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antibody against integrin β3 subunit  (Merck KGaA)

 
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    Merck KGaA antibody against integrin β3 subunit
    Antibody Against Integrin β3 Subunit, supplied by Merck KGaA, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/antibody against integrin β3 subunit/product/Merck KGaA
    Average 90 stars, based on 1 article reviews
    antibody against integrin β3 subunit - by Bioz Stars, 2026-02
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    Expression of integrin αvβ3 in cultured hepatocytes. Human LO2 hepatocytes were cultured with the medium containing 100 μmol/L palmitate acid and 200 μmol/L oleic acid (FFA) for 24 hours, and the cells cultured in the medium without FFA served as the control. A: Representative micrographs of the control and FFA-cultured hepatocytes after stained with Oil-Red O. Images were taken at original magnification (200 ×), scale bars = 20 μm; B and C: Representative fluorescent images of the control (B) and FFA-cultured (C) hepatocytes after separately stained with integrin αv and β3 subunits antibody (green color) and counterstained with albumin antibody (red color). 6-diamidino-2-phenylindole was used for nuclei staining. The merged images show the yellow color area by overlaying images of the counterstaining. Images were taken at original magnification (400 ×), scale bars = 100 μm; D: Comparison of the message RNA levels of integrin αv and β3 subunits in the control and FFA-cultured hepatocytes. The message RNA levels of integrin αv and β3 subunit were determined by quantitative real-time polymerase chain reaction analysis; E and F: Comparison of the protein amounts of integrin αv and β3 subunits in the control and FFA-cultured hepatocytes. The protein amounts of integrin αv and β3 subunits were analyzed by western-blot assay, and β-Tublin was used as the reference. All experiments were undertaken in triplicates. In all panels, data are expressed in means ± SD. FFA: Oleic acid; DAPI: 6-diamidino-2-phenylindole.

    Journal: World Journal of Hepatology

    Article Title: Non-invasively differentiate non-alcoholic steatohepatitis by visualizing hepatic integrin αvβ3 expression with a targeted molecular imaging modality

    doi: 10.4254/wjh.v16.i11.1290

    Figure Lengend Snippet: Expression of integrin αvβ3 in cultured hepatocytes. Human LO2 hepatocytes were cultured with the medium containing 100 μmol/L palmitate acid and 200 μmol/L oleic acid (FFA) for 24 hours, and the cells cultured in the medium without FFA served as the control. A: Representative micrographs of the control and FFA-cultured hepatocytes after stained with Oil-Red O. Images were taken at original magnification (200 ×), scale bars = 20 μm; B and C: Representative fluorescent images of the control (B) and FFA-cultured (C) hepatocytes after separately stained with integrin αv and β3 subunits antibody (green color) and counterstained with albumin antibody (red color). 6-diamidino-2-phenylindole was used for nuclei staining. The merged images show the yellow color area by overlaying images of the counterstaining. Images were taken at original magnification (400 ×), scale bars = 100 μm; D: Comparison of the message RNA levels of integrin αv and β3 subunits in the control and FFA-cultured hepatocytes. The message RNA levels of integrin αv and β3 subunit were determined by quantitative real-time polymerase chain reaction analysis; E and F: Comparison of the protein amounts of integrin αv and β3 subunits in the control and FFA-cultured hepatocytes. The protein amounts of integrin αv and β3 subunits were analyzed by western-blot assay, and β-Tublin was used as the reference. All experiments were undertaken in triplicates. In all panels, data are expressed in means ± SD. FFA: Oleic acid; DAPI: 6-diamidino-2-phenylindole.

    Article Snippet: Secondly, after being fixed with 4% paraformaldehyde and permeabilized with phosphate-buffered saline (PBS) containing 0.1% Triton X-100 and 0.1 mg/mL RNase A when appropriate, the control and FFA-cultured hepatocytes were incubated with primary antibodies against integrin αv subunit (1:1000, Abmart, T56887) or integrin β3 subunit (1:1000, Abmart, M015908), and albumin (1:1000, Servicebio, GB122080) at 4 °C overnight.

    Techniques: Expressing, Cell Culture, Control, Staining, Comparison, Real-time Polymerase Chain Reaction, Western Blot

    Expression of integrin αvβ3 in livers of rabbits with non-alcoholic fatty liver disease. Non-alcoholic fatty liver disease was induced in rabbits by high-fat diet (HFD) for 2, 6, and 8 months (referred to as HFD-2M, 6M and 8M), and rabbits fed with regular diet for 8 months served as the control group ( n = 6 per group). A: Representative micrographs of hepatic histology stained with hematoxylin-eosin staining (200 ×), Sirius red (100 ×), and immunohistochemistry for integrin β3 subunit (400 ×). In immunohistochemistry staining images, the brown areas indicated integrin β3 subunit positive staining, scale bars = 50 μm; B: Comparison of non-alcoholic fatty liver disease activity score in the control and HFD-fed rabbits; C: Comparison of the percentage of integrin β3 subunit positive-staining area in liver sections of the control and HFD-fed rabbits. For semi-quantitative analysis of hepatic integrin αvβ3 expression level, 10 fields were randomly selected and recorded from each section stained with immunohistochemistry for integrin β3 subunit. Then integrin β3 subunit positive-staining area was measured, and the percentages of the positive-staining area in liver sections were compared. In all panels, data are expressed in means ± SD. IHC: Immunohistochemistry; HE: Hematoxylin-eosin staining; CTRL: Normal control group; M: Month; NS: Not significant; NAFLD: Non-alcoholic fatty liver disease.

    Journal: World Journal of Hepatology

    Article Title: Non-invasively differentiate non-alcoholic steatohepatitis by visualizing hepatic integrin αvβ3 expression with a targeted molecular imaging modality

    doi: 10.4254/wjh.v16.i11.1290

    Figure Lengend Snippet: Expression of integrin αvβ3 in livers of rabbits with non-alcoholic fatty liver disease. Non-alcoholic fatty liver disease was induced in rabbits by high-fat diet (HFD) for 2, 6, and 8 months (referred to as HFD-2M, 6M and 8M), and rabbits fed with regular diet for 8 months served as the control group ( n = 6 per group). A: Representative micrographs of hepatic histology stained with hematoxylin-eosin staining (200 ×), Sirius red (100 ×), and immunohistochemistry for integrin β3 subunit (400 ×). In immunohistochemistry staining images, the brown areas indicated integrin β3 subunit positive staining, scale bars = 50 μm; B: Comparison of non-alcoholic fatty liver disease activity score in the control and HFD-fed rabbits; C: Comparison of the percentage of integrin β3 subunit positive-staining area in liver sections of the control and HFD-fed rabbits. For semi-quantitative analysis of hepatic integrin αvβ3 expression level, 10 fields were randomly selected and recorded from each section stained with immunohistochemistry for integrin β3 subunit. Then integrin β3 subunit positive-staining area was measured, and the percentages of the positive-staining area in liver sections were compared. In all panels, data are expressed in means ± SD. IHC: Immunohistochemistry; HE: Hematoxylin-eosin staining; CTRL: Normal control group; M: Month; NS: Not significant; NAFLD: Non-alcoholic fatty liver disease.

    Article Snippet: Secondly, after being fixed with 4% paraformaldehyde and permeabilized with phosphate-buffered saline (PBS) containing 0.1% Triton X-100 and 0.1 mg/mL RNase A when appropriate, the control and FFA-cultured hepatocytes were incubated with primary antibodies against integrin αv subunit (1:1000, Abmart, T56887) or integrin β3 subunit (1:1000, Abmart, M015908), and albumin (1:1000, Servicebio, GB122080) at 4 °C overnight.

    Techniques: Expressing, Control, Staining, Immunohistochemistry, Comparison, Activity Assay

    Expression of integrin αvβ3 in livers of rats with non-alcoholic fatty liver disease. Non-alcoholic fatty liver disease was induced in rats by high-fat high-carbohydrate diet (HFCD) for 2, 4, and 6 months (referred to as HFCD-2M, 4M and 6M), and rats fed with regular diet for 6 months served as the control group ( n = 6 per group). A: Representative micrographs of hepatic histology stained with H&E (200 ×), Masson (100 ×), and Oil-red O (200 ×), scale bars = 50 μm; B: Comparison of non-alcoholic fatty liver disease activity score in the control and HFCD-fed rats; C: Comparison of hepatic integrin αvβ3 message RNA level in the control and HFCD-fed rats. Hepatic message RNA levels of integrin αv and β3 subunits were respectively determined by quantitative real-time polymerase chain reaction analysis; D-F: Comparison of the protein amounts of integrin αvβ3 in livers of the control and HFCD-fed rats. The protein amounts of integrin αv and β3 subunits were analyzed by western-blot assay, and β-Tublin was used as the reference. In all panels, data are expressed in means ± SD. HE: Hematoxylin-eosin staining; CTRL: Normal control group; M: Month; NS: Not significant; NAFLD: Non-alcoholic fatty liver disease.

    Journal: World Journal of Hepatology

    Article Title: Non-invasively differentiate non-alcoholic steatohepatitis by visualizing hepatic integrin αvβ3 expression with a targeted molecular imaging modality

    doi: 10.4254/wjh.v16.i11.1290

    Figure Lengend Snippet: Expression of integrin αvβ3 in livers of rats with non-alcoholic fatty liver disease. Non-alcoholic fatty liver disease was induced in rats by high-fat high-carbohydrate diet (HFCD) for 2, 4, and 6 months (referred to as HFCD-2M, 4M and 6M), and rats fed with regular diet for 6 months served as the control group ( n = 6 per group). A: Representative micrographs of hepatic histology stained with H&E (200 ×), Masson (100 ×), and Oil-red O (200 ×), scale bars = 50 μm; B: Comparison of non-alcoholic fatty liver disease activity score in the control and HFCD-fed rats; C: Comparison of hepatic integrin αvβ3 message RNA level in the control and HFCD-fed rats. Hepatic message RNA levels of integrin αv and β3 subunits were respectively determined by quantitative real-time polymerase chain reaction analysis; D-F: Comparison of the protein amounts of integrin αvβ3 in livers of the control and HFCD-fed rats. The protein amounts of integrin αv and β3 subunits were analyzed by western-blot assay, and β-Tublin was used as the reference. In all panels, data are expressed in means ± SD. HE: Hematoxylin-eosin staining; CTRL: Normal control group; M: Month; NS: Not significant; NAFLD: Non-alcoholic fatty liver disease.

    Article Snippet: Secondly, after being fixed with 4% paraformaldehyde and permeabilized with phosphate-buffered saline (PBS) containing 0.1% Triton X-100 and 0.1 mg/mL RNase A when appropriate, the control and FFA-cultured hepatocytes were incubated with primary antibodies against integrin αv subunit (1:1000, Abmart, T56887) or integrin β3 subunit (1:1000, Abmart, M015908), and albumin (1:1000, Servicebio, GB122080) at 4 °C overnight.

    Techniques: Expressing, Control, Staining, Comparison, Activity Assay, Real-time Polymerase Chain Reaction, Western Blot

    Immunofluorescent co-localization of integrin αvβ3 and the markers of various hepatic cells including α-smooth muscle actin, cluster of differentiation 31, cluster of differentiation 68 or cluster of differentiation 163 in livers of the control and high-fat high-carbohydrate diet-fed rats. Representative fluorescent images of integrin β3 subunit (green color) and albumin, α-smooth muscle actin, cluster of differentiation (CD) 31, CD68 and CD163 (red color) in liver sections, which were separately stained with specific first antibodies and visualized by second antibodies, and counterstained with 6-diamidino-2-phenylindole for nuclei staining. The merged images show the yellow color area by overlaying images of the counterstaining, and amplified images corresponding to the indicated areas in boxes are present. Images were recorded at original magnification (400 ×), scale bars = 100 μm. A: Control; B: High-fat high-carbohydrate diet (HFCD)-2M; C: HFCD-4M; D: HFCD-6M rats; E: Comparison of the percentage of integrin β3 subunit positive-staining area in liver sections of the control and HFCD-fed rats. Ten fields were randomly selected and recorded from each section. Then integrin β3 positive-staining area was measured, and the percentages of the positive-staining area in liver sections were compared; F: Comparison of the ratio of the overlapped yellow area to integrin β3 subunit positive-staining green area in liver sections of HFCD-6M rats. Ten fields were randomly selected and recorded from each section. Then integrin β3 subunit positive-staining area and the area of integrin β3 subunit positive-staining overlapped with hepatic cellular markers positive-staining were respectively measured, and the ratios were compared. In all panels, data are expressed in means ± SD. DAPI: 6-diamidino-2-phenylindole; CTRL: Normal control group; M: Month; CD: Cluster of differentiation; αSMA: α-smooth muscle actin.

    Journal: World Journal of Hepatology

    Article Title: Non-invasively differentiate non-alcoholic steatohepatitis by visualizing hepatic integrin αvβ3 expression with a targeted molecular imaging modality

    doi: 10.4254/wjh.v16.i11.1290

    Figure Lengend Snippet: Immunofluorescent co-localization of integrin αvβ3 and the markers of various hepatic cells including α-smooth muscle actin, cluster of differentiation 31, cluster of differentiation 68 or cluster of differentiation 163 in livers of the control and high-fat high-carbohydrate diet-fed rats. Representative fluorescent images of integrin β3 subunit (green color) and albumin, α-smooth muscle actin, cluster of differentiation (CD) 31, CD68 and CD163 (red color) in liver sections, which were separately stained with specific first antibodies and visualized by second antibodies, and counterstained with 6-diamidino-2-phenylindole for nuclei staining. The merged images show the yellow color area by overlaying images of the counterstaining, and amplified images corresponding to the indicated areas in boxes are present. Images were recorded at original magnification (400 ×), scale bars = 100 μm. A: Control; B: High-fat high-carbohydrate diet (HFCD)-2M; C: HFCD-4M; D: HFCD-6M rats; E: Comparison of the percentage of integrin β3 subunit positive-staining area in liver sections of the control and HFCD-fed rats. Ten fields were randomly selected and recorded from each section. Then integrin β3 positive-staining area was measured, and the percentages of the positive-staining area in liver sections were compared; F: Comparison of the ratio of the overlapped yellow area to integrin β3 subunit positive-staining green area in liver sections of HFCD-6M rats. Ten fields were randomly selected and recorded from each section. Then integrin β3 subunit positive-staining area and the area of integrin β3 subunit positive-staining overlapped with hepatic cellular markers positive-staining were respectively measured, and the ratios were compared. In all panels, data are expressed in means ± SD. DAPI: 6-diamidino-2-phenylindole; CTRL: Normal control group; M: Month; CD: Cluster of differentiation; αSMA: α-smooth muscle actin.

    Article Snippet: Secondly, after being fixed with 4% paraformaldehyde and permeabilized with phosphate-buffered saline (PBS) containing 0.1% Triton X-100 and 0.1 mg/mL RNase A when appropriate, the control and FFA-cultured hepatocytes were incubated with primary antibodies against integrin αv subunit (1:1000, Abmart, T56887) or integrin β3 subunit (1:1000, Abmart, M015908), and albumin (1:1000, Servicebio, GB122080) at 4 °C overnight.

    Techniques: Control, Staining, Amplification, Comparison

    A: Distribution of ITGB1, ITGB2, ITGB3 and CAV-1 in THP-1 and HUVEC determined by flow cytometry. Ten thousand cells were analyzed for each of the specimens; B: Leptospires in THP-1 and HUVEC under the laser confocal microscope after infection with L . interrogans strain Lai for 1 h. The blue plaques in the middle of cells indicate the nuclus. The red spots around the nuclus indicate the intracellular leptospires; C: Statistical summary of red fluorescence intensity reflecting the leptospires in THP-1 and HUVEC after infection with L . interrogans strain Lai for 1 h. Statistical data from experiments such as shown in B. Bars show the means ± SD of three independent experiments. One hundred cells were analyzed for each of the specimens. *: p < 0.05 vs the red fluorescence intensity reflecting the leptospires in the wild type cells during infection. D: Relative gene expression of ITGB1, ITGB2 ITGB3, CAV-1 in THP-1 or HUVEC were analysed by comparing treatment of 4h of leptospires infection and non-infection. Bars show the means ± SD of three independent experiments. *: p < 0.05 vs the gene relative expression of treatment of non-infection.

    Journal: PLoS Neglected Tropical Diseases

    Article Title: Internalization of Leptospira interrogans via diverse endocytosis mechanisms in human macrophages and vascular endothelial cells

    doi: 10.1371/journal.pntd.0010778

    Figure Lengend Snippet: A: Distribution of ITGB1, ITGB2, ITGB3 and CAV-1 in THP-1 and HUVEC determined by flow cytometry. Ten thousand cells were analyzed for each of the specimens; B: Leptospires in THP-1 and HUVEC under the laser confocal microscope after infection with L . interrogans strain Lai for 1 h. The blue plaques in the middle of cells indicate the nuclus. The red spots around the nuclus indicate the intracellular leptospires; C: Statistical summary of red fluorescence intensity reflecting the leptospires in THP-1 and HUVEC after infection with L . interrogans strain Lai for 1 h. Statistical data from experiments such as shown in B. Bars show the means ± SD of three independent experiments. One hundred cells were analyzed for each of the specimens. *: p < 0.05 vs the red fluorescence intensity reflecting the leptospires in the wild type cells during infection. D: Relative gene expression of ITGB1, ITGB2 ITGB3, CAV-1 in THP-1 or HUVEC were analysed by comparing treatment of 4h of leptospires infection and non-infection. Bars show the means ± SD of three independent experiments. *: p < 0.05 vs the gene relative expression of treatment of non-infection.

    Article Snippet: The integrin subunit β1-, β2-, β3- or CAV-1-encoding gene depleted, 30 μg antibody against integrin β1, β2 or β3 subunit (Santa Cruz) or 1.5 nM of a caveolae inhibitor filipin (Sigma) treated THP-1 or HUVEC cells were infected with L . interrogans strain Lai at a MOI of 100 for 1 h at 37°C.

    Techniques: Flow Cytometry, Microscopy, Infection, Fluorescence, Gene Expression, Expressing