tissue factor Search Results


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Elabscience Biotechnology mouse ctgf elisa kit
Succinate stimulated macrophage infiltration, activation of profibrotic M2 phenotype, upregulation of profibrotic factors in vivo and in vitro. A F4/80 immunohistochemistry staining indicated succinate markedly increased renal macrophage in the kidney interstitium rather than glomerulus. *** P < 0.001, versus control group, n = 5. B Renal proinflammatory M1 cytokines, including iNOS and IL6 mRNA levels, were reduced by succinate. ** P < 0.01, versus the control group, n = 5. C The mRNA levels of anti-inflammatory M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) in the kidney were markedly increased. ** P < 0.01;*** P < 0.001, versus control group, n = 5. D Succinate upregulated renal M2 macrophages-related profibrotic factors expression (galectin3, MMP9, MMP12, MMP13, PDGF, and <t>CTGF).</t> ns, not significant; ** P < 0.01;*** P < 0.001, versus control group, n = 5. RAW 264.7 cells were treated at 500 μM succinate for 24 h, and quantitative PCR analysis and immunoblotting were adopted to detect the effects of succinate on M2 polarization and expression of profibrotic factors in vitro. E Succinate had no effects on the cell viability of RAW 264.7. Succinate downregulated M1 cytokines (iNOS and IL6) mRNA levels ( F ) while significantly upregulated M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) ( G ). *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. Likewise, succinate remarkably increased M2 macrophage-related profibrotic factor expression (MMP9, MMP12, MMP13, PDGF, and CTGF) ( H ). ns, not significant; *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. The cell supernatant was measured by mouse CTGF <t>ELISA</t> kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD). Similarly, succinate increased CTGF release of macrophages ( I )
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Elabscience Biotechnology sandwich elisa
Succinate stimulated macrophage infiltration, activation of profibrotic M2 phenotype, upregulation of profibrotic factors in vivo and in vitro. A F4/80 immunohistochemistry staining indicated succinate markedly increased renal macrophage in the kidney interstitium rather than glomerulus. *** P < 0.001, versus control group, n = 5. B Renal proinflammatory M1 cytokines, including iNOS and IL6 mRNA levels, were reduced by succinate. ** P < 0.01, versus the control group, n = 5. C The mRNA levels of anti-inflammatory M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) in the kidney were markedly increased. ** P < 0.01;*** P < 0.001, versus control group, n = 5. D Succinate upregulated renal M2 macrophages-related profibrotic factors expression (galectin3, MMP9, MMP12, MMP13, PDGF, and <t>CTGF).</t> ns, not significant; ** P < 0.01;*** P < 0.001, versus control group, n = 5. RAW 264.7 cells were treated at 500 μM succinate for 24 h, and quantitative PCR analysis and immunoblotting were adopted to detect the effects of succinate on M2 polarization and expression of profibrotic factors in vitro. E Succinate had no effects on the cell viability of RAW 264.7. Succinate downregulated M1 cytokines (iNOS and IL6) mRNA levels ( F ) while significantly upregulated M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) ( G ). *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. Likewise, succinate remarkably increased M2 macrophage-related profibrotic factor expression (MMP9, MMP12, MMP13, PDGF, and CTGF) ( H ). ns, not significant; *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. The cell supernatant was measured by mouse CTGF <t>ELISA</t> kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD). Similarly, succinate increased CTGF release of macrophages ( I )
Sandwich Elisa, supplied by Elabscience Biotechnology, 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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Elabscience Biotechnology elisa kit
Succinate stimulated macrophage infiltration, activation of profibrotic M2 phenotype, upregulation of profibrotic factors in vivo and in vitro. A F4/80 immunohistochemistry staining indicated succinate markedly increased renal macrophage in the kidney interstitium rather than glomerulus. *** P < 0.001, versus control group, n = 5. B Renal proinflammatory M1 cytokines, including iNOS and IL6 mRNA levels, were reduced by succinate. ** P < 0.01, versus the control group, n = 5. C The mRNA levels of anti-inflammatory M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) in the kidney were markedly increased. ** P < 0.01;*** P < 0.001, versus control group, n = 5. D Succinate upregulated renal M2 macrophages-related profibrotic factors expression (galectin3, MMP9, MMP12, MMP13, PDGF, and <t>CTGF).</t> ns, not significant; ** P < 0.01;*** P < 0.001, versus control group, n = 5. RAW 264.7 cells were treated at 500 μM succinate for 24 h, and quantitative PCR analysis and immunoblotting were adopted to detect the effects of succinate on M2 polarization and expression of profibrotic factors in vitro. E Succinate had no effects on the cell viability of RAW 264.7. Succinate downregulated M1 cytokines (iNOS and IL6) mRNA levels ( F ) while significantly upregulated M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) ( G ). *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. Likewise, succinate remarkably increased M2 macrophage-related profibrotic factor expression (MMP9, MMP12, MMP13, PDGF, and CTGF) ( H ). ns, not significant; *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. The cell supernatant was measured by mouse CTGF <t>ELISA</t> kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD). Similarly, succinate increased CTGF release of macrophages ( I )
Elisa Kit, supplied by Elabscience Biotechnology, used in various techniques. Bioz Stars score: 92/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


Succinate stimulated macrophage infiltration, activation of profibrotic M2 phenotype, upregulation of profibrotic factors in vivo and in vitro. A F4/80 immunohistochemistry staining indicated succinate markedly increased renal macrophage in the kidney interstitium rather than glomerulus. *** P < 0.001, versus control group, n = 5. B Renal proinflammatory M1 cytokines, including iNOS and IL6 mRNA levels, were reduced by succinate. ** P < 0.01, versus the control group, n = 5. C The mRNA levels of anti-inflammatory M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) in the kidney were markedly increased. ** P < 0.01;*** P < 0.001, versus control group, n = 5. D Succinate upregulated renal M2 macrophages-related profibrotic factors expression (galectin3, MMP9, MMP12, MMP13, PDGF, and CTGF). ns, not significant; ** P < 0.01;*** P < 0.001, versus control group, n = 5. RAW 264.7 cells were treated at 500 μM succinate for 24 h, and quantitative PCR analysis and immunoblotting were adopted to detect the effects of succinate on M2 polarization and expression of profibrotic factors in vitro. E Succinate had no effects on the cell viability of RAW 264.7. Succinate downregulated M1 cytokines (iNOS and IL6) mRNA levels ( F ) while significantly upregulated M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) ( G ). *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. Likewise, succinate remarkably increased M2 macrophage-related profibrotic factor expression (MMP9, MMP12, MMP13, PDGF, and CTGF) ( H ). ns, not significant; *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. The cell supernatant was measured by mouse CTGF ELISA kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD). Similarly, succinate increased CTGF release of macrophages ( I )

Journal: Cell Communication and Signaling : CCS

Article Title: The pathogenic role of succinate-SUCNR1: a critical function that induces renal fibrosis via M2 macrophage

doi: 10.1186/s12964-024-01481-5

Figure Lengend Snippet: Succinate stimulated macrophage infiltration, activation of profibrotic M2 phenotype, upregulation of profibrotic factors in vivo and in vitro. A F4/80 immunohistochemistry staining indicated succinate markedly increased renal macrophage in the kidney interstitium rather than glomerulus. *** P < 0.001, versus control group, n = 5. B Renal proinflammatory M1 cytokines, including iNOS and IL6 mRNA levels, were reduced by succinate. ** P < 0.01, versus the control group, n = 5. C The mRNA levels of anti-inflammatory M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) in the kidney were markedly increased. ** P < 0.01;*** P < 0.001, versus control group, n = 5. D Succinate upregulated renal M2 macrophages-related profibrotic factors expression (galectin3, MMP9, MMP12, MMP13, PDGF, and CTGF). ns, not significant; ** P < 0.01;*** P < 0.001, versus control group, n = 5. RAW 264.7 cells were treated at 500 μM succinate for 24 h, and quantitative PCR analysis and immunoblotting were adopted to detect the effects of succinate on M2 polarization and expression of profibrotic factors in vitro. E Succinate had no effects on the cell viability of RAW 264.7. Succinate downregulated M1 cytokines (iNOS and IL6) mRNA levels ( F ) while significantly upregulated M2 cytokines (Arg1, Fizz1, Mgl2, and IL-10) ( G ). *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. Likewise, succinate remarkably increased M2 macrophage-related profibrotic factor expression (MMP9, MMP12, MMP13, PDGF, and CTGF) ( H ). ns, not significant; *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. The cell supernatant was measured by mouse CTGF ELISA kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD). Similarly, succinate increased CTGF release of macrophages ( I )

Article Snippet: The cell supernatant was measured by mouse CTGF ELISA kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD).

Techniques: Activation Assay, In Vivo, In Vitro, Immunohistochemistry, Staining, Control, Expressing, Real-time Polymerase Chain Reaction, Western Blot, Enzyme-linked Immunosorbent Assay

CTGF neutralizing antibody inhibited the stimulation of fibroblasts by macrophage-conditioned medium. A CTGF antibody prevented the proliferative effects of CM on NRK-49F, indicated by the results of the CCK8 assay. *** P < 0.001, versus control group, n = 6 in CCK8, biologically repeated 3 times. B Also, the CTGF antibody suppressed the activation effects of CM on NRK-49F, as indicated by the results of the protein quantitative analysis of fibronectin and α-SMA. *** P < 0.001, versus control group, &&& P < 0.001, versus the succinate group, n = 3, biologically repeated 3 times

Journal: Cell Communication and Signaling : CCS

Article Title: The pathogenic role of succinate-SUCNR1: a critical function that induces renal fibrosis via M2 macrophage

doi: 10.1186/s12964-024-01481-5

Figure Lengend Snippet: CTGF neutralizing antibody inhibited the stimulation of fibroblasts by macrophage-conditioned medium. A CTGF antibody prevented the proliferative effects of CM on NRK-49F, indicated by the results of the CCK8 assay. *** P < 0.001, versus control group, n = 6 in CCK8, biologically repeated 3 times. B Also, the CTGF antibody suppressed the activation effects of CM on NRK-49F, as indicated by the results of the protein quantitative analysis of fibronectin and α-SMA. *** P < 0.001, versus control group, &&& P < 0.001, versus the succinate group, n = 3, biologically repeated 3 times

Article Snippet: The cell supernatant was measured by mouse CTGF ELISA kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD).

Techniques: CCK-8 Assay, Control, Activation Assay

Succinate promoted CTGF expression through activation of β-catenin. A Succinate increased protein levels of non-p-β-catenin and β-catenin in the mice kidney. *** P < 0.001, versus control group, n = 5. RAW 264.7 was treated with 500 μM succinate for 12 h. B Succinate enhanced protein levels of non-p-β-catenin and β-catenin in the RAW 264.7. *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. C Succinate promoted translocation of non-p-β-catenin into the nucleus. ICG-001 (2 μM) pretreatment RAW 264.7 for 1 h, 500 μM succinate stimulation for 24 h and 48 h. D ICG-001 prevented the increase of CTGF mRNA induced by succinate. *** P < 0.001, versus control group, &&& P < 0.001, versus the succinate group, n = 3, biologically repeated 3 times. E The elevation of CTGF protein level was also lowered by ICG-001. *** P < 0.001, versus control group, &&& P < 0.001, versus the succinate group, n = 3, biologically repeated 3 times

Journal: Cell Communication and Signaling : CCS

Article Title: The pathogenic role of succinate-SUCNR1: a critical function that induces renal fibrosis via M2 macrophage

doi: 10.1186/s12964-024-01481-5

Figure Lengend Snippet: Succinate promoted CTGF expression through activation of β-catenin. A Succinate increased protein levels of non-p-β-catenin and β-catenin in the mice kidney. *** P < 0.001, versus control group, n = 5. RAW 264.7 was treated with 500 μM succinate for 12 h. B Succinate enhanced protein levels of non-p-β-catenin and β-catenin in the RAW 264.7. *** P < 0.001, versus control group, n = 3, biologically repeated 3 times. C Succinate promoted translocation of non-p-β-catenin into the nucleus. ICG-001 (2 μM) pretreatment RAW 264.7 for 1 h, 500 μM succinate stimulation for 24 h and 48 h. D ICG-001 prevented the increase of CTGF mRNA induced by succinate. *** P < 0.001, versus control group, &&& P < 0.001, versus the succinate group, n = 3, biologically repeated 3 times. E The elevation of CTGF protein level was also lowered by ICG-001. *** P < 0.001, versus control group, &&& P < 0.001, versus the succinate group, n = 3, biologically repeated 3 times

Article Snippet: The cell supernatant was measured by mouse CTGF ELISA kit according to the manufacturer’s instructions (E-EL-M0340; Elabscience, Bethesda, MD).

Techniques: Expressing, Activation Assay, Control, Translocation Assay