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Proteintech ccl13
Gene expression levels of candidate genes. Gene expression levels of CXCR1 ( A ), <t>CCL13</t> ( B ), PPBP ( C ), CCR3 ( D ) and MMP9 ( E ) in CRSwNP and control samples. Gene expression levels of CXCR1 ( F ), CCL13 ( G ), PPBP ( H ), CCR3 ( I ) and MMP9 ( J ) in different inflammatory endotypes of CRSwNP. (* P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant).
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1) Product Images from "Immuno-transcriptomic analysis based on machine learning identifies immunity signature genes of chronic rhinosinusitis with nasal polyps"

Article Title: Immuno-transcriptomic analysis based on machine learning identifies immunity signature genes of chronic rhinosinusitis with nasal polyps

Journal: Scientific Reports

doi: 10.1038/s41598-025-02508-8

Gene expression levels of candidate genes. Gene expression levels of CXCR1 ( A ), CCL13 ( B ), PPBP ( C ), CCR3 ( D ) and MMP9 ( E ) in CRSwNP and control samples. Gene expression levels of CXCR1 ( F ), CCL13 ( G ), PPBP ( H ), CCR3 ( I ) and MMP9 ( J ) in different inflammatory endotypes of CRSwNP. (* P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant).
Figure Legend Snippet: Gene expression levels of candidate genes. Gene expression levels of CXCR1 ( A ), CCL13 ( B ), PPBP ( C ), CCR3 ( D ) and MMP9 ( E ) in CRSwNP and control samples. Gene expression levels of CXCR1 ( F ), CCL13 ( G ), PPBP ( H ), CCR3 ( I ) and MMP9 ( J ) in different inflammatory endotypes of CRSwNP. (* P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant).

Techniques Used: Gene Expression, Control

Candidate gene protein expression levels in normal mucosal tissues and chronic rhinosinusitis with nasal polyps (CRSwNP) tissues were analysed using IHC staining. Unpaired t-tests were used to determine the significant differences for candidate gene protein expression between the normal mucosal(n = 5) and CRSwNP (n = 5) groups. ( A ) CXCR1. ( B ) CCL13. ( C ) PPBP. ( D ) CCR3. ( E ) MMP9. (* P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001).
Figure Legend Snippet: Candidate gene protein expression levels in normal mucosal tissues and chronic rhinosinusitis with nasal polyps (CRSwNP) tissues were analysed using IHC staining. Unpaired t-tests were used to determine the significant differences for candidate gene protein expression between the normal mucosal(n = 5) and CRSwNP (n = 5) groups. ( A ) CXCR1. ( B ) CCL13. ( C ) PPBP. ( D ) CCR3. ( E ) MMP9. (* P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001).

Techniques Used: Expressing, Immunohistochemistry



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Gene expression levels of candidate genes. Gene expression levels of CXCR1 ( A ), <t>CCL13</t> ( B ), PPBP ( C ), CCR3 ( D ) and MMP9 ( E ) in CRSwNP and control samples. Gene expression levels of CXCR1 ( F ), CCL13 ( G ), PPBP ( H ), CCR3 ( I ) and MMP9 ( J ) in different inflammatory endotypes of CRSwNP. (* P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant).
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Gene expression levels of candidate genes. Gene expression levels of CXCR1 ( A ), <t>CCL13</t> ( B ), PPBP ( C ), CCR3 ( D ) and MMP9 ( E ) in CRSwNP and control samples. Gene expression levels of CXCR1 ( F ), CCL13 ( G ), PPBP ( H ), CCR3 ( I ) and MMP9 ( J ) in different inflammatory endotypes of CRSwNP. (* P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant).
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In vitro Senescent GBM Model via p16 INK4A Overexpression Exhibit Senescence Phenotype. A The protein (upper panel) and mRNA expression levels (lower panel) of p16 INK4A ( CDKN2A ) in SNU201 after transduction with either an empty vector (Empty) or a p16 INK4A -overexpression vector (p16 INK4A ) is shown. kDa: kilodalton. NC: non-transduced SNU201. B The morphology of SNU201 cells post-transduction is depicted in the left panel, with SA-β-Gal staining results in the middle panel and quantification data on the right. C-D Real-time PCR data for representative SASPs and chemokines in SNU201 cells transduced with either vector. E-F IHC analysis for CCL2 and <t>CCL13</t> in GBM tissues, with quantification data in the lower right panel. Statistical differences in ( A-D ) were analyzed using Student's t-test while those in ( E-F ) were analyzed using the Chi-square test.
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Image Search Results


Gene expression levels of candidate genes. Gene expression levels of CXCR1 ( A ), CCL13 ( B ), PPBP ( C ), CCR3 ( D ) and MMP9 ( E ) in CRSwNP and control samples. Gene expression levels of CXCR1 ( F ), CCL13 ( G ), PPBP ( H ), CCR3 ( I ) and MMP9 ( J ) in different inflammatory endotypes of CRSwNP. (* P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant).

Journal: Scientific Reports

Article Title: Immuno-transcriptomic analysis based on machine learning identifies immunity signature genes of chronic rhinosinusitis with nasal polyps

doi: 10.1038/s41598-025-02508-8

Figure Lengend Snippet: Gene expression levels of candidate genes. Gene expression levels of CXCR1 ( A ), CCL13 ( B ), PPBP ( C ), CCR3 ( D ) and MMP9 ( E ) in CRSwNP and control samples. Gene expression levels of CXCR1 ( F ), CCL13 ( G ), PPBP ( H ), CCR3 ( I ) and MMP9 ( J ) in different inflammatory endotypes of CRSwNP. (* P < 0.05, ** P < 0.01, *** P < 0.001, ns, not significant).

Article Snippet: The primary antibodies were as follows: CXCR1 (1:500; Servicebio, GB11625-100), CCL13(1:1000; Proteintech, Ag24131),PPBP(1:50; Proteintech, 13313-1-AP),CCR3(1:200; Proteintech, 22351-1-AP), MMP-9(1:500; Proteintech, 10375-2-AP), GAPDH(1:3000; Servicebio, GB15004-100).

Techniques: Gene Expression, Control

Candidate gene protein expression levels in normal mucosal tissues and chronic rhinosinusitis with nasal polyps (CRSwNP) tissues were analysed using IHC staining. Unpaired t-tests were used to determine the significant differences for candidate gene protein expression between the normal mucosal(n = 5) and CRSwNP (n = 5) groups. ( A ) CXCR1. ( B ) CCL13. ( C ) PPBP. ( D ) CCR3. ( E ) MMP9. (* P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001).

Journal: Scientific Reports

Article Title: Immuno-transcriptomic analysis based on machine learning identifies immunity signature genes of chronic rhinosinusitis with nasal polyps

doi: 10.1038/s41598-025-02508-8

Figure Lengend Snippet: Candidate gene protein expression levels in normal mucosal tissues and chronic rhinosinusitis with nasal polyps (CRSwNP) tissues were analysed using IHC staining. Unpaired t-tests were used to determine the significant differences for candidate gene protein expression between the normal mucosal(n = 5) and CRSwNP (n = 5) groups. ( A ) CXCR1. ( B ) CCL13. ( C ) PPBP. ( D ) CCR3. ( E ) MMP9. (* P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001).

Article Snippet: The primary antibodies were as follows: CXCR1 (1:500; Servicebio, GB11625-100), CCL13(1:1000; Proteintech, Ag24131),PPBP(1:50; Proteintech, 13313-1-AP),CCR3(1:200; Proteintech, 22351-1-AP), MMP-9(1:500; Proteintech, 10375-2-AP), GAPDH(1:3000; Servicebio, GB15004-100).

Techniques: Expressing, Immunohistochemistry

In vitro Senescent GBM Model via p16 INK4A Overexpression Exhibit Senescence Phenotype. A The protein (upper panel) and mRNA expression levels (lower panel) of p16 INK4A ( CDKN2A ) in SNU201 after transduction with either an empty vector (Empty) or a p16 INK4A -overexpression vector (p16 INK4A ) is shown. kDa: kilodalton. NC: non-transduced SNU201. B The morphology of SNU201 cells post-transduction is depicted in the left panel, with SA-β-Gal staining results in the middle panel and quantification data on the right. C-D Real-time PCR data for representative SASPs and chemokines in SNU201 cells transduced with either vector. E-F IHC analysis for CCL2 and CCL13 in GBM tissues, with quantification data in the lower right panel. Statistical differences in ( A-D ) were analyzed using Student's t-test while those in ( E-F ) were analyzed using the Chi-square test.

Journal: Neoplasia (New York, N.Y.)

Article Title: High p16 INK4A expression in glioblastoma is associated with senescence phenotype and better prognosis

doi: 10.1016/j.neo.2024.101116

Figure Lengend Snippet: In vitro Senescent GBM Model via p16 INK4A Overexpression Exhibit Senescence Phenotype. A The protein (upper panel) and mRNA expression levels (lower panel) of p16 INK4A ( CDKN2A ) in SNU201 after transduction with either an empty vector (Empty) or a p16 INK4A -overexpression vector (p16 INK4A ) is shown. kDa: kilodalton. NC: non-transduced SNU201. B The morphology of SNU201 cells post-transduction is depicted in the left panel, with SA-β-Gal staining results in the middle panel and quantification data on the right. C-D Real-time PCR data for representative SASPs and chemokines in SNU201 cells transduced with either vector. E-F IHC analysis for CCL2 and CCL13 in GBM tissues, with quantification data in the lower right panel. Statistical differences in ( A-D ) were analyzed using Student's t-test while those in ( E-F ) were analyzed using the Chi-square test.

Article Snippet: IHC was conducted using the following primary antibodies: p16 INK4A prediluted solution (805–4713; Roche, Tucson, AZ); αSMA, 1:200 (ab5694, Abcam, Cambridge, UK); CD68, 1:2500 (NBP2-48923, Novus Biologicals, Centennial, CO); GFAP, pre-diluted solution (IR524, Dako, Denmark); CD45, 1:1000 (ab8216, Abcam); CD11b, 1:4000 (ab133357, Abcam); CD3, 1:150 (ab135372, Abcam); Cleaved caspase-3, 1:400 (9661S, Cell Signaling Technology, Danvers, MA); CCL2, 1:100 (MAB2791, R&D Systems, Minneapolis, MN); CCL13 1:50 (sc-271124, Santa Cruz Biotechnology, Dallas, TX).

Techniques: In Vitro, Over Expression, Expressing, Transduction, Plasmid Preparation, Staining, Real-time Polymerase Chain Reaction

The SASPs from Senescent GBM Cells Recruit Immune Cells in vitro . A The left panel shows a migration assay schematic, with quantification of migrated cells in the right panel (Empty: CM from empty vector-transduced SNU201; p16 INK4A : CM from p16 INK4A -overexpressed SNU201). B The left panel depicts a migration assay with si CCL2 or si CCL13 treatment in p16 INK4A -overexpressing SNU201, while the right panel shows CDKN2A (p16 INK4A ) mRNA expression levels. I The mRNA expression levels of CCL2 and CCL13 are shown in the left and right panels, respectively. J The left panel shows the number of migrated THP-1 cells with siControl or si CCL2 in p16 INK4A -overexpressed SNU201, and the right panel shows migrated Jurkat cells with siControl or si CCL13 . Statistical differences in ( A and C-D ) were analyzed using Student's t-test. NC: non-treated control; Empty: empty vector-transduced cells; p16 INK4A : p16 INK4A -overexpression vector-transduced cells. All graphs present mean ± standard deviation.

Journal: Neoplasia (New York, N.Y.)

Article Title: High p16 INK4A expression in glioblastoma is associated with senescence phenotype and better prognosis

doi: 10.1016/j.neo.2024.101116

Figure Lengend Snippet: The SASPs from Senescent GBM Cells Recruit Immune Cells in vitro . A The left panel shows a migration assay schematic, with quantification of migrated cells in the right panel (Empty: CM from empty vector-transduced SNU201; p16 INK4A : CM from p16 INK4A -overexpressed SNU201). B The left panel depicts a migration assay with si CCL2 or si CCL13 treatment in p16 INK4A -overexpressing SNU201, while the right panel shows CDKN2A (p16 INK4A ) mRNA expression levels. I The mRNA expression levels of CCL2 and CCL13 are shown in the left and right panels, respectively. J The left panel shows the number of migrated THP-1 cells with siControl or si CCL2 in p16 INK4A -overexpressed SNU201, and the right panel shows migrated Jurkat cells with siControl or si CCL13 . Statistical differences in ( A and C-D ) were analyzed using Student's t-test. NC: non-treated control; Empty: empty vector-transduced cells; p16 INK4A : p16 INK4A -overexpression vector-transduced cells. All graphs present mean ± standard deviation.

Article Snippet: IHC was conducted using the following primary antibodies: p16 INK4A prediluted solution (805–4713; Roche, Tucson, AZ); αSMA, 1:200 (ab5694, Abcam, Cambridge, UK); CD68, 1:2500 (NBP2-48923, Novus Biologicals, Centennial, CO); GFAP, pre-diluted solution (IR524, Dako, Denmark); CD45, 1:1000 (ab8216, Abcam); CD11b, 1:4000 (ab133357, Abcam); CD3, 1:150 (ab135372, Abcam); Cleaved caspase-3, 1:400 (9661S, Cell Signaling Technology, Danvers, MA); CCL2, 1:100 (MAB2791, R&D Systems, Minneapolis, MN); CCL13 1:50 (sc-271124, Santa Cruz Biotechnology, Dallas, TX).

Techniques: In Vitro, Migration, Plasmid Preparation, Expressing, Control, Over Expression, Standard Deviation

The CCL13 expression is related to prognosis of GBM in TCGA dataset. A The survival graphs of GBM based on CCL13 expression (left panel) and CCL2 expression (right panel) are derived from the TCGA GBM-PanCancer dataset. B The schematic image illustrates how the presence of p16 INK4A -high GBM is linked to the tumor immune microenvironment and impacts patient prognosis.

Journal: Neoplasia (New York, N.Y.)

Article Title: High p16 INK4A expression in glioblastoma is associated with senescence phenotype and better prognosis

doi: 10.1016/j.neo.2024.101116

Figure Lengend Snippet: The CCL13 expression is related to prognosis of GBM in TCGA dataset. A The survival graphs of GBM based on CCL13 expression (left panel) and CCL2 expression (right panel) are derived from the TCGA GBM-PanCancer dataset. B The schematic image illustrates how the presence of p16 INK4A -high GBM is linked to the tumor immune microenvironment and impacts patient prognosis.

Article Snippet: IHC was conducted using the following primary antibodies: p16 INK4A prediluted solution (805–4713; Roche, Tucson, AZ); αSMA, 1:200 (ab5694, Abcam, Cambridge, UK); CD68, 1:2500 (NBP2-48923, Novus Biologicals, Centennial, CO); GFAP, pre-diluted solution (IR524, Dako, Denmark); CD45, 1:1000 (ab8216, Abcam); CD11b, 1:4000 (ab133357, Abcam); CD3, 1:150 (ab135372, Abcam); Cleaved caspase-3, 1:400 (9661S, Cell Signaling Technology, Danvers, MA); CCL2, 1:100 (MAB2791, R&D Systems, Minneapolis, MN); CCL13 1:50 (sc-271124, Santa Cruz Biotechnology, Dallas, TX).

Techniques: Expressing, Derivative Assay