pro collagen type i Search Results


col1  (MedChemExpress)
94
MedChemExpress col1
Biological functional analysis of tri-layer scaffold systems. A) Representative images of migrated cells stained with crystal violet at 48 h. B) Number of migrating cells in control and CE-SKP. C) Glycosaminoglycan concentrations in control and CE-SKP at 7 and 14 days. D) qPCR analysis for COL2, SOX9, and ACAN. E) Western blotting of COL2 and SOX9. F) Alizarin red staining of control and CPH. G) ALP activity of control and CPH. H) qPCR analysis for <t>COL1,</t> COL10, OCN, and RUNX2. I) Western blotting of COL10, COL1, and RUNX2. J) Representative images of migrated cells stained with crystal violet at 48 h. K) Number of migrating cells in control and P2G3. L) Scanning electron microscope micrographs of P2G3. ∗P < 0.05, ∗∗P < 0.01, ∗∗∗P < 0.001.
Col1, supplied by MedChemExpress, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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rat pⅰnp (procollagen ⅰ n-terminal propeptide) elisa kit  (Guangzhou JET Bio-Filtration)
94
Guangzhou JET Bio-Filtration rat pⅰnp (procollagen ⅰ n-terminal propeptide) elisa kit
Biological functional analysis of tri-layer scaffold systems. A) Representative images of migrated cells stained with crystal violet at 48 h. B) Number of migrating cells in control and CE-SKP. C) Glycosaminoglycan concentrations in control and CE-SKP at 7 and 14 days. D) qPCR analysis for COL2, SOX9, and ACAN. E) Western blotting of COL2 and SOX9. F) Alizarin red staining of control and CPH. G) ALP activity of control and CPH. H) qPCR analysis for <t>COL1,</t> COL10, OCN, and RUNX2. I) Western blotting of COL10, COL1, and RUNX2. J) Representative images of migrated cells stained with crystal violet at 48 h. K) Number of migrating cells in control and P2G3. L) Scanning electron microscope micrographs of P2G3. ∗P < 0.05, ∗∗P < 0.01, ∗∗∗P < 0.001.
Rat Pⅰnp (Procollagen ⅰ N Terminal Propeptide) Elisa Kit, supplied by Guangzhou JET Bio-Filtration, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/rat pⅰnp (procollagen ⅰ n-terminal propeptide) elisa kit/product/Guangzhou JET Bio-Filtration
Average 94 stars, based on 1 article reviews
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o c collagen i secretion col1a1  (Boster Bio)
93
Boster Bio o c collagen i secretion col1a1
Study schema. Primary human fibroblast and human keloid fibroblast lines were plated into 96-well plates 1 day before drug treatment. One hundred ninety-nine kinase inhibitors from the HMS LINCS collection were added to replicate 96-well plates. One plate each was placed in 20% oxygen or 1% oxygen incubators concurrently. Twenty-four hours after drug addition, the supernatants were removed and assayed for <t>Col1a1</t> by anti-Col1a1 ELISA, whereas Cell-TiterGo was used to determine viability. The percentage CI for each drug is calculated as the drug COL1A1 levels relative to the average COL1A1 levels from multiple DMSO wells in that specific drug plate (ie, Drug col1a1 ÷ DMSO average col1a1 ) × 100. The percentage viability is defined as the drug viability levels to the average viability from multiple DMSO wells in that specific drug plate (ie, Drug viability ÷ DMSO average viability ) × 100. The CI norm is an approximation of the amount of collagen suppression per cell (ie, divided by viability): (drug col1a1 ÷ DMSO average col1a1 )/(drug viability ÷ DMSO average viability ). The mean normalized CI index (denoted as CI ¯ norm ) is the average of the CI norm from all the cell lines. The most suppressive agent (CGP60474) was then subjected to secondary validation with confocal, dose–response curves, phosphokinome, and western blot analyses. O 2 denotes oxygen. CI, collagen inhibition; CI norm , normalized collagen inhibition index; HMS, Havard Medical School.
O C Collagen I Secretion Col1a1, supplied by Boster Bio, 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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elisa for type i collagen c-terminal pro-peptide (cicp) (technoclone, dorking, uk)  (Technoclone gmbh)
90
Technoclone gmbh elisa for type i collagen c-terminal pro-peptide (cicp) (technoclone, dorking, uk)
Study schema. Primary human fibroblast and human keloid fibroblast lines were plated into 96-well plates 1 day before drug treatment. One hundred ninety-nine kinase inhibitors from the HMS LINCS collection were added to replicate 96-well plates. One plate each was placed in 20% oxygen or 1% oxygen incubators concurrently. Twenty-four hours after drug addition, the supernatants were removed and assayed for <t>Col1a1</t> by anti-Col1a1 ELISA, whereas Cell-TiterGo was used to determine viability. The percentage CI for each drug is calculated as the drug COL1A1 levels relative to the average COL1A1 levels from multiple DMSO wells in that specific drug plate (ie, Drug col1a1 ÷ DMSO average col1a1 ) × 100. The percentage viability is defined as the drug viability levels to the average viability from multiple DMSO wells in that specific drug plate (ie, Drug viability ÷ DMSO average viability ) × 100. The CI norm is an approximation of the amount of collagen suppression per cell (ie, divided by viability): (drug col1a1 ÷ DMSO average col1a1 )/(drug viability ÷ DMSO average viability ). The mean normalized CI index (denoted as CI ¯ norm ) is the average of the CI norm from all the cell lines. The most suppressive agent (CGP60474) was then subjected to secondary validation with confocal, dose–response curves, phosphokinome, and western blot analyses. O 2 denotes oxygen. CI, collagen inhibition; CI norm , normalized collagen inhibition index; HMS, Havard Medical School.
Elisa For Type I Collagen C Terminal Pro Peptide (Cicp) (Technoclone, Dorking, Uk), supplied by Technoclone gmbh, 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/elisa for type i collagen c-terminal pro-peptide (cicp) (technoclone, dorking, uk)/product/Technoclone gmbh
Average 90 stars, based on 1 article reviews
elisa for type i collagen c-terminal pro-peptide (cicp) (technoclone, dorking, uk) - by Bioz Stars, 2026-05
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pro-collagen type i- procol1 antibody  (QED Bioscience)
90
QED Bioscience pro-collagen type i- procol1 antibody
Study schema. Primary human fibroblast and human keloid fibroblast lines were plated into 96-well plates 1 day before drug treatment. One hundred ninety-nine kinase inhibitors from the HMS LINCS collection were added to replicate 96-well plates. One plate each was placed in 20% oxygen or 1% oxygen incubators concurrently. Twenty-four hours after drug addition, the supernatants were removed and assayed for <t>Col1a1</t> by anti-Col1a1 ELISA, whereas Cell-TiterGo was used to determine viability. The percentage CI for each drug is calculated as the drug COL1A1 levels relative to the average COL1A1 levels from multiple DMSO wells in that specific drug plate (ie, Drug col1a1 ÷ DMSO average col1a1 ) × 100. The percentage viability is defined as the drug viability levels to the average viability from multiple DMSO wells in that specific drug plate (ie, Drug viability ÷ DMSO average viability ) × 100. The CI norm is an approximation of the amount of collagen suppression per cell (ie, divided by viability): (drug col1a1 ÷ DMSO average col1a1 )/(drug viability ÷ DMSO average viability ). The mean normalized CI index (denoted as CI ¯ norm ) is the average of the CI norm from all the cell lines. The most suppressive agent (CGP60474) was then subjected to secondary validation with confocal, dose–response curves, phosphokinome, and western blot analyses. O 2 denotes oxygen. CI, collagen inhibition; CI norm , normalized collagen inhibition index; HMS, Havard Medical School.
Pro Collagen Type I Procol1 Antibody, supplied by QED Bioscience, 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/pro-collagen type i- procol1 antibody/product/QED Bioscience
Average 90 stars, based on 1 article reviews
pro-collagen type i- procol1 antibody - by Bioz Stars, 2026-05
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pro-collagen 1 polyclonal antibody  (Bioss)
95
Bioss pro-collagen 1 polyclonal antibody
Study schema. Primary human fibroblast and human keloid fibroblast lines were plated into 96-well plates 1 day before drug treatment. One hundred ninety-nine kinase inhibitors from the HMS LINCS collection were added to replicate 96-well plates. One plate each was placed in 20% oxygen or 1% oxygen incubators concurrently. Twenty-four hours after drug addition, the supernatants were removed and assayed for <t>Col1a1</t> by anti-Col1a1 ELISA, whereas Cell-TiterGo was used to determine viability. The percentage CI for each drug is calculated as the drug COL1A1 levels relative to the average COL1A1 levels from multiple DMSO wells in that specific drug plate (ie, Drug col1a1 ÷ DMSO average col1a1 ) × 100. The percentage viability is defined as the drug viability levels to the average viability from multiple DMSO wells in that specific drug plate (ie, Drug viability ÷ DMSO average viability ) × 100. The CI norm is an approximation of the amount of collagen suppression per cell (ie, divided by viability): (drug col1a1 ÷ DMSO average col1a1 )/(drug viability ÷ DMSO average viability ). The mean normalized CI index (denoted as CI ¯ norm ) is the average of the CI norm from all the cell lines. The most suppressive agent (CGP60474) was then subjected to secondary validation with confocal, dose–response curves, phosphokinome, and western blot analyses. O 2 denotes oxygen. CI, collagen inhibition; CI norm , normalized collagen inhibition index; HMS, Havard Medical School.
Pro Collagen 1 Polyclonal Antibody, supplied by Bioss, 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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Average 95 stars, based on 1 article reviews
pro-collagen 1 polyclonal antibody - by Bioz Stars, 2026-05
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Image Search Results


Biological functional analysis of tri-layer scaffold systems. A) Representative images of migrated cells stained with crystal violet at 48 h. B) Number of migrating cells in control and CE-SKP. C) Glycosaminoglycan concentrations in control and CE-SKP at 7 and 14 days. D) qPCR analysis for COL2, SOX9, and ACAN. E) Western blotting of COL2 and SOX9. F) Alizarin red staining of control and CPH. G) ALP activity of control and CPH. H) qPCR analysis for COL1, COL10, OCN, and RUNX2. I) Western blotting of COL10, COL1, and RUNX2. J) Representative images of migrated cells stained with crystal violet at 48 h. K) Number of migrating cells in control and P2G3. L) Scanning electron microscope micrographs of P2G3. ∗P < 0.05, ∗∗P < 0.01, ∗∗∗P < 0.001.

Journal: Bioactive Materials

Article Title: Bioinspired scaffold recapitulating chondrogenic ontogeny and microenvironment for functional cartilage regeneration

doi: 10.1016/j.bioactmat.2025.11.041

Figure Lengend Snippet: Biological functional analysis of tri-layer scaffold systems. A) Representative images of migrated cells stained with crystal violet at 48 h. B) Number of migrating cells in control and CE-SKP. C) Glycosaminoglycan concentrations in control and CE-SKP at 7 and 14 days. D) qPCR analysis for COL2, SOX9, and ACAN. E) Western blotting of COL2 and SOX9. F) Alizarin red staining of control and CPH. G) ALP activity of control and CPH. H) qPCR analysis for COL1, COL10, OCN, and RUNX2. I) Western blotting of COL10, COL1, and RUNX2. J) Representative images of migrated cells stained with crystal violet at 48 h. K) Number of migrating cells in control and P2G3. L) Scanning electron microscope micrographs of P2G3. ∗P < 0.05, ∗∗P < 0.01, ∗∗∗P < 0.001.

Article Snippet: To evaluate the regeneration of cartilage, COL1 (1:100, HY- P81227 , MCE), COL2 (1:100, ARG20787 , Arigobio), and COL10 (1:100, BA2023, Boster) were used as a marker in immunohistochemistry (IHC) staining.

Techniques: Functional Assay, Staining, Control, Western Blot, Activity Assay, Microscopy

Regeneration of the femoral trochlea in a rabbit model. Representative images of IHC staining for A) COL1, B) COL10.

Journal: Bioactive Materials

Article Title: Bioinspired scaffold recapitulating chondrogenic ontogeny and microenvironment for functional cartilage regeneration

doi: 10.1016/j.bioactmat.2025.11.041

Figure Lengend Snippet: Regeneration of the femoral trochlea in a rabbit model. Representative images of IHC staining for A) COL1, B) COL10.

Article Snippet: To evaluate the regeneration of cartilage, COL1 (1:100, HY- P81227 , MCE), COL2 (1:100, ARG20787 , Arigobio), and COL10 (1:100, BA2023, Boster) were used as a marker in immunohistochemistry (IHC) staining.

Techniques: Immunohistochemistry

Study schema. Primary human fibroblast and human keloid fibroblast lines were plated into 96-well plates 1 day before drug treatment. One hundred ninety-nine kinase inhibitors from the HMS LINCS collection were added to replicate 96-well plates. One plate each was placed in 20% oxygen or 1% oxygen incubators concurrently. Twenty-four hours after drug addition, the supernatants were removed and assayed for Col1a1 by anti-Col1a1 ELISA, whereas Cell-TiterGo was used to determine viability. The percentage CI for each drug is calculated as the drug COL1A1 levels relative to the average COL1A1 levels from multiple DMSO wells in that specific drug plate (ie, Drug col1a1 ÷ DMSO average col1a1 ) × 100. The percentage viability is defined as the drug viability levels to the average viability from multiple DMSO wells in that specific drug plate (ie, Drug viability ÷ DMSO average viability ) × 100. The CI norm is an approximation of the amount of collagen suppression per cell (ie, divided by viability): (drug col1a1 ÷ DMSO average col1a1 )/(drug viability ÷ DMSO average viability ). The mean normalized CI index (denoted as CI ¯ norm ) is the average of the CI norm from all the cell lines. The most suppressive agent (CGP60474) was then subjected to secondary validation with confocal, dose–response curves, phosphokinome, and western blot analyses. O 2 denotes oxygen. CI, collagen inhibition; CI norm , normalized collagen inhibition index; HMS, Havard Medical School.

Journal: JID Innovations

Article Title: Identification of Collagen-Suppressive Agents in Keloidal Fibroblasts Using a High-Content, Phenotype-Based Drug Screen

doi: 10.1016/j.xjidi.2023.100248

Figure Lengend Snippet: Study schema. Primary human fibroblast and human keloid fibroblast lines were plated into 96-well plates 1 day before drug treatment. One hundred ninety-nine kinase inhibitors from the HMS LINCS collection were added to replicate 96-well plates. One plate each was placed in 20% oxygen or 1% oxygen incubators concurrently. Twenty-four hours after drug addition, the supernatants were removed and assayed for Col1a1 by anti-Col1a1 ELISA, whereas Cell-TiterGo was used to determine viability. The percentage CI for each drug is calculated as the drug COL1A1 levels relative to the average COL1A1 levels from multiple DMSO wells in that specific drug plate (ie, Drug col1a1 ÷ DMSO average col1a1 ) × 100. The percentage viability is defined as the drug viability levels to the average viability from multiple DMSO wells in that specific drug plate (ie, Drug viability ÷ DMSO average viability ) × 100. The CI norm is an approximation of the amount of collagen suppression per cell (ie, divided by viability): (drug col1a1 ÷ DMSO average col1a1 )/(drug viability ÷ DMSO average viability ). The mean normalized CI index (denoted as CI ¯ norm ) is the average of the CI norm from all the cell lines. The most suppressive agent (CGP60474) was then subjected to secondary validation with confocal, dose–response curves, phosphokinome, and western blot analyses. O 2 denotes oxygen. CI, collagen inhibition; CI norm , normalized collagen inhibition index; HMS, Havard Medical School.

Article Snippet: After 24 hours of drug treatment, the supernatant was removed and saved at −80 o C. Collagen I secretion (Col1a1) and IL-6 secretion were measured using ELISA after optimization by Human Procollagen I alpha 1/Col1a1 PicoKine ELISA Kit and Human IL-6/Interleukin-6 ELISA Kit PicoKine from Boster Bio (Pleasanton, CA).

Techniques: Enzyme-linked Immunosorbent Assay, Biomarker Discovery, Western Blot, Inhibition

Screen of 199 kinase inhibitors on normal and KFs. ( a ) BJ fibroblasts and 4 KFs were treated with kinase inhibitor drug panel at 1% oxygen. Relative viability was measured with CellTiter-Glo and normalized to DMSO. Extracellular COL1A1 was measured using ELISA and normalized to DMSO. Each blue dot represents the percentage viability (drug viability ÷ DMSO average viability [Y-axis]) graphed against the percentage collagen inhibition (drug col1a1 ÷ DMSO average col1a1 [X-axis]) for a single drug. The experiment was replicated 5 times each using a different cell line once. ( b ) The mean CI norm ( CI ¯ norm ; ie, the average CI norm for BJ, KF1, KF4, KF5, and KF6; orange line) is ranked from most suppressive (left side) to most inductive (right side). The SDs for each drug across the 5 biological replicates (ie, the 5 cell lines) are shown as blue bars. ( c ) Table showing the top 10 most COL1A1-suppressive and collagen-inducive drugs ranked by CI ¯ norm . Akt, protein kinase B; KF, keloid fibroblast; MET, MAPK/extracellular signal–regulated kinase; PI3K, phosphoinositide 3-kinase.

Journal: JID Innovations

Article Title: Identification of Collagen-Suppressive Agents in Keloidal Fibroblasts Using a High-Content, Phenotype-Based Drug Screen

doi: 10.1016/j.xjidi.2023.100248

Figure Lengend Snippet: Screen of 199 kinase inhibitors on normal and KFs. ( a ) BJ fibroblasts and 4 KFs were treated with kinase inhibitor drug panel at 1% oxygen. Relative viability was measured with CellTiter-Glo and normalized to DMSO. Extracellular COL1A1 was measured using ELISA and normalized to DMSO. Each blue dot represents the percentage viability (drug viability ÷ DMSO average viability [Y-axis]) graphed against the percentage collagen inhibition (drug col1a1 ÷ DMSO average col1a1 [X-axis]) for a single drug. The experiment was replicated 5 times each using a different cell line once. ( b ) The mean CI norm ( CI ¯ norm ; ie, the average CI norm for BJ, KF1, KF4, KF5, and KF6; orange line) is ranked from most suppressive (left side) to most inductive (right side). The SDs for each drug across the 5 biological replicates (ie, the 5 cell lines) are shown as blue bars. ( c ) Table showing the top 10 most COL1A1-suppressive and collagen-inducive drugs ranked by CI ¯ norm . Akt, protein kinase B; KF, keloid fibroblast; MET, MAPK/extracellular signal–regulated kinase; PI3K, phosphoinositide 3-kinase.

Article Snippet: After 24 hours of drug treatment, the supernatant was removed and saved at −80 o C. Collagen I secretion (Col1a1) and IL-6 secretion were measured using ELISA after optimization by Human Procollagen I alpha 1/Col1a1 PicoKine ELISA Kit and Human IL-6/Interleukin-6 ELISA Kit PicoKine from Boster Bio (Pleasanton, CA).

Techniques: Enzyme-linked Immunosorbent Assay, Inhibition

Cellular screen for CGP60474. ( a ) Confocal microscopy shows loss of intracellular COL1A1 (green) in the BJ fibroblast and 5 KF lines after exposure to 1 μM CGP60474 for 24 hrs. DAPI stain is shown in blue. Bar = 20 μm ( b ) Dose–response curves for CGP60474 in 2 KF lines showing normalized (to DMSO) viability and extracellular COL1A1. ( c ) Effect of 1 μM CGP60474 on both Col1a1 and Col7a1 in KF-1762, KF1, KF4, and KF6 showing suppression of both collagens. hr, hour; KF, keloid fibroblast.

Journal: JID Innovations

Article Title: Identification of Collagen-Suppressive Agents in Keloidal Fibroblasts Using a High-Content, Phenotype-Based Drug Screen

doi: 10.1016/j.xjidi.2023.100248

Figure Lengend Snippet: Cellular screen for CGP60474. ( a ) Confocal microscopy shows loss of intracellular COL1A1 (green) in the BJ fibroblast and 5 KF lines after exposure to 1 μM CGP60474 for 24 hrs. DAPI stain is shown in blue. Bar = 20 μm ( b ) Dose–response curves for CGP60474 in 2 KF lines showing normalized (to DMSO) viability and extracellular COL1A1. ( c ) Effect of 1 μM CGP60474 on both Col1a1 and Col7a1 in KF-1762, KF1, KF4, and KF6 showing suppression of both collagens. hr, hour; KF, keloid fibroblast.

Article Snippet: After 24 hours of drug treatment, the supernatant was removed and saved at −80 o C. Collagen I secretion (Col1a1) and IL-6 secretion were measured using ELISA after optimization by Human Procollagen I alpha 1/Col1a1 PicoKine ELISA Kit and Human IL-6/Interleukin-6 ELISA Kit PicoKine from Boster Bio (Pleasanton, CA).

Techniques: Confocal Microscopy, Staining

CGP60474 and MAPK signaling. ( a ) Representative phosphokinome array for KF-1762 (Proteome Profiler—Human Phospho-Kinase Array—(R&D Systems, ARY003C) showing most upregulated phosphoproteins (p-Erk T202/Y204,T185/Y187 , p-Hsp27 S78/S82 , p-Gsk-3α/β S21/S9 ). ( b ) Normalized (to background) and relative (to DMSO) densitometry units for the p-Erk T202/Y204,T185/Y187 , p-Hsp27 S78/S82 , and p-Gsk-3α/β S21/S9 based on 3 independent phosphokinome arrays. ( c ) Western blots showing levels of COL1A1, p-ERK, total ERK, and GAPDH in KF-1762 and KF5 at 20 and 1% oxygen. ERK, extracellular signal–regulated kinase; KF, keloid fibroblast; p-ERK, phosphorylated extracellular signal–regulated kinase; p-Gsk, phosphorylated Gsk; p-Hsp27, phosphorylated Hsp27.

Journal: JID Innovations

Article Title: Identification of Collagen-Suppressive Agents in Keloidal Fibroblasts Using a High-Content, Phenotype-Based Drug Screen

doi: 10.1016/j.xjidi.2023.100248

Figure Lengend Snippet: CGP60474 and MAPK signaling. ( a ) Representative phosphokinome array for KF-1762 (Proteome Profiler—Human Phospho-Kinase Array—(R&D Systems, ARY003C) showing most upregulated phosphoproteins (p-Erk T202/Y204,T185/Y187 , p-Hsp27 S78/S82 , p-Gsk-3α/β S21/S9 ). ( b ) Normalized (to background) and relative (to DMSO) densitometry units for the p-Erk T202/Y204,T185/Y187 , p-Hsp27 S78/S82 , and p-Gsk-3α/β S21/S9 based on 3 independent phosphokinome arrays. ( c ) Western blots showing levels of COL1A1, p-ERK, total ERK, and GAPDH in KF-1762 and KF5 at 20 and 1% oxygen. ERK, extracellular signal–regulated kinase; KF, keloid fibroblast; p-ERK, phosphorylated extracellular signal–regulated kinase; p-Gsk, phosphorylated Gsk; p-Hsp27, phosphorylated Hsp27.

Article Snippet: After 24 hours of drug treatment, the supernatant was removed and saved at −80 o C. Collagen I secretion (Col1a1) and IL-6 secretion were measured using ELISA after optimization by Human Procollagen I alpha 1/Col1a1 PicoKine ELISA Kit and Human IL-6/Interleukin-6 ELISA Kit PicoKine from Boster Bio (Pleasanton, CA).

Techniques: Western Blot

CGP60474 and IL-6. ( a ) Various primary KFs (different color circles) were treated with 1 and 3 μM CGP60474 for 24 hrs in either 20 oxygen or 1% oxygen (raw data are in <xref ref-type=Supplementary Table S5 ). Levels of secreted IL-6 (pg/ml) were assayed by ELISA (human IL-6/IL-6 ELISA Kit PicoKine). Except for KF4, in general, there were decreases in secreted IL-6. ( b ) Effect of adding IL-6 (100 nM) and anti–IL-6R (3 μg) on COL1A1, p-ERK, and total ERK in KF6. Erk, extracellular signal–regulated kinase; hr, hour; IL-6R, IL-6 receptor; KF, keloid fibroblast; p-Erk, phosphorylated extracellular signal–regulated kinase; RLU, Relative Luminescence Units. " width="100%" height="100%">

Journal: JID Innovations

Article Title: Identification of Collagen-Suppressive Agents in Keloidal Fibroblasts Using a High-Content, Phenotype-Based Drug Screen

doi: 10.1016/j.xjidi.2023.100248

Figure Lengend Snippet: CGP60474 and IL-6. ( a ) Various primary KFs (different color circles) were treated with 1 and 3 μM CGP60474 for 24 hrs in either 20 oxygen or 1% oxygen (raw data are in Supplementary Table S5 ). Levels of secreted IL-6 (pg/ml) were assayed by ELISA (human IL-6/IL-6 ELISA Kit PicoKine). Except for KF4, in general, there were decreases in secreted IL-6. ( b ) Effect of adding IL-6 (100 nM) and anti–IL-6R (3 μg) on COL1A1, p-ERK, and total ERK in KF6. Erk, extracellular signal–regulated kinase; hr, hour; IL-6R, IL-6 receptor; KF, keloid fibroblast; p-Erk, phosphorylated extracellular signal–regulated kinase; RLU, Relative Luminescence Units.

Article Snippet: After 24 hours of drug treatment, the supernatant was removed and saved at −80 o C. Collagen I secretion (Col1a1) and IL-6 secretion were measured using ELISA after optimization by Human Procollagen I alpha 1/Col1a1 PicoKine ELISA Kit and Human IL-6/Interleukin-6 ELISA Kit PicoKine from Boster Bio (Pleasanton, CA).

Techniques: Enzyme-linked Immunosorbent Assay