bio rad wet blot transfer cell apparatus Search Results


goat anti human igg  (Bio-Rad)
95
Bio-Rad goat anti human igg
Goat Anti Human Igg, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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semidry electroblotting system  (Bio-Rad)
99
Bio-Rad semidry electroblotting system
Semidry Electroblotting System, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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mini trans blot  (Bio-Rad)
90
Bio-Rad mini trans blot
Mini Trans Blot, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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imagelab software version 6 1  (Bio-Rad)
99
Bio-Rad imagelab software version 6 1
Imagelab Software Version 6 1, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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rat cd47  (Bio-Rad)
93
Bio-Rad rat cd47
Figure 1. Galectin-5 is present on the surface of rat red cells. (A) Freshly isolated reticulocytes or erythrocytes were adsorbed on glass coverslips and processed for immunofluorescence as described in “Fluorescence-activated cell-sorting analysis of exosomes and red cells, fluorescence microscopy of red cells.” Transmission images of red cells (left) and corresponding fluorescence imaging (right) were recorded on cells by the use of purified rabbit anti–galectin-5 antibody followed by incubation withAlexa 488 anti–rabbit antibody. (B) Young reticulocytes and erythrocytes were analyzed by flow cytometry by the use of antibodies raised against Gal-2 (dashed line), Gal-4 (dotted line), and Gal-5 (solid line), already tested for their specificity (top), or the produced anti–galectin-5 serum (solid line) and the preimmune serum (bottom, dashed line). Tinted patterns indicate cell labeling obtained in the absence of primary antibodies. (C) Lymphocytes isolated from rat blood, as described in “Cells,” were analyzed by flow cytometry for Gal-5 (left, solid line), <t>CD47</t> (middle, solid line) and Syto 16 green (right, solid line). Tinted patterns indicate cell labeling in the absence of primary antibodies. (D) Ghost and raft extracts isolated from reticulocytes or mature erythrocytes, as described in “Red cell subcellular fractionation,” were processed by SDS-PAGE and analyzed by Western blot for the indicated proteins. The molecular mass (kDa) standards are indicated on the left.
Rat Cd47, supplied by Bio-Rad, 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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sheep anti ngf polyclonal ab  (Bio-Rad)
85
Bio-Rad sheep anti ngf polyclonal ab
FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine <t>NGF</t> was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF <t>by</t> <t>anti-NGF</t> Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with <t>polyclonal</t> anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.
Sheep Anti Ngf Polyclonal Ab, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 85/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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immun blot polyvinylidene fluoride membrane  (Bio-Rad)
96
Bio-Rad immun blot polyvinylidene fluoride membrane
FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine <t>NGF</t> was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF <t>by</t> <t>anti-NGF</t> Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with <t>polyclonal</t> anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.
Immun Blot Polyvinylidene Fluoride Membrane, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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mini trans blot cell  (Bio-Rad)
96
Bio-Rad mini trans blot cell
FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine <t>NGF</t> was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF <t>by</t> <t>anti-NGF</t> Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with <t>polyclonal</t> anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.
Mini Trans Blot Cell, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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quantity one software  (Bio-Rad)
96
Bio-Rad quantity one software
FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine <t>NGF</t> was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF <t>by</t> <t>anti-NGF</t> Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with <t>polyclonal</t> anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.
Quantity One Software, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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bis tris xt gel  (Bio-Rad)
98
Bio-Rad bis tris xt gel
FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine <t>NGF</t> was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF <t>by</t> <t>anti-NGF</t> Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with <t>polyclonal</t> anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.
Bis Tris Xt Gel, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 98/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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protein signals  (Bio-Rad)
99
Bio-Rad protein signals
FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine <t>NGF</t> was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF <t>by</t> <t>anti-NGF</t> Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with <t>polyclonal</t> anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.
Protein Signals, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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ecl plus western blotting detection reagents  (Bio-Rad)
96
Bio-Rad ecl plus western blotting detection reagents
FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine <t>NGF</t> was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF <t>by</t> <t>anti-NGF</t> Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with <t>polyclonal</t> anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.
Ecl Plus Western Blotting Detection Reagents, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


Figure 1. Galectin-5 is present on the surface of rat red cells. (A) Freshly isolated reticulocytes or erythrocytes were adsorbed on glass coverslips and processed for immunofluorescence as described in “Fluorescence-activated cell-sorting analysis of exosomes and red cells, fluorescence microscopy of red cells.” Transmission images of red cells (left) and corresponding fluorescence imaging (right) were recorded on cells by the use of purified rabbit anti–galectin-5 antibody followed by incubation withAlexa 488 anti–rabbit antibody. (B) Young reticulocytes and erythrocytes were analyzed by flow cytometry by the use of antibodies raised against Gal-2 (dashed line), Gal-4 (dotted line), and Gal-5 (solid line), already tested for their specificity (top), or the produced anti–galectin-5 serum (solid line) and the preimmune serum (bottom, dashed line). Tinted patterns indicate cell labeling obtained in the absence of primary antibodies. (C) Lymphocytes isolated from rat blood, as described in “Cells,” were analyzed by flow cytometry for Gal-5 (left, solid line), CD47 (middle, solid line) and Syto 16 green (right, solid line). Tinted patterns indicate cell labeling in the absence of primary antibodies. (D) Ghost and raft extracts isolated from reticulocytes or mature erythrocytes, as described in “Red cell subcellular fractionation,” were processed by SDS-PAGE and analyzed by Western blot for the indicated proteins. The molecular mass (kDa) standards are indicated on the left.

Journal: Blood

Article Title: Galectin-5 is bound onto the surface of rat reticulocyte exosomes and modulates vesicle uptake by macrophages.

doi: 10.1182/blood-2009-07-231449

Figure Lengend Snippet: Figure 1. Galectin-5 is present on the surface of rat red cells. (A) Freshly isolated reticulocytes or erythrocytes were adsorbed on glass coverslips and processed for immunofluorescence as described in “Fluorescence-activated cell-sorting analysis of exosomes and red cells, fluorescence microscopy of red cells.” Transmission images of red cells (left) and corresponding fluorescence imaging (right) were recorded on cells by the use of purified rabbit anti–galectin-5 antibody followed by incubation withAlexa 488 anti–rabbit antibody. (B) Young reticulocytes and erythrocytes were analyzed by flow cytometry by the use of antibodies raised against Gal-2 (dashed line), Gal-4 (dotted line), and Gal-5 (solid line), already tested for their specificity (top), or the produced anti–galectin-5 serum (solid line) and the preimmune serum (bottom, dashed line). Tinted patterns indicate cell labeling obtained in the absence of primary antibodies. (C) Lymphocytes isolated from rat blood, as described in “Cells,” were analyzed by flow cytometry for Gal-5 (left, solid line), CD47 (middle, solid line) and Syto 16 green (right, solid line). Tinted patterns indicate cell labeling in the absence of primary antibodies. (D) Ghost and raft extracts isolated from reticulocytes or mature erythrocytes, as described in “Red cell subcellular fractionation,” were processed by SDS-PAGE and analyzed by Western blot for the indicated proteins. The molecular mass (kDa) standards are indicated on the left.

Article Snippet: Mouse anti–rat CD47 was from Serotec Limited.

Techniques: Isolation, Fluorescence, FACS, Microscopy, Transmission Assay, Imaging, Incubation, Cytometry, Produced, Labeling, Fractionation, SDS Page, Western Blot

FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine NGF was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF by anti-NGF Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with polyclonal anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.

Journal: Journal of immunology (Baltimore, Md. : 1950)

Article Title: A virus-like particle-based anti-nerve growth factor vaccine reduces inflammatory hyperalgesia: potential long-term therapy for chronic pain.

doi: 10.4049/jimmunol.1000030

Figure Lengend Snippet: FIGURE 1. Production and functional analysis of the rNGFQb vaccine. A, Production of rNGF. Murine NGF was expressed in HEK293T cells. Antipentahistidine immunoblot analysis of HEK293T lysates (first lane) and cell-culture supernatants (second lane) revealed expression of the NGF proprotein by HEK293T cells and secretion of the processed 14.7-kDa mature form of NGF into the cell-culture supernatant. Coomassie staining of NGF purified from supernatants by affinity chromatography confirmed homogeneity (third lane). B, Recognition of NGF by anti-NGF Abs. Recombinantly expressed NGF (white circles) was compared with ex vivo- purified NGF (black squares). Different dilutions of both proteins were applied to ELISA plates coated with anti-NGF mAb. Bound NGF was detected with polyclonal anti-NGF Abs. Averages of triplicates 6 SEM. C, NGF receptor binding. The NGF-specific receptor TrkA was coated onto ELISA plates and descending concentrations of both proteins applied. Receptor bound NGF was detected with polyclonal NGF Abs as in B. Averages of triplicates 6 SEM. D, Bioactivity of NGF. The NGF re- sponsive cell line TF-1 was stimulated with descending concentrations of NGF and proliferation determined by BrdU incorporation during DNA synthesis. Averages of triplicates 6 SEM. E, Analysis of NGFQb vaccine. NGF was cross-linked to VLPs with a heterobifunctional cross-linker. An immunoblot of NGF (left lane) or the NGFQb conjugate vaccine (right lane) analyzed with an anti-pentahistidine–specific Ab showed a dominant band appearing at 29 kDa corresponding to a Qb monomer (14.2 kDa) conjugated to one molecule NGF (14.7 kDa). Higher molecular mass bands correspond to Qb-oligomers linked to one NGF molecule. F, Binding of TrkA to NGFQb. Ascending concentrations of Qb (filled squares) or NGFQb (open circles) were immobilized on an ELISA plate coated with anti-Qb mAb. Bound vaccine was incubated with TrkA re- ceptor containing a human Fc domain. Binding of receptor to NGF dis- played on VLP was detected with peroxidase-conjugated goat anti-human Abs. Averages of triplicates 6 SEM. LY, lysates; SN, supernatants.

Article Snippet: Then, plates were washed six times with PBS-T and incubated with a 1:500 dilution of a sheep anti-NGF polyclonal Ab (AbD Serotec) for 1 h at RT.

Techniques: Functional Assay, Western Blot, Cell Culture, Expressing, Staining, Chromatography, Ex Vivo, Enzyme-linked Immunosorbent Assay, Binding Assay, BrdU Incorporation Assay, DNA Synthesis, Incubation