2 and total ERK1/2; (b) Egr-1 protein. Quantitative densitometric data were expressed as percentages of the level observed in the CaCon group. All values are expressed as mean ± SEM of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.

    Journal: Oxidative Medicine and Cellular Longevity

    Article Title: N -n-Butyl Haloperidol Iodide Ameliorates Cardiomyocytes Hypoxia/Reoxygenation Injury by Extracellular Calcium-Dependent and -Independent Mechanisms

    doi: 10.1155/2013/912310

    Figure Lengend Snippet: Effects of F 2 , Verapamil, and ERK1/2 inhibitors and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-ERK1/2 and total ERK1/2; (b) Egr-1 protein. Quantitative densitometric data were expressed as percentages of the level observed in the CaCon group. All values are expressed as mean ± SEM of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.

    Article Snippet: Anti-p-PKC α , anti-total PKC α , anti-PKA, and chemiluminescence luminol reagents were purchased from Santa Cruz Biotechnology (U.S.); anti-p-ERK1/2, anti-total ERK1/2, and anti-Egr-1 were purchased from Cell Signaling Technology (U.S.); anti- β -actin and horseradish peroxidase-conjugated secondary antibodies were purchased from Wuhan Boster Biotechnology Limited Company (China); all the other chemicals and reagents were purchased from local agencies.

    Techniques: Expressing, Western Blot

    Effects of F 2 , Verapamil, and PKC α inhibitor and activator on p-PKC α , total PKC α , p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-PKC α and total PKC α protein levels; (b) p-ERK1/2 and total ERK1/2 protein levels; (c) Egr-1 protein levels. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.

    Journal: Oxidative Medicine and Cellular Longevity

    Article Title: N -n-Butyl Haloperidol Iodide Ameliorates Cardiomyocytes Hypoxia/Reoxygenation Injury by Extracellular Calcium-Dependent and -Independent Mechanisms

    doi: 10.1155/2013/912310

    Figure Lengend Snippet: Effects of F 2 , Verapamil, and PKC α inhibitor and activator on p-PKC α , total PKC α , p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-containing myocardial H/R by western-blot assay. (a) p-PKC α and total PKC α protein levels; (b) p-ERK1/2 and total ERK1/2 protein levels; (c) Egr-1 protein levels. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus CaCon group; # P < 0.05 versus CaH/R group; † P < 0.05 versus CaH/R+F 2 group.

    Article Snippet: Anti-p-PKC α , anti-total PKC α , anti-PKA, and chemiluminescence luminol reagents were purchased from Santa Cruz Biotechnology (U.S.); anti-p-ERK1/2, anti-total ERK1/2, and anti-Egr-1 were purchased from Cell Signaling Technology (U.S.); anti- β -actin and horseradish peroxidase-conjugated secondary antibodies were purchased from Wuhan Boster Biotechnology Limited Company (China); all the other chemicals and reagents were purchased from local agencies.

    Techniques: Expressing, Western Blot

    Effects of F 2 , ERK1/2 inhibitors, and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-free myocardial H/R by western-blot assay. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus 0CaCon group; # P < 0.05 versus 0CaH/R group; † P < 0.05 versus 0CaH/R+F 2 group.

    Journal: Oxidative Medicine and Cellular Longevity

    Article Title: N -n-Butyl Haloperidol Iodide Ameliorates Cardiomyocytes Hypoxia/Reoxygenation Injury by Extracellular Calcium-Dependent and -Independent Mechanisms

    doi: 10.1155/2013/912310

    Figure Lengend Snippet: Effects of F 2 , ERK1/2 inhibitors, and activator on p-ERK1/2, total ERK1/2, and Egr-1 expression in extracellular-calcium-free myocardial H/R by western-blot assay. All values are expressed as mean ± S.E.M. of at least six individual experiments. * P < 0.05 versus 0CaCon group; # P < 0.05 versus 0CaH/R group; † P < 0.05 versus 0CaH/R+F 2 group.

    Article Snippet: Anti-p-PKC α , anti-total PKC α , anti-PKA, and chemiluminescence luminol reagents were purchased from Santa Cruz Biotechnology (U.S.); anti-p-ERK1/2, anti-total ERK1/2, and anti-Egr-1 were purchased from Cell Signaling Technology (U.S.); anti- β -actin and horseradish peroxidase-conjugated secondary antibodies were purchased from Wuhan Boster Biotechnology Limited Company (China); all the other chemicals and reagents were purchased from local agencies.

    Techniques: Expressing, Western Blot

    (A) HMEC-1s and HUVECs were incubated with SW480-derived EVs (1 µg/mL) or untreated control. mRNA was isolated from untreated control cells or cells treated with EVs for 0, 0.5, 1, 2, and 4 h and analyzed using real time RT-PCR (n = 3). Values represent Egr-1 mRNA/GAPDH mRNA normalized to untreated control cells. (B) HMEC-1s were treated with EVs (1 µg/mL) derived from HCT116 colorectal carcinoma, A549 lung adenocarcinoma, HT1080 fibrosarcoma, PC3 prostate carcinoma, SH-SY5Y neuroblastoma, and BEAS-2B normal bronchial epithelial cells for 0.5 h (n = 3). (C, D) In HMEC-1s, nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 0.5, 1, 2, and 4 h was analyzed under confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel C. Scale bars represent 30 µm. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over that of total cells (D). Data are represented as mean ± SD. * P <0.05; ** P <0.01; ** P <0.001; n.s., not significant.

    Journal: PLoS ONE

    Article Title: Egr-1 Activation by Cancer-Derived Extracellular Vesicles Promotes Endothelial Cell Migration via ERK1/2 and JNK Signaling Pathways

    doi: 10.1371/journal.pone.0115170

    Figure Lengend Snippet: (A) HMEC-1s and HUVECs were incubated with SW480-derived EVs (1 µg/mL) or untreated control. mRNA was isolated from untreated control cells or cells treated with EVs for 0, 0.5, 1, 2, and 4 h and analyzed using real time RT-PCR (n = 3). Values represent Egr-1 mRNA/GAPDH mRNA normalized to untreated control cells. (B) HMEC-1s were treated with EVs (1 µg/mL) derived from HCT116 colorectal carcinoma, A549 lung adenocarcinoma, HT1080 fibrosarcoma, PC3 prostate carcinoma, SH-SY5Y neuroblastoma, and BEAS-2B normal bronchial epithelial cells for 0.5 h (n = 3). (C, D) In HMEC-1s, nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 0.5, 1, 2, and 4 h was analyzed under confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel C. Scale bars represent 30 µm. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over that of total cells (D). Data are represented as mean ± SD. * P <0.05; ** P <0.01; ** P <0.001; n.s., not significant.

    Article Snippet: Cells were treated with SW480-derived EVs (1 µg/mL, 0.5 mL), fixed with 4% paraformaldehyde, and incubated with rabbit anti-Egr-1 antibody (Cell Signaling Technology, Hitchin, United Kingdom) followed by AlexaFluor488 goat anti-rabbit IgG antibody (Invitrogen).

    Techniques: Incubation, Derivative Assay, Isolation, Quantitative RT-PCR, Translocation Assay, Confocal Microscopy, Staining, Fluorescence

    (A) HMEC-1s were transfected with 50 nM of scrambled siRNA or Egr-1 siRNA-1, Egr-1 siRNA-2, or Egr-1 siRNA-3. mRNAs were isolated from the cells after 48 h and the level of Egr-1 mRNA was analyzed using real time RT-PCR (n = 3). (B) Nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 1 h was analyzed in scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) transfected HMEC-1s (n = 3). (C, D) Confluent HMEC-1s transfected with scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) were scratched and treated with SW480-derived EVs (1 µg/mL); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). The number of migrated cells in the denuded zone of each group is shown in panel D. Scale bars represent 100 µm. Data are represented as mean ± SD. * P <0.05; ** P <0.01; *** P <0.001; n.s., not significant.

    Journal: PLoS ONE

    Article Title: Egr-1 Activation by Cancer-Derived Extracellular Vesicles Promotes Endothelial Cell Migration via ERK1/2 and JNK Signaling Pathways

    doi: 10.1371/journal.pone.0115170

    Figure Lengend Snippet: (A) HMEC-1s were transfected with 50 nM of scrambled siRNA or Egr-1 siRNA-1, Egr-1 siRNA-2, or Egr-1 siRNA-3. mRNAs were isolated from the cells after 48 h and the level of Egr-1 mRNA was analyzed using real time RT-PCR (n = 3). (B) Nuclear translocation of Egr-1 protein after stimulation with SW480-derived EVs (1 µg/mL) for 1 h was analyzed in scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) transfected HMEC-1s (n = 3). (C, D) Confluent HMEC-1s transfected with scrambled siRNA (50 nM) or Egr-1 siRNA-1 (50 nM) were scratched and treated with SW480-derived EVs (1 µg/mL); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). The number of migrated cells in the denuded zone of each group is shown in panel D. Scale bars represent 100 µm. Data are represented as mean ± SD. * P <0.05; ** P <0.01; *** P <0.001; n.s., not significant.

    Article Snippet: Cells were treated with SW480-derived EVs (1 µg/mL, 0.5 mL), fixed with 4% paraformaldehyde, and incubated with rabbit anti-Egr-1 antibody (Cell Signaling Technology, Hitchin, United Kingdom) followed by AlexaFluor488 goat anti-rabbit IgG antibody (Invitrogen).

    Techniques: Transfection, Isolation, Quantitative RT-PCR, Translocation Assay, Derivative Assay

    (A, B) HMEC-1s were pretreated with signaling inhibitors for 1 h and then stimulated for 1 h with SW480-derived EVs (1 µg/mL). Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel A. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over total cells (B). (C, D) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of signaling inhibitors; then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). Representative photographs of confocal microscopic imaging are shown in panel C and the number of migrated cells in the denuded zone of each group is shown in panel D. ERK1/2 inhibitor, PD98059 (20 µM); p38 MAPK inhibitor, SB203580 (10 µM); JNK inhibitor, SP600125 (20 µM); Akt inhibitor, BML-257 (20 µM). (E, F) C57BL/6 mice were subcutaneously injected with Matrigel containing SW480-derived EVs (20 µg) with PD98059 (20 µM) or SP600125 (20 µM). After 7 days, whole-mount staining of Matrigel with anti-CD31 antibody was conducted (n = 5). Representative confocal Z-stack photographs of whole mounts stained for CD31 (green) are shown in panel E. Fluorescence intensities of CD31 in the Z-stack plane of the Matrigel were measured as described in the (F). Scale bars in panels A, C, and E represent 30, 100, and 100 µm, respectively. Data are represented as mean ± SD. *** P <0.001.

    Journal: PLoS ONE

    Article Title: Egr-1 Activation by Cancer-Derived Extracellular Vesicles Promotes Endothelial Cell Migration via ERK1/2 and JNK Signaling Pathways

    doi: 10.1371/journal.pone.0115170

    Figure Lengend Snippet: (A, B) HMEC-1s were pretreated with signaling inhibitors for 1 h and then stimulated for 1 h with SW480-derived EVs (1 µg/mL). Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy (n = 3). Nuclei and Egr-1 proteins were stained with Hoechst (blue) and anti-Egr-1 antibody (red), respectively. Co-localized fluorescence signals (purple) indicate the translocation of Egr-1 into the nucleus. Representative photographs are shown in panel A. The percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus colocalized signals over total cells (B). (C, D) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of signaling inhibitors; then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). Representative photographs of confocal microscopic imaging are shown in panel C and the number of migrated cells in the denuded zone of each group is shown in panel D. ERK1/2 inhibitor, PD98059 (20 µM); p38 MAPK inhibitor, SB203580 (10 µM); JNK inhibitor, SP600125 (20 µM); Akt inhibitor, BML-257 (20 µM). (E, F) C57BL/6 mice were subcutaneously injected with Matrigel containing SW480-derived EVs (20 µg) with PD98059 (20 µM) or SP600125 (20 µM). After 7 days, whole-mount staining of Matrigel with anti-CD31 antibody was conducted (n = 5). Representative confocal Z-stack photographs of whole mounts stained for CD31 (green) are shown in panel E. Fluorescence intensities of CD31 in the Z-stack plane of the Matrigel were measured as described in the (F). Scale bars in panels A, C, and E represent 30, 100, and 100 µm, respectively. Data are represented as mean ± SD. *** P <0.001.

    Article Snippet: Cells were treated with SW480-derived EVs (1 µg/mL, 0.5 mL), fixed with 4% paraformaldehyde, and incubated with rabbit anti-Egr-1 antibody (Cell Signaling Technology, Hitchin, United Kingdom) followed by AlexaFluor488 goat anti-rabbit IgG antibody (Invitrogen).

    Techniques: Derivative Assay, Translocation Assay, Confocal Microscopy, Staining, Fluorescence, Imaging, Injection

    (A) HMEC-1s were treated with DiI-labeled SW480-derived EVs (1 µg/mL) for 1 h in the presence or absence of MβCD (10 mM) (n = 3). SW480-derived EVs and nuclei were stained with DiI (red) and Hoechst (blue) respectively. Representative photographs are shown in panel A. Scale bars represent 10 µm. (B) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of MβCD (10 mM); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). (C, D) HMEC-1s were pretreated with MβCD (10 mM) for 1 h and then stimulated with SW480-derived EVs (1 µg/mL) for 1 h. Scale bars represent 30 µm. Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy and the percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus co-localized signals over that of total cells (n = 3). Data are represented as mean ± SD. *** P <0.001.

    Journal: PLoS ONE

    Article Title: Egr-1 Activation by Cancer-Derived Extracellular Vesicles Promotes Endothelial Cell Migration via ERK1/2 and JNK Signaling Pathways

    doi: 10.1371/journal.pone.0115170

    Figure Lengend Snippet: (A) HMEC-1s were treated with DiI-labeled SW480-derived EVs (1 µg/mL) for 1 h in the presence or absence of MβCD (10 mM) (n = 3). SW480-derived EVs and nuclei were stained with DiI (red) and Hoechst (blue) respectively. Representative photographs are shown in panel A. Scale bars represent 10 µm. (B) Confluent HMEC-1s were scratched and treated with SW480-derived EVs (1 µg/mL) in the presence or absence of MβCD (10 mM); then the number of migrated cells in the denuded zone was evaluated after 12 h (n = 3). (C, D) HMEC-1s were pretreated with MβCD (10 mM) for 1 h and then stimulated with SW480-derived EVs (1 µg/mL) for 1 h. Scale bars represent 30 µm. Nuclear translocation of Egr-1 protein was analyzed using confocal microscopy and the percentage of Egr-1-positive nuclei was determined by measuring the number of cells with nucleus co-localized signals over that of total cells (n = 3). Data are represented as mean ± SD. *** P <0.001.

    Article Snippet: Cells were treated with SW480-derived EVs (1 µg/mL, 0.5 mL), fixed with 4% paraformaldehyde, and incubated with rabbit anti-Egr-1 antibody (Cell Signaling Technology, Hitchin, United Kingdom) followed by AlexaFluor488 goat anti-rabbit IgG antibody (Invitrogen).

    Techniques: Labeling, Derivative Assay, Staining, Translocation Assay, Confocal Microscopy

    Growth-quiescent SMCs were treated with MMP inhibitor GM6001+ (25 µM) and TAPI-1 (10 µM) for 30 min before stimulation with IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in GM6001+ or GM6001- treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs treated with GM6001+ or GM6001-. ( C ) Egr-1 mRNA levels in TAPI-1 treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( D ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with TAPI-1. DMSO was used as a carrier. ( E ) Western blotting for ADAM17, ADAM10, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ADAM17 siRNA (0.1 µM) and treated with IL-1beta for 30 min.

    Journal: PLoS ONE

    Article Title: IL-1beta Signals through the EGF Receptor and Activates Egr-1 through MMP-ADAM

    doi: 10.1371/journal.pone.0039811

    Figure Lengend Snippet: Growth-quiescent SMCs were treated with MMP inhibitor GM6001+ (25 µM) and TAPI-1 (10 µM) for 30 min before stimulation with IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in GM6001+ or GM6001- treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs treated with GM6001+ or GM6001-. ( C ) Egr-1 mRNA levels in TAPI-1 treated SMCs treated with IL-1beta by qPCR. Data were normalized to beta-actin. ( D ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with TAPI-1. DMSO was used as a carrier. ( E ) Western blotting for ADAM17, ADAM10, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ADAM17 siRNA (0.1 µM) and treated with IL-1beta for 30 min.

    Article Snippet: Rabbit monoclonal antibodies Egr-1 were obtained from Cell Signaling (Danvers, MA, USA).

    Techniques: Western Blot, Transfection

    Growth-quiescent SMCs were incubated with EGFR inhibitors AG1478 (5 µM) and PD153035 (5 µM) for 30 min, and exposed to IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in AG1478- and PD153035-treated SMCs incubated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with AG1478 or PD153035. ( C ) Western blotting for EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with EGFR siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( D ) Western blotting for ErbB4, EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ErbB4 siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( E ) Egr-1 mRNA levels in AG825 (10 µM for 30 min)-treated SMCs incubated with IL-1beta for 30 min by qPCR. Data were normalized to beta-actin. ( F ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs pretreated with AG825 (10 µM for 30 min) then stimulated with IL-1beta for another 30 min.

    Journal: PLoS ONE

    Article Title: IL-1beta Signals through the EGF Receptor and Activates Egr-1 through MMP-ADAM

    doi: 10.1371/journal.pone.0039811

    Figure Lengend Snippet: Growth-quiescent SMCs were incubated with EGFR inhibitors AG1478 (5 µM) and PD153035 (5 µM) for 30 min, and exposed to IL-1beta (10 ng/ml) for another 30 min (unless indicated otherwise). ( A ) Egr-1 mRNA levels in AG1478- and PD153035-treated SMCs incubated with IL-1beta by qPCR. Data were normalized to beta-actin. ( B ) Western blotting for Egr-1 or beta-actin of total extracts of SMCs treated with AG1478 or PD153035. ( C ) Western blotting for EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with EGFR siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( D ) Western blotting for ErbB4, EGFR, Egr-1 or beta-actin of total extracts of SMCs transfected overnight with ErbB4 siRNA (0.1 µM) and treated with IL-1beta for 30 min. ( E ) Egr-1 mRNA levels in AG825 (10 µM for 30 min)-treated SMCs incubated with IL-1beta for 30 min by qPCR. Data were normalized to beta-actin. ( F ) Western blotting for Egr-1 or beta-actin in total extracts of SMCs pretreated with AG825 (10 µM for 30 min) then stimulated with IL-1beta for another 30 min.

    Article Snippet: Rabbit monoclonal antibodies Egr-1 were obtained from Cell Signaling (Danvers, MA, USA).

    Techniques: Incubation, Western Blot, Transfection

    ( A ) Growth-quiescent SMCs were stimulated with IL-1beta (10 ng/ml) for the indicated times. Total protein extracts were resolved by SDS-PAGE and subjected to Western blot analysis using antibodies for Egr-1, EGFR phospho-Tyr 845 , total EGFR and beta-actin. Alternatively, Western blotting for EGFR phospho-Tyr 845 or EGFR of total extracts of SMCs treated with ( B ) AG1478 (5 µM), ( C ) GM6001+ or GM6001- (25 µM) ( D ) TAPI-1 (10 µM), PD153035 (5 µM) for 30 min followed by IL-1beta stimulation for 5 min.

    Journal: PLoS ONE

    Article Title: IL-1beta Signals through the EGF Receptor and Activates Egr-1 through MMP-ADAM

    doi: 10.1371/journal.pone.0039811

    Figure Lengend Snippet: ( A ) Growth-quiescent SMCs were stimulated with IL-1beta (10 ng/ml) for the indicated times. Total protein extracts were resolved by SDS-PAGE and subjected to Western blot analysis using antibodies for Egr-1, EGFR phospho-Tyr 845 , total EGFR and beta-actin. Alternatively, Western blotting for EGFR phospho-Tyr 845 or EGFR of total extracts of SMCs treated with ( B ) AG1478 (5 µM), ( C ) GM6001+ or GM6001- (25 µM) ( D ) TAPI-1 (10 µM), PD153035 (5 µM) for 30 min followed by IL-1beta stimulation for 5 min.

    Article Snippet: Rabbit monoclonal antibodies Egr-1 were obtained from Cell Signaling (Danvers, MA, USA).

    Techniques: SDS Page, Western Blot

    ( A ) Western blotting for Egr-1, ADAM17, EGFR, IL-1RI or beta-actin using total extracts of growth-quiescent wild-type or ADAM17-deficient mEFs treated with IL-1beta for 30 or 60 min. ( B ) Interaction of 125 I-IL-1beta with ADAM17WT and ADAM17-deficient cells. Growth-quiescent ADAM17WT and ADAM17−/− mEFs (1.8×10 4 cells/well) were incubated with increasing amounts of 125 I-IL-1beta in 1% BSA/PBS for 1 h at 4°C. The cells were washed and lysed with 1M NaOH prior to assessment of counts in an automated gamma-counter.

    Journal: PLoS ONE

    Article Title: IL-1beta Signals through the EGF Receptor and Activates Egr-1 through MMP-ADAM

    doi: 10.1371/journal.pone.0039811

    Figure Lengend Snippet: ( A ) Western blotting for Egr-1, ADAM17, EGFR, IL-1RI or beta-actin using total extracts of growth-quiescent wild-type or ADAM17-deficient mEFs treated with IL-1beta for 30 or 60 min. ( B ) Interaction of 125 I-IL-1beta with ADAM17WT and ADAM17-deficient cells. Growth-quiescent ADAM17WT and ADAM17−/− mEFs (1.8×10 4 cells/well) were incubated with increasing amounts of 125 I-IL-1beta in 1% BSA/PBS for 1 h at 4°C. The cells were washed and lysed with 1M NaOH prior to assessment of counts in an automated gamma-counter.

    Article Snippet: Rabbit monoclonal antibodies Egr-1 were obtained from Cell Signaling (Danvers, MA, USA).

    Techniques: Western Blot, Incubation

    EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.

    Journal: Theranostics

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    doi: 10.7150/thno.40664

    Figure Lengend Snippet: EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.

    Article Snippet: EGR-1 antibody (#4154S; Cell signaling) was used to immunoprecipitate the EGR-1 protein and DNA complexes.

    Techniques: Immunofluorescence, Staining, Isolation, Western Blot

    Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.

    Journal: Theranostics

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    doi: 10.7150/thno.40664

    Figure Lengend Snippet: Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.

    Article Snippet: EGR-1 antibody (#4154S; Cell signaling) was used to immunoprecipitate the EGR-1 protein and DNA complexes.

    Techniques: Binding Assay, Expressing, Isolation, Software, Real-time Polymerase Chain Reaction, Amplification

    The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.

    Journal: Theranostics

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    doi: 10.7150/thno.40664

    Figure Lengend Snippet: The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.

    Article Snippet: EGR-1 antibody (#4154S; Cell signaling) was used to immunoprecipitate the EGR-1 protein and DNA complexes.

    Techniques: Expressing

    EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.

    Journal: Theranostics

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    doi: 10.7150/thno.40664

    Figure Lengend Snippet: EGR-1 deficiency exhibits reduced proliferation and neogenesis in the islet upon HF feeding. A : Immunofluorescence staining for Ki67 ( green ) and B : quantification of Ki67 + cells in the pancreas of 5-month-old male WT ( n =4) and Egr1 -/- ( n =4) mice fed a HF diet for 3 months. Numbers inside bars are accumulated percentages of different categories of Ki67 + cell number per islet. C : Quantification of Ki67-positive insulin-positive cells. Scale bar: 50 μm. D : Immunofluorescence staining for cleaved caspase-3 ( green ) in the pancreatic islets. Images are co-stained for insulin ( red ) and nuclei ( blue ). Scale bar: 200 μm. E : Quantification of caspases-3-positive insulin-positive cells. F : mRNA levels of proliferation markers in the isolated islets of HF-fed Egr1 -/- ( n =10) mice relative to WT ( n =6) mice. G : Immunoblot analysis on proliferation-related markers and signaling molecules. The relative intensities of the bands by densitometric quantification to WT are indicated. * P <0.05 and *** P <0.001.

    Article Snippet: EGR-1 antibody (#4154S; Cell signaling) was used to immunoprecipitate the EGR-1 protein and DNA complexes.

    Techniques: Immunofluorescence, Staining, Isolation, Western Blot

    Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.

    Journal: Theranostics

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    doi: 10.7150/thno.40664

    Figure Lengend Snippet: Decreased transcriptional network in the islets of HF-fed Egr1 -/- mice. A : Bioinformatics analysis in identification of transcriptional factors and endocrine molecules that contain potential EGR-1 binding site. Sequences for proteins involved in the development program of islet lineages were analyzed for potential EGR-1 binding site using the PROMO transcription factor binding site database. B : Expression of genes for pancreatic development, endocrine lineage specification and β-cell identity in the isolated islets of HF-fed Egr1 -/- ( n =10) relative to WT ( n =6) mice. * P <0.05 and ** P <0.01 compared to WT mice. Pathway analysis of the response of HF feeding on the islets of ( C ) WT and ( D ) Egr1 -/- mice using Ingenuity Pathways Analysis (IPA) software. Pathway analysis of the effect of EGR-1 deficiency on the transcription network in ( E ) RC and ( F ) HF diet feeding. Color shading corresponds to the type of dysregulation: red for up-regulated and green for down-regulated genes according to the results of quantitative PCR. The shape of the node indicates the major function of the protein: transcription regulators (dumbbell); kinases (three arrows); and others (circle). G : Expression of genes in EGR-1 knockdowned ( n =5) relative to control ( n =5) MIN6 cells. H : ChIP assay in EGR-1 overexpressed and control (pCMV) MIN6 cells. Sequences containing the potential EGR-1 binding sites in Pdx1 and Arx were amplified by real-time PCR. n =3 in each group. * P <0.05, ** P <0.01, and *** P <0.001.

    Article Snippet: EGR-1 antibody (#4154S; Cell signaling) was used to immunoprecipitate the EGR-1 protein and DNA complexes.

    Techniques: Binding Assay, Expressing, Isolation, Software, Real-time Polymerase Chain Reaction, Amplification

    The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.

    Journal: Theranostics

    Article Title: Loss of EGR-1 uncouples compensatory responses of pancreatic β cells

    doi: 10.7150/thno.40664

    Figure Lengend Snippet: The correlation between EGR-1 expression and compensatory genes in human pancreatic tissues. Scatter plot illustrating the Spearman's correlation of normalized reads per patient between EGR1 and PDX1 , as well as compensatory genes, such as CCND1 (cyclin D1), INS (insulin), and GCK (glucokinase), in ( A ) non-diabetic (upper panels) and diabetic (lower panels) subjects; and ( B ) normal weight (BMI < 23, upper panels) and overweight/obese (BMI ≥ 23, lower panels) subjects. Spearman's rank correlation coefficients r and P value are provided in each plot. * P <0.05, ** P <0.01, and *** P <0.001.

    Article Snippet: EGR-1 antibody (#4154S; Cell signaling) was used to immunoprecipitate the EGR-1 protein and DNA complexes.

    Techniques: Expressing