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skp2 inhibitor c1 (MedChemExpress)

Name: skp2 inhibitor c1
Brand: MedChemExpress
Rating: 93 (9 reviews)

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MedChemExpress skp2 inhibitor c1

Fig. 4 <t>SKP2</t> is crucial for regulating p27 and AIS. A GSEA analysis of RNA-seq data showing the negative enrichment of the cell-cycle gene signature in ARv7-depleted 22Rv1 cells. B Heat map analysis between two groups of 22Rv1 cells (shctrl or shARv7) shows where expression is high (red) or low (green) for each hallmark cell-cycle gene. C LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for IB. D LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for qRT-PCR analysis. Data represent the average of three independent experiments ± SD. PSA levels were also checked for measuring the efficacy of ADT-mimicking treatment. E LNCaP cells were cultured in CSS medium for different times and then harvested for IB using an antibody against SKP2. F LNCaP and LNCaP-AI cells were harvested for IB and qRT-PCR analysis. G LNCaP cells were pretreated w/o 1 μM SKP2 inhibitor <t>C1</t> for 24 h and then cultured with 10 μg/ml CHX for different times as indicated before being harvested for IB. H LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for the SA-β-gal activity assay. I LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for EdU assay. J LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for FACS analysis

Skp2 Inhibitor C1, supplied by MedChemExpress, used in various techniques. Bioz Stars score: 93/100, based on 9 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 93 stars, based on 9 article reviews

skp2 inhibitor c1 - by Bioz Stars, 2026-02

93/100 stars

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1) Product Images from "ARv7 promotes the escape of prostate cancer cells from androgen deprivation therapy-induced senescence by mediating the SKP2/p27 axis."

Article Title: ARv7 promotes the escape of prostate cancer cells from androgen deprivation therapy-induced senescence by mediating the SKP2/p27 axis.

Journal: BMC biology

doi: 10.1186/s12915-025-02172-4

Fig. 4 SKP2 is crucial for regulating p27 and AIS. A GSEA analysis of RNA-seq data showing the negative enrichment of the cell-cycle gene signature in ARv7-depleted 22Rv1 cells. B Heat map analysis between two groups of 22Rv1 cells (shctrl or shARv7) shows where expression is high (red) or low (green) for each hallmark cell-cycle gene. C LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for IB. D LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for qRT-PCR analysis. Data represent the average of three independent experiments ± SD. PSA levels were also checked for measuring the efficacy of ADT-mimicking treatment. E LNCaP cells were cultured in CSS medium for different times and then harvested for IB using an antibody against SKP2. F LNCaP and LNCaP-AI cells were harvested for IB and qRT-PCR analysis. G LNCaP cells were pretreated w/o 1 μM SKP2 inhibitor C1 for 24 h and then cultured with 10 μg/ml CHX for different times as indicated before being harvested for IB. H LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for the SA-β-gal activity assay. I LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for EdU assay. J LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for FACS analysis

Figure Legend Snippet: Fig. 4 SKP2 is crucial for regulating p27 and AIS. A GSEA analysis of RNA-seq data showing the negative enrichment of the cell-cycle gene signature in ARv7-depleted 22Rv1 cells. B Heat map analysis between two groups of 22Rv1 cells (shctrl or shARv7) shows where expression is high (red) or low (green) for each hallmark cell-cycle gene. C LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for IB. D LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for qRT-PCR analysis. Data represent the average of three independent experiments ± SD. PSA levels were also checked for measuring the efficacy of ADT-mimicking treatment. E LNCaP cells were cultured in CSS medium for different times and then harvested for IB using an antibody against SKP2. F LNCaP and LNCaP-AI cells were harvested for IB and qRT-PCR analysis. G LNCaP cells were pretreated w/o 1 μM SKP2 inhibitor C1 for 24 h and then cultured with 10 μg/ml CHX for different times as indicated before being harvested for IB. H LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for the SA-β-gal activity assay. I LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for EdU assay. J LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for FACS analysis

Techniques Used: RNA Sequencing, Expressing, Quantitative RT-PCR, Cell Culture, Activity Assay, EdU Assay

Fig. 5 ARv7 mediates AIS in an SKP2-dependent manner. A Integrative Genomics Viewer (IGV) image showing the enrichment for the indicated factor at SKP2 and UBE2C in 22Rv1 cells, ATAC-seq data was applied to show the area of open chromatin. B ChIP-qPCR of ARv7 and IgG control at the promoter site in 22Rv1 cells. Data represent the average of three independent experiments ± SD. C HEK293T cells were co-transfected with SKP2 reporter plasmid, Renilla plasmid, and w/o GFP-ARv7 plasmid for 48 h, then cells were subjected to luciferase assay. Relative luciferase activity was calculated after normalized to Renilla luciferase unit. D Stable virus-infected LNCaP cells (vector or ARv7 OE) were harvested for IB. E Stable virus-infected 22Rv1 cells (shctrl or shARv7) were harvested for IB. F Stable virus-infected LNCaP cells (vector or ARv7 OE) were harvested for qRT-PCR analysis. G Stable virus-infected 22Rv1 cells (shctrl or shARv7) were harvested for qRT-PCR analysis. H Upper panel, PC-3 cells were transfected with empty vector or GFP-ARv7 for 48 h and harvested for IB; LNCaP cell lysate was analyzed together as a positive control for AR-FL expression. Lower panel, PC-3 cells were transfected with empty vector or GFP-ARv7 for 48 h and harvested for qRT-PCR analysis. I Stable virus-infected LNCaP cells (vector or ARv7 OE) were treated with normal medium or CSS medium for 7 days then treated w/o 1 μM SKP2 inhibitor C1 for another 24 h before being harvested for EdU assay

Figure Legend Snippet: Fig. 5 ARv7 mediates AIS in an SKP2-dependent manner. A Integrative Genomics Viewer (IGV) image showing the enrichment for the indicated factor at SKP2 and UBE2C in 22Rv1 cells, ATAC-seq data was applied to show the area of open chromatin. B ChIP-qPCR of ARv7 and IgG control at the promoter site in 22Rv1 cells. Data represent the average of three independent experiments ± SD. C HEK293T cells were co-transfected with SKP2 reporter plasmid, Renilla plasmid, and w/o GFP-ARv7 plasmid for 48 h, then cells were subjected to luciferase assay. Relative luciferase activity was calculated after normalized to Renilla luciferase unit. D Stable virus-infected LNCaP cells (vector or ARv7 OE) were harvested for IB. E Stable virus-infected 22Rv1 cells (shctrl or shARv7) were harvested for IB. F Stable virus-infected LNCaP cells (vector or ARv7 OE) were harvested for qRT-PCR analysis. G Stable virus-infected 22Rv1 cells (shctrl or shARv7) were harvested for qRT-PCR analysis. H Upper panel, PC-3 cells were transfected with empty vector or GFP-ARv7 for 48 h and harvested for IB; LNCaP cell lysate was analyzed together as a positive control for AR-FL expression. Lower panel, PC-3 cells were transfected with empty vector or GFP-ARv7 for 48 h and harvested for qRT-PCR analysis. I Stable virus-infected LNCaP cells (vector or ARv7 OE) were treated with normal medium or CSS medium for 7 days then treated w/o 1 μM SKP2 inhibitor C1 for another 24 h before being harvested for EdU assay

Techniques Used: ChIP-qPCR, Control, Transfection, Plasmid Preparation, Luciferase, Activity Assay, Virus, Infection, Quantitative RT-PCR, Positive Control, Expressing, EdU Assay

Fig. 7 SKP2 inhibitor exerts a synergistic effect with ADT in androgen-independent PCa cells. A LNCaP-AI cells were seeded in 6-well plates (2000 cells per well), treated with CSS medium, 50 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. B 22Rv1 cells were seeded in 6-well plates (2000 cells per well), treated with CSS medium, 20 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. C IC50 values of SKP2i C1 and enzalutamide in LNCaP-AI cells. The combination index was calculated and displayed below the table. D LNCaP-AI cells were seeded in 6-well plates (2000 cells per well), treated with 400 nM enzalutamide, 50 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. E 22Rv1 cells were seeded in 6-well plates (2000 cells per well), treated with 800 nM enzalutamide, 20 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. F The proposed model for this study

Figure Legend Snippet: Fig. 7 SKP2 inhibitor exerts a synergistic effect with ADT in androgen-independent PCa cells. A LNCaP-AI cells were seeded in 6-well plates (2000 cells per well), treated with CSS medium, 50 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. B 22Rv1 cells were seeded in 6-well plates (2000 cells per well), treated with CSS medium, 20 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. C IC50 values of SKP2i C1 and enzalutamide in LNCaP-AI cells. The combination index was calculated and displayed below the table. D LNCaP-AI cells were seeded in 6-well plates (2000 cells per well), treated with 400 nM enzalutamide, 50 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. E 22Rv1 cells were seeded in 6-well plates (2000 cells per well), treated with 800 nM enzalutamide, 20 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. F The proposed model for this study

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Journal: BMC biology

Article Title: ARv7 promotes the escape of prostate cancer cells from androgen deprivation therapy-induced senescence by mediating the SKP2/p27 axis.

doi: 10.1186/s12915-025-02172-4

Figure Lengend Snippet: Fig. 4 SKP2 is crucial for regulating p27 and AIS. A GSEA analysis of RNA-seq data showing the negative enrichment of the cell-cycle gene signature in ARv7-depleted 22Rv1 cells. B Heat map analysis between two groups of 22Rv1 cells (shctrl or shARv7) shows where expression is high (red) or low (green) for each hallmark cell-cycle gene. C LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for IB. D LNCaP cells were treated with 10 μM enzalutamide for 72 h or CSS medium for 7 days and then harvested for qRT-PCR analysis. Data represent the average of three independent experiments ± SD. PSA levels were also checked for measuring the efficacy of ADT-mimicking treatment. E LNCaP cells were cultured in CSS medium for different times and then harvested for IB using an antibody against SKP2. F LNCaP and LNCaP-AI cells were harvested for IB and qRT-PCR analysis. G LNCaP cells were pretreated w/o 1 μM SKP2 inhibitor C1 for 24 h and then cultured with 10 μg/ml CHX for different times as indicated before being harvested for IB. H LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for the SA-β-gal activity assay. I LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for EdU assay. J LNCaP cells were treated with 1 μM SKP2 inhibitor C1 for 24 h and then harvested for FACS analysis

Article Snippet: SKP2 inhibitor C1, cycloheximide, MG132, and enzalutamide were purchased from TargetMol (Boston, MA, USA), while puromycin was purchased from MedChemExpress (Monmouth Junction, NJ, USA).

Techniques: RNA Sequencing, Expressing, Quantitative RT-PCR, Cell Culture, Activity Assay, EdU Assay

Journal: BMC biology

Article Title: ARv7 promotes the escape of prostate cancer cells from androgen deprivation therapy-induced senescence by mediating the SKP2/p27 axis.

doi: 10.1186/s12915-025-02172-4

Figure Lengend Snippet: Fig. 5 ARv7 mediates AIS in an SKP2-dependent manner. A Integrative Genomics Viewer (IGV) image showing the enrichment for the indicated factor at SKP2 and UBE2C in 22Rv1 cells, ATAC-seq data was applied to show the area of open chromatin. B ChIP-qPCR of ARv7 and IgG control at the promoter site in 22Rv1 cells. Data represent the average of three independent experiments ± SD. C HEK293T cells were co-transfected with SKP2 reporter plasmid, Renilla plasmid, and w/o GFP-ARv7 plasmid for 48 h, then cells were subjected to luciferase assay. Relative luciferase activity was calculated after normalized to Renilla luciferase unit. D Stable virus-infected LNCaP cells (vector or ARv7 OE) were harvested for IB. E Stable virus-infected 22Rv1 cells (shctrl or shARv7) were harvested for IB. F Stable virus-infected LNCaP cells (vector or ARv7 OE) were harvested for qRT-PCR analysis. G Stable virus-infected 22Rv1 cells (shctrl or shARv7) were harvested for qRT-PCR analysis. H Upper panel, PC-3 cells were transfected with empty vector or GFP-ARv7 for 48 h and harvested for IB; LNCaP cell lysate was analyzed together as a positive control for AR-FL expression. Lower panel, PC-3 cells were transfected with empty vector or GFP-ARv7 for 48 h and harvested for qRT-PCR analysis. I Stable virus-infected LNCaP cells (vector or ARv7 OE) were treated with normal medium or CSS medium for 7 days then treated w/o 1 μM SKP2 inhibitor C1 for another 24 h before being harvested for EdU assay

Techniques: ChIP-qPCR, Control, Transfection, Plasmid Preparation, Luciferase, Activity Assay, Virus, Infection, Quantitative RT-PCR, Positive Control, Expressing, EdU Assay

Journal: BMC biology

Article Title: ARv7 promotes the escape of prostate cancer cells from androgen deprivation therapy-induced senescence by mediating the SKP2/p27 axis.

doi: 10.1186/s12915-025-02172-4

Figure Lengend Snippet: Fig. 7 SKP2 inhibitor exerts a synergistic effect with ADT in androgen-independent PCa cells. A LNCaP-AI cells were seeded in 6-well plates (2000 cells per well), treated with CSS medium, 50 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. B 22Rv1 cells were seeded in 6-well plates (2000 cells per well), treated with CSS medium, 20 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. C IC50 values of SKP2i C1 and enzalutamide in LNCaP-AI cells. The combination index was calculated and displayed below the table. D LNCaP-AI cells were seeded in 6-well plates (2000 cells per well), treated with 400 nM enzalutamide, 50 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. E 22Rv1 cells were seeded in 6-well plates (2000 cells per well), treated with 800 nM enzalutamide, 20 nM SKP2i C1, or both for 14 days, and harvested for colony formation assays. F The proposed model for this study

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