h2bub1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc h2bub1
    a , Schematic of the knockin strategy for BRD4-dTAG. b , Agarose gel electrophoretic analysis of PCR products from MCF7 parental cells and MCF7 BRD4-dTAG knockin cells. c , Immunoblot for BRD4 expression in BRD4-dTAG cells treated with dTAG-7 or dTAG V -1 at indicated concentrations for indicated times. dBET6 was added for 2 hours to show changes in Pol II CTD Ser2-P. d , Immunoblot showing effects of different 2-hour treatments on Pol II and <t>H2Bub1</t> in BRD4-dTAG cells. e , Percentage of MCF7 BRD4-dTAG cell survival after treatment with or without BET inhibitors and dTAG-7 (250 nM) for 6 days. Data shown as mean ± s.d. from biological triplicates. f , Immunoblot showing reduced ER expression in BRD4-dTAG cells upon overnight treatment with JQ1 and dTAG-7. g,h, qPCR of MYC, Cyclin D1 ( h ) and ESR1-Y537 g, mRNA levels in MCF7 BRD4-dTAG ESR1-Y537S cells upon overnight treatment with BET inhibitors and dTAG-7 (500 nM). Because ESR1-Y537S-IRES-GFP is transcribed as a single transcript, ESR1 -Y537S RNA level was monitored by GFP RNA. All cells were grown in normal full medium containing 10% FBS. Data shown as mean ± s.d. from independent triplicates. p values from two-tailed t-tests are depicted with asterisks.
    H2bub1, 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 "Resistance of estrogen receptor function to BET bromodomain inhibition is mediated by transcriptional coactivator cooperativity"

    Article Title: Resistance of estrogen receptor function to BET bromodomain inhibition is mediated by transcriptional coactivator cooperativity

    Journal: bioRxiv

    doi: 10.1101/2024.07.25.605008

    a , Schematic of the knockin strategy for BRD4-dTAG. b , Agarose gel electrophoretic analysis of PCR products from MCF7 parental cells and MCF7 BRD4-dTAG knockin cells. c , Immunoblot for BRD4 expression in BRD4-dTAG cells treated with dTAG-7 or dTAG V -1 at indicated concentrations for indicated times. dBET6 was added for 2 hours to show changes in Pol II CTD Ser2-P. d , Immunoblot showing effects of different 2-hour treatments on Pol II and H2Bub1 in BRD4-dTAG cells. e , Percentage of MCF7 BRD4-dTAG cell survival after treatment with or without BET inhibitors and dTAG-7 (250 nM) for 6 days. Data shown as mean ± s.d. from biological triplicates. f , Immunoblot showing reduced ER expression in BRD4-dTAG cells upon overnight treatment with JQ1 and dTAG-7. g,h, qPCR of MYC, Cyclin D1 ( h ) and ESR1-Y537 g, mRNA levels in MCF7 BRD4-dTAG ESR1-Y537S cells upon overnight treatment with BET inhibitors and dTAG-7 (500 nM). Because ESR1-Y537S-IRES-GFP is transcribed as a single transcript, ESR1 -Y537S RNA level was monitored by GFP RNA. All cells were grown in normal full medium containing 10% FBS. Data shown as mean ± s.d. from independent triplicates. p values from two-tailed t-tests are depicted with asterisks.
    Figure Legend Snippet: a , Schematic of the knockin strategy for BRD4-dTAG. b , Agarose gel electrophoretic analysis of PCR products from MCF7 parental cells and MCF7 BRD4-dTAG knockin cells. c , Immunoblot for BRD4 expression in BRD4-dTAG cells treated with dTAG-7 or dTAG V -1 at indicated concentrations for indicated times. dBET6 was added for 2 hours to show changes in Pol II CTD Ser2-P. d , Immunoblot showing effects of different 2-hour treatments on Pol II and H2Bub1 in BRD4-dTAG cells. e , Percentage of MCF7 BRD4-dTAG cell survival after treatment with or without BET inhibitors and dTAG-7 (250 nM) for 6 days. Data shown as mean ± s.d. from biological triplicates. f , Immunoblot showing reduced ER expression in BRD4-dTAG cells upon overnight treatment with JQ1 and dTAG-7. g,h, qPCR of MYC, Cyclin D1 ( h ) and ESR1-Y537 g, mRNA levels in MCF7 BRD4-dTAG ESR1-Y537S cells upon overnight treatment with BET inhibitors and dTAG-7 (500 nM). Because ESR1-Y537S-IRES-GFP is transcribed as a single transcript, ESR1 -Y537S RNA level was monitored by GFP RNA. All cells were grown in normal full medium containing 10% FBS. Data shown as mean ± s.d. from independent triplicates. p values from two-tailed t-tests are depicted with asterisks.

    Techniques Used: Knock-In, Agarose Gel Electrophoresis, Western Blot, Expressing, Two Tailed Test

    anti h2bub1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc anti h2bub1
    (A) and (B) Loss of RAF24 increases <t>H2Bub1</t> levels. Immunoblotting analysis of 10d-old WT and raf24-2 plants constitutively over-expressing TAP-HUB2. 50 μg of protein samples were loaded in each lane. Biological replicates (n=3) were examined and quantified with ImageJ software, with levels of H2Bub1 normalized to H2B levels. (C) and (D) Over-expression of TAP-HUB2 in raf24-2 also leads to an early flowering phenotype. Two independent lines of 29d-old WT and raf24-2 plants (denoted by the number) constitutively expressing TAP-HUB2 were grown and imaged (C), with flowering time determined by days to bolting (upper) and rosette number at bolting (bottom) (D). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05 ).
    Anti H2bub1, 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 "B4 Raf-like MAPKKK RAF24 regulates Arabidopsis thaliana flowering time through HISTONE MONO-UBIQUITINATION 2"

    Article Title: B4 Raf-like MAPKKK RAF24 regulates Arabidopsis thaliana flowering time through HISTONE MONO-UBIQUITINATION 2

    Journal: bioRxiv

    doi: 10.1101/2024.06.12.598286

    (A) and (B) Loss of RAF24 increases H2Bub1 levels. Immunoblotting analysis of 10d-old WT and raf24-2 plants constitutively over-expressing TAP-HUB2. 50 μg of protein samples were loaded in each lane. Biological replicates (n=3) were examined and quantified with ImageJ software, with levels of H2Bub1 normalized to H2B levels. (C) and (D) Over-expression of TAP-HUB2 in raf24-2 also leads to an early flowering phenotype. Two independent lines of 29d-old WT and raf24-2 plants (denoted by the number) constitutively expressing TAP-HUB2 were grown and imaged (C), with flowering time determined by days to bolting (upper) and rosette number at bolting (bottom) (D). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05 ).
    Figure Legend Snippet: (A) and (B) Loss of RAF24 increases H2Bub1 levels. Immunoblotting analysis of 10d-old WT and raf24-2 plants constitutively over-expressing TAP-HUB2. 50 μg of protein samples were loaded in each lane. Biological replicates (n=3) were examined and quantified with ImageJ software, with levels of H2Bub1 normalized to H2B levels. (C) and (D) Over-expression of TAP-HUB2 in raf24-2 also leads to an early flowering phenotype. Two independent lines of 29d-old WT and raf24-2 plants (denoted by the number) constitutively expressing TAP-HUB2 were grown and imaged (C), with flowering time determined by days to bolting (upper) and rosette number at bolting (bottom) (D). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05 ).

    Techniques Used: Western Blot, Expressing, Software, Over Expression

    (A) and (B) Comparison of flowering time in raf4-2 plants constitutively over-expressing HA-HUB2 with no (S314S), phospho-ablative (S314A) and phospho-mimetic (S314D) mutations (A). Flowering time was determined by days to bolting and rosette number at bolting (B). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05). (C) Immunoblot analysis of raf24-2 plants constitutively over-expressing phospho-ablative (HA-HUB2 S314A ), phospho-mimetic (HA-HUB2 S314D ), which finds HA-HUB2 S314D maintains lower H2Bub1 levels. 50 μg of protein samples were loaded in each lane. Equal amounts of HA-HUB over-expression in the raf24-2 background was observed across the lines depicted here (Supplemental Figure 7).
    Figure Legend Snippet: (A) and (B) Comparison of flowering time in raf4-2 plants constitutively over-expressing HA-HUB2 with no (S314S), phospho-ablative (S314A) and phospho-mimetic (S314D) mutations (A). Flowering time was determined by days to bolting and rosette number at bolting (B). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05). (C) Immunoblot analysis of raf24-2 plants constitutively over-expressing phospho-ablative (HA-HUB2 S314A ), phospho-mimetic (HA-HUB2 S314D ), which finds HA-HUB2 S314D maintains lower H2Bub1 levels. 50 μg of protein samples were loaded in each lane. Equal amounts of HA-HUB over-expression in the raf24-2 background was observed across the lines depicted here (Supplemental Figure 7).

    Techniques Used: Comparison, Expressing, Western Blot, Over Expression

    (A) In WT, the presence of RAF24 phosphorylates SnRK2s to induce phosphorylation of HUB2, ensuring appropriately tuned HUB2-ligase activity. This in turn optimizes HUB2ub1 levels to maintain proper transcriptional activation of FLC expression and flowering time . Upon the loss of RAF24, SnRK2 fails to phosphorylate HUB2, causing an over-accumulation of H2Bub1 and reduced transcriptional activation of FLC expression. This results in earlier flowering (B) Both the phosphoproteomic and HUB2-TAP pulldowns find that RAF24 acts upstream of a wide variety of floral regulators, including BES1 and FBH3 as well as HUB2 to fine-tune flower time. Identification of both known HUB2 interactors (with straight line) and new, candidate HUB2 interactors (with a dash line) related to flowering time indicates that RAF24 possesses versatile functions / mechanisms in controlling flowering time.
    Figure Legend Snippet: (A) In WT, the presence of RAF24 phosphorylates SnRK2s to induce phosphorylation of HUB2, ensuring appropriately tuned HUB2-ligase activity. This in turn optimizes HUB2ub1 levels to maintain proper transcriptional activation of FLC expression and flowering time . Upon the loss of RAF24, SnRK2 fails to phosphorylate HUB2, causing an over-accumulation of H2Bub1 and reduced transcriptional activation of FLC expression. This results in earlier flowering (B) Both the phosphoproteomic and HUB2-TAP pulldowns find that RAF24 acts upstream of a wide variety of floral regulators, including BES1 and FBH3 as well as HUB2 to fine-tune flower time. Identification of both known HUB2 interactors (with straight line) and new, candidate HUB2 interactors (with a dash line) related to flowering time indicates that RAF24 possesses versatile functions / mechanisms in controlling flowering time.

    Techniques Used: Activity Assay, Activation Assay, Expressing

    anti h2bub1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc anti h2bub1
    Anti H2bub1, 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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    anti h2bub1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc anti h2bub1
    Anti H2bub1, 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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    Millipore anti h2bub1 antibody
    Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of <t>H2Bub1</t> (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates
    Anti H2bub1 Antibody, supplied by Millipore, 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 "USP22 supports the aggressive behavior of basal-like breast cancer by stimulating cellular respiration"

    Article Title: USP22 supports the aggressive behavior of basal-like breast cancer by stimulating cellular respiration

    Journal: Cell Communication and Signaling : CCS

    doi: 10.1186/s12964-023-01441-5

    Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of H2Bub1 (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates
    Figure Legend Snippet: Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of H2Bub1 (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates

    Techniques Used: Staining, Ex Vivo, Cell Culture, Tube Formation Assay, Immunohistochemistry, Western Blot, Colony Assay, High Throughput Screening Assay, RNA Sequencing Assay


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    MediMabs Inc lg anti h2bub1
    Lg Anti H2bub1, supplied by MediMabs 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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    anti h2bub1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc anti h2bub1
    ( A ) NCOA4 interacts with RNF20 as determined by Coomassie bright blue staining. IgG, immunoglobulin G; IP, immunoprecipitation; WCL, whole-cell lysate. ( B ) Interaction between endogenous NCOA4 and RNF20 in C2C12 cells was confirmed by Co-IP with Western blotting ( n = 9). ( C ) Western blot analysis of RNF20 and <t>H2Bub1</t> expression in C2C12 cells treated with 0, 10, 15, 20, 25, and 30 μM DFO in differentiation medium for 3 days ( n = 9). ( D ) Western blot analysis of RNF20 and H2Bub1 in C2C12 cells treated as indicated in differentiation medium for 3 days ( n = 9). ( E ) Western blot analysis of NCOA4, RNF20, and H2Bub1 in C2C12 cells treated as indicated in differentiation medium for 3 days ( n = 9). The results represent the means ± SD. * P < 0.05 and ** P < 0.01.
    Anti H2bub1, 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/anti h2bub1/product/Cell Signaling Technology Inc
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    1) Product Images from "Iron deficiency–induced ferritinophagy impairs skeletal muscle regeneration through RNF20-mediated H2Bub1 modification"

    Article Title: Iron deficiency–induced ferritinophagy impairs skeletal muscle regeneration through RNF20-mediated H2Bub1 modification

    Journal: Science Advances

    doi: 10.1126/sciadv.adf4345

    ( A ) NCOA4 interacts with RNF20 as determined by Coomassie bright blue staining. IgG, immunoglobulin G; IP, immunoprecipitation; WCL, whole-cell lysate. ( B ) Interaction between endogenous NCOA4 and RNF20 in C2C12 cells was confirmed by Co-IP with Western blotting ( n = 9). ( C ) Western blot analysis of RNF20 and H2Bub1 expression in C2C12 cells treated with 0, 10, 15, 20, 25, and 30 μM DFO in differentiation medium for 3 days ( n = 9). ( D ) Western blot analysis of RNF20 and H2Bub1 in C2C12 cells treated as indicated in differentiation medium for 3 days ( n = 9). ( E ) Western blot analysis of NCOA4, RNF20, and H2Bub1 in C2C12 cells treated as indicated in differentiation medium for 3 days ( n = 9). The results represent the means ± SD. * P < 0.05 and ** P < 0.01.
    Figure Legend Snippet: ( A ) NCOA4 interacts with RNF20 as determined by Coomassie bright blue staining. IgG, immunoglobulin G; IP, immunoprecipitation; WCL, whole-cell lysate. ( B ) Interaction between endogenous NCOA4 and RNF20 in C2C12 cells was confirmed by Co-IP with Western blotting ( n = 9). ( C ) Western blot analysis of RNF20 and H2Bub1 expression in C2C12 cells treated with 0, 10, 15, 20, 25, and 30 μM DFO in differentiation medium for 3 days ( n = 9). ( D ) Western blot analysis of RNF20 and H2Bub1 in C2C12 cells treated as indicated in differentiation medium for 3 days ( n = 9). ( E ) Western blot analysis of NCOA4, RNF20, and H2Bub1 in C2C12 cells treated as indicated in differentiation medium for 3 days ( n = 9). The results represent the means ± SD. * P < 0.05 and ** P < 0.01.

    Techniques Used: Staining, Immunoprecipitation, Co-Immunoprecipitation Assay, Western Blot, Expressing

    ( A ) mRNA expression of RNF20 , MyHC , MyoD , and MyoG was measured by qRT-PCR after knockdown of RNF20 by siRNA in C2C12 cells cultured for 3 days in differentiation medium ( n = 9). ( B ) Western blot analysis of RNF20, H2Bub1, MyHC, MyoD, and MyoG protein expression in the RNF20 knockdown or control group of C2C12 cells cultured for 3 days in differentiation medium ( n = 9). ( C ) Immunofluorescence staining for MyHC in the RNF20 knockdown and control group of C2C12 cells cultured for 3 days in differentiation medium ( n = 9). Scale bars, 100 μm. ( D ) mRNA expression of RNF20 , MyHC , MyoD , and MyoG in the RNF20 overexpression group of C2C12 cells treated with or without DFO (20 μM) ( n = 9). ( E ) Western blot analysis of RNF20, H2Bub1, MyHC, MyoD and MyoG expression in the RNF20 overexpression group of C2C12 cells treated with or without DFO (20 μM) ( n = 9). ( F ) Immunofluorescence staining for MyHC in the RNF20 overexpression group of C2C12 cells treated with or without DFO (20 μM) ( n = 9). Scale bars, 100 μm. ( G ) Results of ChIP-qPCR confirmed changes in H2Bub1 modification and binding to the promoter of MyoD and MyoG in control and iron-deficient C2C12 cells treated with or without DC661 following the induction of differentiation for 3 days ( n = 9). ( H ) ChIP-qPCR analysis of changes in H2Bub1 binding to the promoters of MyoD and MyoG in RNF20-overexpressing C2C12 cells under DFO (20 μM), treated or untreated ( n = 9). The results represent the means ± SD. * P < 0.05 and ** P < 0.01. ID, iron-deficient.
    Figure Legend Snippet: ( A ) mRNA expression of RNF20 , MyHC , MyoD , and MyoG was measured by qRT-PCR after knockdown of RNF20 by siRNA in C2C12 cells cultured for 3 days in differentiation medium ( n = 9). ( B ) Western blot analysis of RNF20, H2Bub1, MyHC, MyoD, and MyoG protein expression in the RNF20 knockdown or control group of C2C12 cells cultured for 3 days in differentiation medium ( n = 9). ( C ) Immunofluorescence staining for MyHC in the RNF20 knockdown and control group of C2C12 cells cultured for 3 days in differentiation medium ( n = 9). Scale bars, 100 μm. ( D ) mRNA expression of RNF20 , MyHC , MyoD , and MyoG in the RNF20 overexpression group of C2C12 cells treated with or without DFO (20 μM) ( n = 9). ( E ) Western blot analysis of RNF20, H2Bub1, MyHC, MyoD and MyoG expression in the RNF20 overexpression group of C2C12 cells treated with or without DFO (20 μM) ( n = 9). ( F ) Immunofluorescence staining for MyHC in the RNF20 overexpression group of C2C12 cells treated with or without DFO (20 μM) ( n = 9). Scale bars, 100 μm. ( G ) Results of ChIP-qPCR confirmed changes in H2Bub1 modification and binding to the promoter of MyoD and MyoG in control and iron-deficient C2C12 cells treated with or without DC661 following the induction of differentiation for 3 days ( n = 9). ( H ) ChIP-qPCR analysis of changes in H2Bub1 binding to the promoters of MyoD and MyoG in RNF20-overexpressing C2C12 cells under DFO (20 μM), treated or untreated ( n = 9). The results represent the means ± SD. * P < 0.05 and ** P < 0.01. ID, iron-deficient.

    Techniques Used: Expressing, Quantitative RT-PCR, Cell Culture, Western Blot, Immunofluorescence, Staining, Over Expression, Modification, Binding Assay

    ( A and B ) Immunofluorescence staining for RNF20 and H2Bub1 in different groups of mice. The mean fluorescence intensities of RNF20 and H2Bub1 are shown below ( n = 9). Scale bars, 50 μm. ( C ) Western blot analysis of RNF20 and H2Bub1 expression in different groups of mice ( n = 9). The results represent the means ± SD. ** P < 0.01. ID, iron-deficient.
    Figure Legend Snippet: ( A and B ) Immunofluorescence staining for RNF20 and H2Bub1 in different groups of mice. The mean fluorescence intensities of RNF20 and H2Bub1 are shown below ( n = 9). Scale bars, 50 μm. ( C ) Western blot analysis of RNF20 and H2Bub1 expression in different groups of mice ( n = 9). The results represent the means ± SD. ** P < 0.01. ID, iron-deficient.

    Techniques Used: Immunofluorescence, Staining, Fluorescence, Western Blot, Expressing

    The mice were divided into the following four groups with nine mice per group: NC group (NCOA4 fl/fl ), cKO group (Pax7 CreER , NCOA4 fl/fl ), iron-deficient group (NCOA4 fl/fl ) group, and ID + cKO group (Pax7 CreER , NCOA4 fl/fl ) group. ( A ) Schematic diagram of the procedures for iron deficiency induction, NCOA4 cKO, and CTX-induced muscle injury. ( B ) Schematic diagram of SC isolation. ( C ) Western blot analysis of NCOA4, RNF20, and H2Bub1 protein levels in GA muscle samples from different groups of mice at 7 dpi ( n = 9). ( D ) Representative images of myofibers isolated from the extensor digitorum longus (EDL) muscle of NCOA4 SCs/WT and NCOA4 SCs/KO mice ( n = 9). Immunofluorescence staining of Pax7 (pink), NCOA4 (red), RNF20 (green), and DAPI (blue). Scale bars, 20 μm. ( E ) Representative images of myofibers isolated from the EDL muscle of NCOA4 SCs/WT and NCOA4 SCs/KO mice ( n = 9). Immunofluorescence of Pax7 (pink), NCOA4 (red), H2Bub1 (green), and DAPI (blue) staining. Scale bars, 20 μm. The results represent the means ± SD. * P < 0.05 and ** P < 0.01. ID, iron-deficient.
    Figure Legend Snippet: The mice were divided into the following four groups with nine mice per group: NC group (NCOA4 fl/fl ), cKO group (Pax7 CreER , NCOA4 fl/fl ), iron-deficient group (NCOA4 fl/fl ) group, and ID + cKO group (Pax7 CreER , NCOA4 fl/fl ) group. ( A ) Schematic diagram of the procedures for iron deficiency induction, NCOA4 cKO, and CTX-induced muscle injury. ( B ) Schematic diagram of SC isolation. ( C ) Western blot analysis of NCOA4, RNF20, and H2Bub1 protein levels in GA muscle samples from different groups of mice at 7 dpi ( n = 9). ( D ) Representative images of myofibers isolated from the extensor digitorum longus (EDL) muscle of NCOA4 SCs/WT and NCOA4 SCs/KO mice ( n = 9). Immunofluorescence staining of Pax7 (pink), NCOA4 (red), RNF20 (green), and DAPI (blue). Scale bars, 20 μm. ( E ) Representative images of myofibers isolated from the EDL muscle of NCOA4 SCs/WT and NCOA4 SCs/KO mice ( n = 9). Immunofluorescence of Pax7 (pink), NCOA4 (red), H2Bub1 (green), and DAPI (blue) staining. Scale bars, 20 μm. The results represent the means ± SD. * P < 0.05 and ** P < 0.01. ID, iron-deficient.

    Techniques Used: Isolation, Western Blot, Immunofluorescence, Staining

    h2bub1  (Cell Signaling Technology Inc)


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    Cell Signaling Technology Inc h2bub1
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    Santa Cruz Biotechnology h2bub1
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    Cell Signaling Technology Inc h2bub1
    a , Schematic of the knockin strategy for BRD4-dTAG. b , Agarose gel electrophoretic analysis of PCR products from MCF7 parental cells and MCF7 BRD4-dTAG knockin cells. c , Immunoblot for BRD4 expression in BRD4-dTAG cells treated with dTAG-7 or dTAG V -1 at indicated concentrations for indicated times. dBET6 was added for 2 hours to show changes in Pol II CTD Ser2-P. d , Immunoblot showing effects of different 2-hour treatments on Pol II and <t>H2Bub1</t> in BRD4-dTAG cells. e , Percentage of MCF7 BRD4-dTAG cell survival after treatment with or without BET inhibitors and dTAG-7 (250 nM) for 6 days. Data shown as mean ± s.d. from biological triplicates. f , Immunoblot showing reduced ER expression in BRD4-dTAG cells upon overnight treatment with JQ1 and dTAG-7. g,h, qPCR of MYC, Cyclin D1 ( h ) and ESR1-Y537 g, mRNA levels in MCF7 BRD4-dTAG ESR1-Y537S cells upon overnight treatment with BET inhibitors and dTAG-7 (500 nM). Because ESR1-Y537S-IRES-GFP is transcribed as a single transcript, ESR1 -Y537S RNA level was monitored by GFP RNA. All cells were grown in normal full medium containing 10% FBS. Data shown as mean ± s.d. from independent triplicates. p values from two-tailed t-tests are depicted with asterisks.
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    (A) and (B) Loss of RAF24 increases <t>H2Bub1</t> levels. Immunoblotting analysis of 10d-old WT and raf24-2 plants constitutively over-expressing TAP-HUB2. 50 μg of protein samples were loaded in each lane. Biological replicates (n=3) were examined and quantified with ImageJ software, with levels of H2Bub1 normalized to H2B levels. (C) and (D) Over-expression of TAP-HUB2 in raf24-2 also leads to an early flowering phenotype. Two independent lines of 29d-old WT and raf24-2 plants (denoted by the number) constitutively expressing TAP-HUB2 were grown and imaged (C), with flowering time determined by days to bolting (upper) and rosette number at bolting (bottom) (D). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05 ).
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    Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of <t>H2Bub1</t> (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates
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    Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of <t>H2Bub1</t> (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates
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    Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of <t>H2Bub1</t> (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates
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    Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of <t>H2Bub1</t> (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates
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    a , Schematic of the knockin strategy for BRD4-dTAG. b , Agarose gel electrophoretic analysis of PCR products from MCF7 parental cells and MCF7 BRD4-dTAG knockin cells. c , Immunoblot for BRD4 expression in BRD4-dTAG cells treated with dTAG-7 or dTAG V -1 at indicated concentrations for indicated times. dBET6 was added for 2 hours to show changes in Pol II CTD Ser2-P. d , Immunoblot showing effects of different 2-hour treatments on Pol II and H2Bub1 in BRD4-dTAG cells. e , Percentage of MCF7 BRD4-dTAG cell survival after treatment with or without BET inhibitors and dTAG-7 (250 nM) for 6 days. Data shown as mean ± s.d. from biological triplicates. f , Immunoblot showing reduced ER expression in BRD4-dTAG cells upon overnight treatment with JQ1 and dTAG-7. g,h, qPCR of MYC, Cyclin D1 ( h ) and ESR1-Y537 g, mRNA levels in MCF7 BRD4-dTAG ESR1-Y537S cells upon overnight treatment with BET inhibitors and dTAG-7 (500 nM). Because ESR1-Y537S-IRES-GFP is transcribed as a single transcript, ESR1 -Y537S RNA level was monitored by GFP RNA. All cells were grown in normal full medium containing 10% FBS. Data shown as mean ± s.d. from independent triplicates. p values from two-tailed t-tests are depicted with asterisks.

    Journal: bioRxiv

    Article Title: Resistance of estrogen receptor function to BET bromodomain inhibition is mediated by transcriptional coactivator cooperativity

    doi: 10.1101/2024.07.25.605008

    Figure Lengend Snippet: a , Schematic of the knockin strategy for BRD4-dTAG. b , Agarose gel electrophoretic analysis of PCR products from MCF7 parental cells and MCF7 BRD4-dTAG knockin cells. c , Immunoblot for BRD4 expression in BRD4-dTAG cells treated with dTAG-7 or dTAG V -1 at indicated concentrations for indicated times. dBET6 was added for 2 hours to show changes in Pol II CTD Ser2-P. d , Immunoblot showing effects of different 2-hour treatments on Pol II and H2Bub1 in BRD4-dTAG cells. e , Percentage of MCF7 BRD4-dTAG cell survival after treatment with or without BET inhibitors and dTAG-7 (250 nM) for 6 days. Data shown as mean ± s.d. from biological triplicates. f , Immunoblot showing reduced ER expression in BRD4-dTAG cells upon overnight treatment with JQ1 and dTAG-7. g,h, qPCR of MYC, Cyclin D1 ( h ) and ESR1-Y537 g, mRNA levels in MCF7 BRD4-dTAG ESR1-Y537S cells upon overnight treatment with BET inhibitors and dTAG-7 (500 nM). Because ESR1-Y537S-IRES-GFP is transcribed as a single transcript, ESR1 -Y537S RNA level was monitored by GFP RNA. All cells were grown in normal full medium containing 10% FBS. Data shown as mean ± s.d. from independent triplicates. p values from two-tailed t-tests are depicted with asterisks.

    Article Snippet: ERα (#D8H8, WB), H2Bub1 (#5546), MED26 (#13641), and Rpb1 NTD (#D8L4Y, ChIP) antibodies were from Cell Signaling.

    Techniques: Knock-In, Agarose Gel Electrophoresis, Western Blot, Expressing, Two Tailed Test

    (A) and (B) Loss of RAF24 increases H2Bub1 levels. Immunoblotting analysis of 10d-old WT and raf24-2 plants constitutively over-expressing TAP-HUB2. 50 μg of protein samples were loaded in each lane. Biological replicates (n=3) were examined and quantified with ImageJ software, with levels of H2Bub1 normalized to H2B levels. (C) and (D) Over-expression of TAP-HUB2 in raf24-2 also leads to an early flowering phenotype. Two independent lines of 29d-old WT and raf24-2 plants (denoted by the number) constitutively expressing TAP-HUB2 were grown and imaged (C), with flowering time determined by days to bolting (upper) and rosette number at bolting (bottom) (D). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05 ).

    Journal: bioRxiv

    Article Title: B4 Raf-like MAPKKK RAF24 regulates Arabidopsis thaliana flowering time through HISTONE MONO-UBIQUITINATION 2

    doi: 10.1101/2024.06.12.598286

    Figure Lengend Snippet: (A) and (B) Loss of RAF24 increases H2Bub1 levels. Immunoblotting analysis of 10d-old WT and raf24-2 plants constitutively over-expressing TAP-HUB2. 50 μg of protein samples were loaded in each lane. Biological replicates (n=3) were examined and quantified with ImageJ software, with levels of H2Bub1 normalized to H2B levels. (C) and (D) Over-expression of TAP-HUB2 in raf24-2 also leads to an early flowering phenotype. Two independent lines of 29d-old WT and raf24-2 plants (denoted by the number) constitutively expressing TAP-HUB2 were grown and imaged (C), with flowering time determined by days to bolting (upper) and rosette number at bolting (bottom) (D). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05 ).

    Article Snippet: After blocking 1 hour with 5% (w/v) non-fat milk, PVDF membranes were incubated overnight with anti-H2B (1:2500, abcam, ab1790), anti-H2Bub1 (1:1000, Cell Signaling, #5546), anti-GFP (1:2000, ChromoTek, PABG1), anti-HA(1:1000, Invitrogen, 26183), anti-H3 (1:2000, Invitrogen, PA5-16183) or anti-PAP (1:1000, SIGMA, P1291) followed by a 2-hour incubation with secondary antibodies, anti-rabbit (1:10000, Invitrogen, G-21234) or anti-mouse (1:5000, Invitrogen, G-21040).

    Techniques: Western Blot, Expressing, Software, Over Expression

    (A) and (B) Comparison of flowering time in raf4-2 plants constitutively over-expressing HA-HUB2 with no (S314S), phospho-ablative (S314A) and phospho-mimetic (S314D) mutations (A). Flowering time was determined by days to bolting and rosette number at bolting (B). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05). (C) Immunoblot analysis of raf24-2 plants constitutively over-expressing phospho-ablative (HA-HUB2 S314A ), phospho-mimetic (HA-HUB2 S314D ), which finds HA-HUB2 S314D maintains lower H2Bub1 levels. 50 μg of protein samples were loaded in each lane. Equal amounts of HA-HUB over-expression in the raf24-2 background was observed across the lines depicted here (Supplemental Figure 7).

    Journal: bioRxiv

    Article Title: B4 Raf-like MAPKKK RAF24 regulates Arabidopsis thaliana flowering time through HISTONE MONO-UBIQUITINATION 2

    doi: 10.1101/2024.06.12.598286

    Figure Lengend Snippet: (A) and (B) Comparison of flowering time in raf4-2 plants constitutively over-expressing HA-HUB2 with no (S314S), phospho-ablative (S314A) and phospho-mimetic (S314D) mutations (A). Flowering time was determined by days to bolting and rosette number at bolting (B). Letters indicate significant differences between genotypes (one-way ANOVA p-value < 0.05). (C) Immunoblot analysis of raf24-2 plants constitutively over-expressing phospho-ablative (HA-HUB2 S314A ), phospho-mimetic (HA-HUB2 S314D ), which finds HA-HUB2 S314D maintains lower H2Bub1 levels. 50 μg of protein samples were loaded in each lane. Equal amounts of HA-HUB over-expression in the raf24-2 background was observed across the lines depicted here (Supplemental Figure 7).

    Article Snippet: After blocking 1 hour with 5% (w/v) non-fat milk, PVDF membranes were incubated overnight with anti-H2B (1:2500, abcam, ab1790), anti-H2Bub1 (1:1000, Cell Signaling, #5546), anti-GFP (1:2000, ChromoTek, PABG1), anti-HA(1:1000, Invitrogen, 26183), anti-H3 (1:2000, Invitrogen, PA5-16183) or anti-PAP (1:1000, SIGMA, P1291) followed by a 2-hour incubation with secondary antibodies, anti-rabbit (1:10000, Invitrogen, G-21234) or anti-mouse (1:5000, Invitrogen, G-21040).

    Techniques: Comparison, Expressing, Western Blot, Over Expression

    (A) In WT, the presence of RAF24 phosphorylates SnRK2s to induce phosphorylation of HUB2, ensuring appropriately tuned HUB2-ligase activity. This in turn optimizes HUB2ub1 levels to maintain proper transcriptional activation of FLC expression and flowering time . Upon the loss of RAF24, SnRK2 fails to phosphorylate HUB2, causing an over-accumulation of H2Bub1 and reduced transcriptional activation of FLC expression. This results in earlier flowering (B) Both the phosphoproteomic and HUB2-TAP pulldowns find that RAF24 acts upstream of a wide variety of floral regulators, including BES1 and FBH3 as well as HUB2 to fine-tune flower time. Identification of both known HUB2 interactors (with straight line) and new, candidate HUB2 interactors (with a dash line) related to flowering time indicates that RAF24 possesses versatile functions / mechanisms in controlling flowering time.

    Journal: bioRxiv

    Article Title: B4 Raf-like MAPKKK RAF24 regulates Arabidopsis thaliana flowering time through HISTONE MONO-UBIQUITINATION 2

    doi: 10.1101/2024.06.12.598286

    Figure Lengend Snippet: (A) In WT, the presence of RAF24 phosphorylates SnRK2s to induce phosphorylation of HUB2, ensuring appropriately tuned HUB2-ligase activity. This in turn optimizes HUB2ub1 levels to maintain proper transcriptional activation of FLC expression and flowering time . Upon the loss of RAF24, SnRK2 fails to phosphorylate HUB2, causing an over-accumulation of H2Bub1 and reduced transcriptional activation of FLC expression. This results in earlier flowering (B) Both the phosphoproteomic and HUB2-TAP pulldowns find that RAF24 acts upstream of a wide variety of floral regulators, including BES1 and FBH3 as well as HUB2 to fine-tune flower time. Identification of both known HUB2 interactors (with straight line) and new, candidate HUB2 interactors (with a dash line) related to flowering time indicates that RAF24 possesses versatile functions / mechanisms in controlling flowering time.

    Article Snippet: After blocking 1 hour with 5% (w/v) non-fat milk, PVDF membranes were incubated overnight with anti-H2B (1:2500, abcam, ab1790), anti-H2Bub1 (1:1000, Cell Signaling, #5546), anti-GFP (1:2000, ChromoTek, PABG1), anti-HA(1:1000, Invitrogen, 26183), anti-H3 (1:2000, Invitrogen, PA5-16183) or anti-PAP (1:1000, SIGMA, P1291) followed by a 2-hour incubation with secondary antibodies, anti-rabbit (1:10000, Invitrogen, G-21234) or anti-mouse (1:5000, Invitrogen, G-21040).

    Techniques: Activity Assay, Activation Assay, Expressing

    Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of H2Bub1 (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates

    Journal: Cell Communication and Signaling : CCS

    Article Title: USP22 supports the aggressive behavior of basal-like breast cancer by stimulating cellular respiration

    doi: 10.1186/s12964-023-01441-5

    Figure Lengend Snippet: Mammary tissue-specific loss of Usp22 impairs the stem cell-like properties of the growing murine mammary gland: A Schematic representation of the two transgenes of the MMTV-cre; Usp22 fl/fl mouse model. B Whole mounts staining of mammary glands showing a significant decrease of mammary duct branching density in MMTV-cre; Usp22 fl/fl mice compared to the control group with representative brightfield pictures (left panel) and the respective quantification of branching density and number of ex vivo cultured mammospheres (right panel). C Mammosphere formation assay mammary epithelial cells from MMTV; Usp22 wt/wt and MMTV; Usp22 fl/fl mice. D Hematoxylin and eosin staining (left panel) and immunohistochemical detection of H2Bub1 (right panel) on mammary gland sections from MMTV-cre; Usp22 fl/fl mice and MMTV-cre mice. E-I Brightfield pictures (white scale bar: 100 µm) ( E ), western blot analysis of USP22 protein ( F ), growth kinetics ( G ), colony formation assay ( H ) and mammosphere formation assay ( I ) in siControl- and siUSP22-treated MCF10A and MCF12A cells. J Gene set enrichment analysis (GSEA) performed on the high-throughput RNA sequencing data of siControl- and siUSP22-treated MCF10A cells (accession number: E-MTAB-8247). Statistics: B (right panel): One-way Anova; C, G (based on the area under the curve = AUC); I: Student t-test. * p <0.05, *** p <0.005. All experiments were performed in at least three biological replicates

    Article Snippet: Anti-H2Bub1 antibody (mouse, homemade at 1:50 dilution) or anti-USP22 (Sigma-Aldrich, HPA044980 at 1:100 dilution) was diluted on blocking solution and samples were treated overnight.

    Techniques: Staining, Ex Vivo, Cell Culture, Tube Formation Assay, Immunohistochemistry, Western Blot, Colony Assay, High Throughput Screening Assay, RNA Sequencing Assay