control sirnas  (OriGene)


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    OriGene control sirnas
    Control Sirnas, supplied by OriGene, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    cyclin d1 ccnd1 sirnas  (Thermo Fisher)


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    Thermo Fisher cyclin d1 ccnd1 sirnas
    Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), <t>cyclin</t> <t>D1</t> <t>[CCND1;</t> (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.
    Cyclin D1 Ccnd1 Sirnas, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    1) Product Images from "Survivin as a mediator of stiffness-induced cell cycle progression and proliferation of vascular smooth muscle cells"

    Article Title: Survivin as a mediator of stiffness-induced cell cycle progression and proliferation of vascular smooth muscle cells

    Journal: APL Bioengineering

    doi: 10.1063/5.0150532

    Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), cyclin D1 [CCND1; (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.
    Figure Legend Snippet: Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), cyclin D1 [CCND1; (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.

    Techniques Used: Transfection, Quantitative RT-PCR, Western Blot, Expressing, Over Expression, Cell Counting, Infection

    Survivin is an upstream regulator of stiffness-induced cell cycle progression. (a) and (b) hVSMCs were transfected with control siRNA or siRNAs to cyclin D1, synchronized to G 0 via serum starvation, and plated on stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR to determine mRNA levels of cyclin D1 (CCND1) (a) and survivin (b). Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 3, independent experiments. (c) G 0 -synchronized hVSMCs were treated with either 5 or 30 μ M mitomycin C (MMC) and then cultured on soft or stiff hydrogels for 24 h. Survivin induction was analyzed by immunoblotting. Survivin protein levels were normalized to those in hVSMCs treated with DMSO on stiff hydrogels (d). n = 4–8, independent experiments.
    Figure Legend Snippet: Survivin is an upstream regulator of stiffness-induced cell cycle progression. (a) and (b) hVSMCs were transfected with control siRNA or siRNAs to cyclin D1, synchronized to G 0 via serum starvation, and plated on stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR to determine mRNA levels of cyclin D1 (CCND1) (a) and survivin (b). Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 3, independent experiments. (c) G 0 -synchronized hVSMCs were treated with either 5 or 30 μ M mitomycin C (MMC) and then cultured on soft or stiff hydrogels for 24 h. Survivin induction was analyzed by immunoblotting. Survivin protein levels were normalized to those in hVSMCs treated with DMSO on stiff hydrogels (d). n = 4–8, independent experiments.

    Techniques Used: Transfection, Quantitative RT-PCR, Expressing, Cell Culture, Western Blot


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    Santa Cruz Biotechnology ccnd1 sirna
    Ccnd1 Sirna, supplied by Santa Cruz 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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    Bioneer Corporation cyclin d1 ccnd1 sirna
    Cyclin D1 Ccnd1 Sirna, supplied by Bioneer Corporation, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/cyclin d1 ccnd1 sirna/product/Bioneer Corporation
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    control sirnas  (OriGene)


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    OriGene control sirnas
    Control Sirnas, supplied by OriGene, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    cyclin d1 no sr300410 genes  (OriGene)


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    OriGene cyclin d1 no sr300410 genes
    Cyclin D1 No Sr300410 Genes, supplied by OriGene, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    sirnas  (OriGene)


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    OriGene sirnas
    Sirnas, supplied by OriGene, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    cyclin d1  (OriGene)


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    OriGene cyclin d1
    Cyclin D1, supplied by OriGene, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Santa Cruz Biotechnology ccnd1 sirna
    Ccnd1 Sirna, supplied by Santa Cruz 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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    ccnd1 sirna  (OriGene)


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    OriGene ccnd1 sirna
    MYF5 target transcripts include mRNAs that encode proteins involved in myoblast proliferation and differentiation. ( A ) RIP assay using cytoplasmic lysates prepared from C2C12 cells using either anti-MYF5 antibody or IgG under conditions that preserved mRNA-RBP (mRNP) complexes. ( B ) Western blot analysis of MYF5 recovered in IP samples. ( C ) Following MYF5 RIP, MYF5-bound mRNAs were identified by microarray (RIP-chip) analysis in growing (GM) C2C12 cells. Data represent the Z -ratio of mRNAs in MYF5 RIP relative to IgG RIP. ( D ) RIP followed by RT-qPCR analysis to validate the association of MYF5 with mRNAs encoding myogenic proteins in proliferating C2C12 myoblasts; the levels of mRNAs in MYF5 IP were normalized to the levels of Gapdh mRNA and plotted as fold enrichment relative to the levels seen in control IgG IP samples. Discontinuous gray line: twofold enrichment in mRNAs bound to MYF5. ( E ) RIP analysis of Flag-MYF5 interaction with <t>Ccnd1</t> mRNA. Forty-eight hours after C2C12 transfection with Flag-MYF5, RIP analysis was carried out using IgG or anti-Flag antibodies. Ccnd1 mRNA was detected by RT-qPCR analysis and its levels in Flag IP were compared with those in control IgG IP samples; Actn mRNA (encoding the housekeeping protein β-Actin) was measured to normalize sample input. Data in (D,E) represent the means and S.E.M. from three or more independent experiments. ( F ) Ingenuity pathway analysis (IPA) of mRNAs enriched in MYF5 IP relative to IgG in C2C12 growing myoblasts. *, P < 0.05 and **, P < 0.01 (Student's t -test).
    Ccnd1 Sirna, supplied by OriGene, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    1) Product Images from "Novel RNA-binding activity of MYF5 enhances Ccnd1 / Cyclin D1 mRNA translation during myogenesis"

    Article Title: Novel RNA-binding activity of MYF5 enhances Ccnd1 / Cyclin D1 mRNA translation during myogenesis

    Journal: Nucleic Acids Research

    doi: 10.1093/nar/gkw023

    MYF5 target transcripts include mRNAs that encode proteins involved in myoblast proliferation and differentiation. ( A ) RIP assay using cytoplasmic lysates prepared from C2C12 cells using either anti-MYF5 antibody or IgG under conditions that preserved mRNA-RBP (mRNP) complexes. ( B ) Western blot analysis of MYF5 recovered in IP samples. ( C ) Following MYF5 RIP, MYF5-bound mRNAs were identified by microarray (RIP-chip) analysis in growing (GM) C2C12 cells. Data represent the Z -ratio of mRNAs in MYF5 RIP relative to IgG RIP. ( D ) RIP followed by RT-qPCR analysis to validate the association of MYF5 with mRNAs encoding myogenic proteins in proliferating C2C12 myoblasts; the levels of mRNAs in MYF5 IP were normalized to the levels of Gapdh mRNA and plotted as fold enrichment relative to the levels seen in control IgG IP samples. Discontinuous gray line: twofold enrichment in mRNAs bound to MYF5. ( E ) RIP analysis of Flag-MYF5 interaction with Ccnd1 mRNA. Forty-eight hours after C2C12 transfection with Flag-MYF5, RIP analysis was carried out using IgG or anti-Flag antibodies. Ccnd1 mRNA was detected by RT-qPCR analysis and its levels in Flag IP were compared with those in control IgG IP samples; Actn mRNA (encoding the housekeeping protein β-Actin) was measured to normalize sample input. Data in (D,E) represent the means and S.E.M. from three or more independent experiments. ( F ) Ingenuity pathway analysis (IPA) of mRNAs enriched in MYF5 IP relative to IgG in C2C12 growing myoblasts. *, P < 0.05 and **, P < 0.01 (Student's t -test).
    Figure Legend Snippet: MYF5 target transcripts include mRNAs that encode proteins involved in myoblast proliferation and differentiation. ( A ) RIP assay using cytoplasmic lysates prepared from C2C12 cells using either anti-MYF5 antibody or IgG under conditions that preserved mRNA-RBP (mRNP) complexes. ( B ) Western blot analysis of MYF5 recovered in IP samples. ( C ) Following MYF5 RIP, MYF5-bound mRNAs were identified by microarray (RIP-chip) analysis in growing (GM) C2C12 cells. Data represent the Z -ratio of mRNAs in MYF5 RIP relative to IgG RIP. ( D ) RIP followed by RT-qPCR analysis to validate the association of MYF5 with mRNAs encoding myogenic proteins in proliferating C2C12 myoblasts; the levels of mRNAs in MYF5 IP were normalized to the levels of Gapdh mRNA and plotted as fold enrichment relative to the levels seen in control IgG IP samples. Discontinuous gray line: twofold enrichment in mRNAs bound to MYF5. ( E ) RIP analysis of Flag-MYF5 interaction with Ccnd1 mRNA. Forty-eight hours after C2C12 transfection with Flag-MYF5, RIP analysis was carried out using IgG or anti-Flag antibodies. Ccnd1 mRNA was detected by RT-qPCR analysis and its levels in Flag IP were compared with those in control IgG IP samples; Actn mRNA (encoding the housekeeping protein β-Actin) was measured to normalize sample input. Data in (D,E) represent the means and S.E.M. from three or more independent experiments. ( F ) Ingenuity pathway analysis (IPA) of mRNAs enriched in MYF5 IP relative to IgG in C2C12 growing myoblasts. *, P < 0.05 and **, P < 0.01 (Student's t -test).

    Techniques Used: Western Blot, Microarray, Quantitative RT-PCR, Transfection

    MYF5 binds to specific sequences on the Ccnd1 mRNA. (A) Top , schematic showing biotinylated RNA fragments spanning the 5′UTR, coding region (CR), and 3′UTR of Ccnd1 mRNA used for pulldown. Bottom , biotinylated RNA fragments were incubated with cytoplasmic lysates from C2C12 cells (GM); after pulldown using streptavidin beads, the levels of MYF5 bound to the biotinylated RNA segments were detected by western blot analysis. (B) Recombinant purified His-MYF5 was incubated with biotinylated Ccnd1 RNA fragments followed by pulldown and detection of MYF5 by western blot analysis using anti-MYF5 antibody. (C) Schematic of biotinylated RNA fragments spanning the Ccnd1 3′UTR-C transcript ( top ), were tested for binding to His-MYF5 after pull-down using streptavidin beads; His-MYF5 interaction with RNA segments of fragment C ( middle ) and smaller RNAs after closer subdivision of fragments 9 through 11 ( bottom ) were assessed by western blot analysis using anti-MYF5 antibody. (D) GST or GST-MYF5 were incubated with radiolabeled Ccnd1 3′UTR-C10–1, then either resolved on native acrylamide gels ( left ) by RNA electrophoretic mobility shift assay (EMSA), or crosslinked by UV irradiation and resolved by SDS-PAGE ( right ). (E) The domain of MYF5 that interacts with the Ccnd1 3′-C fragment was mapped by creating GST-tagged truncations of MYF5 ( left ) and testing their interaction by biotin pulldown and western blot analysis using anti-GST antibody ( right ).
    Figure Legend Snippet: MYF5 binds to specific sequences on the Ccnd1 mRNA. (A) Top , schematic showing biotinylated RNA fragments spanning the 5′UTR, coding region (CR), and 3′UTR of Ccnd1 mRNA used for pulldown. Bottom , biotinylated RNA fragments were incubated with cytoplasmic lysates from C2C12 cells (GM); after pulldown using streptavidin beads, the levels of MYF5 bound to the biotinylated RNA segments were detected by western blot analysis. (B) Recombinant purified His-MYF5 was incubated with biotinylated Ccnd1 RNA fragments followed by pulldown and detection of MYF5 by western blot analysis using anti-MYF5 antibody. (C) Schematic of biotinylated RNA fragments spanning the Ccnd1 3′UTR-C transcript ( top ), were tested for binding to His-MYF5 after pull-down using streptavidin beads; His-MYF5 interaction with RNA segments of fragment C ( middle ) and smaller RNAs after closer subdivision of fragments 9 through 11 ( bottom ) were assessed by western blot analysis using anti-MYF5 antibody. (D) GST or GST-MYF5 were incubated with radiolabeled Ccnd1 3′UTR-C10–1, then either resolved on native acrylamide gels ( left ) by RNA electrophoretic mobility shift assay (EMSA), or crosslinked by UV irradiation and resolved by SDS-PAGE ( right ). (E) The domain of MYF5 that interacts with the Ccnd1 3′-C fragment was mapped by creating GST-tagged truncations of MYF5 ( left ) and testing their interaction by biotin pulldown and western blot analysis using anti-GST antibody ( right ).

    Techniques Used: Incubation, Western Blot, Recombinant, Purification, Binding Assay, Electrophoretic Mobility Shift Assay, Irradiation, SDS Page

    MYF5 regulates CCND1 expression in C2C12 myoblasts. (A) Western blot analysis of MYF5 and CCND1 expression during C2C12 differentiation; heat shock protein 90 (HSP90) was included as loading control. (B,C) Forty-eight hours after transfecting C2C12 cells with MYF5 siRNA or Ctrl siRNA, the levels of MYF5, CCND1 and loading control GAPDH were analyzed by western blot analysis (B) and the levels of Ccnd1 pre-mRNA and mRNA by RT-qPCR analysis (C). (D–F) Forty-eight hours after transfection of proliferating C2C12 myoblasts with Ctrl or CCND1 siRNAs, the levels of CCND1 and HSP90 were assessed by western blot analysis (D) and cell numbers were measured using a TC10 automated cell counter (BioRad) and represented as fold change in cell number after CCND1 silencing relative to those in the Ctrl siRNA group (E). At day 6 in differentiation medium (DM6) C2C12 differentiation was monitored by measuring creatine kinase activity (F). (G) Forty-eight hours after MYF5 was overexpressed using pFlag-MYF5 pcDNA3, the levels of MYF5, CCND1 and loading control HSP90 were studied by western blot analysis. Data in (B-F) represent the means and S.E.M. from three or four independent experiments. *, P < 0.05 and **, P < 0.01 (Student's t -test).
    Figure Legend Snippet: MYF5 regulates CCND1 expression in C2C12 myoblasts. (A) Western blot analysis of MYF5 and CCND1 expression during C2C12 differentiation; heat shock protein 90 (HSP90) was included as loading control. (B,C) Forty-eight hours after transfecting C2C12 cells with MYF5 siRNA or Ctrl siRNA, the levels of MYF5, CCND1 and loading control GAPDH were analyzed by western blot analysis (B) and the levels of Ccnd1 pre-mRNA and mRNA by RT-qPCR analysis (C). (D–F) Forty-eight hours after transfection of proliferating C2C12 myoblasts with Ctrl or CCND1 siRNAs, the levels of CCND1 and HSP90 were assessed by western blot analysis (D) and cell numbers were measured using a TC10 automated cell counter (BioRad) and represented as fold change in cell number after CCND1 silencing relative to those in the Ctrl siRNA group (E). At day 6 in differentiation medium (DM6) C2C12 differentiation was monitored by measuring creatine kinase activity (F). (G) Forty-eight hours after MYF5 was overexpressed using pFlag-MYF5 pcDNA3, the levels of MYF5, CCND1 and loading control HSP90 were studied by western blot analysis. Data in (B-F) represent the means and S.E.M. from three or four independent experiments. *, P < 0.05 and **, P < 0.01 (Student's t -test).

    Techniques Used: Expressing, Western Blot, Quantitative RT-PCR, Transfection, Activity Assay

    MYF5 promotes translation of Ccnd1 mRNA. (A,B) Forty-eight hours after Ctrl or MYF5 siRNA transfection of C2C12 cells, cytoplasmic extracts were fractionated through sucrose gradients to obtain cytoplasmic components of progressively larger weight: ribosomal subunits (40S, 60S), monosomes (80S) and low-molecular-weight (LMW) and high-molecular-weight (HMW) polysomes (A). The relative distribution of Gapdh mRNA, encoding a housekeeping protein, and Ccnd1 mRNA were measured by RT-qPCR analysis of RNA in each of the gradient fractions and represented as percentage of total RNA in the gradient (B). (C) Schematic of the dual luciferase reporter plasmids derived from the parent vector psiCHECK2 (psi), which expresses renilla luciferase (RL) and the internal control firefly luciferase (FL), and psiCHECK2-derived plasmids bearing the Ccnd1 fragments downstream of the RL coding region. (D) Top , Influence of MYF5 silencing on the expression of the reporter constructs. Twenty-four h after transfection of C2C12 cells with either MYF5 siRNA or Ctrl siRNA, each reporter plasmid was transfected, and 16 h later the ratio of RL activity to FL activity was measured. The decrease in relative RL/FL ratio of MYF5 siRNA-transfected cells relative to the RL/FL ratio of Ctrl siRNA-transfected cells is indicated. Bottom , RT-qPCR analysis of RL mRNA levels normalized to FL mRNA levels in each transfection group. Data represent the means and S.E.M. from 3 independent experiments. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).
    Figure Legend Snippet: MYF5 promotes translation of Ccnd1 mRNA. (A,B) Forty-eight hours after Ctrl or MYF5 siRNA transfection of C2C12 cells, cytoplasmic extracts were fractionated through sucrose gradients to obtain cytoplasmic components of progressively larger weight: ribosomal subunits (40S, 60S), monosomes (80S) and low-molecular-weight (LMW) and high-molecular-weight (HMW) polysomes (A). The relative distribution of Gapdh mRNA, encoding a housekeeping protein, and Ccnd1 mRNA were measured by RT-qPCR analysis of RNA in each of the gradient fractions and represented as percentage of total RNA in the gradient (B). (C) Schematic of the dual luciferase reporter plasmids derived from the parent vector psiCHECK2 (psi), which expresses renilla luciferase (RL) and the internal control firefly luciferase (FL), and psiCHECK2-derived plasmids bearing the Ccnd1 fragments downstream of the RL coding region. (D) Top , Influence of MYF5 silencing on the expression of the reporter constructs. Twenty-four h after transfection of C2C12 cells with either MYF5 siRNA or Ctrl siRNA, each reporter plasmid was transfected, and 16 h later the ratio of RL activity to FL activity was measured. The decrease in relative RL/FL ratio of MYF5 siRNA-transfected cells relative to the RL/FL ratio of Ctrl siRNA-transfected cells is indicated. Bottom , RT-qPCR analysis of RL mRNA levels normalized to FL mRNA levels in each transfection group. Data represent the means and S.E.M. from 3 independent experiments. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).

    Techniques Used: Transfection, Molecular Weight, Quantitative RT-PCR, Luciferase, Derivative Assay, Plasmid Preparation, Expressing, Construct, Activity Assay

    Influence of MYF5 on myogenesis via regulation of CCND1 expression. (A,B) C2C12 cells were transfected with MYF5 siRNA or Ctrl siRNA, along with a control vector [pcDNA3-Flag (pV)] or a plasmid vector that expressed Myc-tagged CCND1. Forty-eight hours later, the levels of CCND1 and MYF5 were analyzed by western blot analysis (A) and the degree of differentiation was analyzed by measuring creatine kinase activity at day 6 into differentiation (B). Data presented are the means and S.E.M. from four independent experiments; significance (P) is indicated. (C) Proposed model whereby MYF5 modulates myogenesis by acting upon CCND1 expression on two levels: first, MYF5 activates Ccnd1 transcription moderately, and second, MYF5 binds the Ccnd1 mRNA at the CR and 3′UTR, promoting Ccnd1 mRNA translation. The net effect is a CCND1-mediated increase in myoblast proliferation necessary at the initiation of myogenesis. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).
    Figure Legend Snippet: Influence of MYF5 on myogenesis via regulation of CCND1 expression. (A,B) C2C12 cells were transfected with MYF5 siRNA or Ctrl siRNA, along with a control vector [pcDNA3-Flag (pV)] or a plasmid vector that expressed Myc-tagged CCND1. Forty-eight hours later, the levels of CCND1 and MYF5 were analyzed by western blot analysis (A) and the degree of differentiation was analyzed by measuring creatine kinase activity at day 6 into differentiation (B). Data presented are the means and S.E.M. from four independent experiments; significance (P) is indicated. (C) Proposed model whereby MYF5 modulates myogenesis by acting upon CCND1 expression on two levels: first, MYF5 activates Ccnd1 transcription moderately, and second, MYF5 binds the Ccnd1 mRNA at the CR and 3′UTR, promoting Ccnd1 mRNA translation. The net effect is a CCND1-mediated increase in myoblast proliferation necessary at the initiation of myogenesis. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).

    Techniques Used: Expressing, Transfection, Plasmid Preparation, Western Blot, Activity Assay

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    OriGene control sirnas
    Control Sirnas, supplied by OriGene, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), <t>cyclin</t> <t>D1</t> <t>[CCND1;</t> (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.
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    Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), <t>cyclin</t> <t>D1</t> <t>[CCND1;</t> (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.
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    Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), <t>cyclin</t> <t>D1</t> <t>[CCND1;</t> (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.
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    MYF5 target transcripts include mRNAs that encode proteins involved in myoblast proliferation and differentiation. ( A ) RIP assay using cytoplasmic lysates prepared from C2C12 cells using either anti-MYF5 antibody or IgG under conditions that preserved mRNA-RBP (mRNP) complexes. ( B ) Western blot analysis of MYF5 recovered in IP samples. ( C ) Following MYF5 RIP, MYF5-bound mRNAs were identified by microarray (RIP-chip) analysis in growing (GM) C2C12 cells. Data represent the Z -ratio of mRNAs in MYF5 RIP relative to IgG RIP. ( D ) RIP followed by RT-qPCR analysis to validate the association of MYF5 with mRNAs encoding myogenic proteins in proliferating C2C12 myoblasts; the levels of mRNAs in MYF5 IP were normalized to the levels of Gapdh mRNA and plotted as fold enrichment relative to the levels seen in control IgG IP samples. Discontinuous gray line: twofold enrichment in mRNAs bound to MYF5. ( E ) RIP analysis of Flag-MYF5 interaction with <t>Ccnd1</t> mRNA. Forty-eight hours after C2C12 transfection with Flag-MYF5, RIP analysis was carried out using IgG or anti-Flag antibodies. Ccnd1 mRNA was detected by RT-qPCR analysis and its levels in Flag IP were compared with those in control IgG IP samples; Actn mRNA (encoding the housekeeping protein β-Actin) was measured to normalize sample input. Data in (D,E) represent the means and S.E.M. from three or more independent experiments. ( F ) Ingenuity pathway analysis (IPA) of mRNAs enriched in MYF5 IP relative to IgG in C2C12 growing myoblasts. *, P < 0.05 and **, P < 0.01 (Student's t -test).
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    Image Search Results


    Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), cyclin D1 [CCND1; (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.

    Journal: APL Bioengineering

    Article Title: Survivin as a mediator of stiffness-induced cell cycle progression and proliferation of vascular smooth muscle cells

    doi: 10.1063/5.0150532

    Figure Lengend Snippet: Survivin is required for stiffness-mediated cell cycle progression and proliferation. (a)–(g) hVSMCs were transfected with control siRNA or siRNAs to survivin [#1 and #2], synchronized to G 0 via serum starvation, and plated on soft or stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR (a)–(c) or immunoblotting (d)–(g) to determine mRNA and protein levels of survivin (a) and (e), cyclin D1 [CCND1; (b) and (f)], and cyclin A [CCNA; (c) and (g)]. Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 4 (a), n = 3 (b), n = 3 (c), n = 5 (e), n = 3 (f), and n = 5 (g), independent experiments. S-phase entry and cell proliferation with survivin knockdown (h)–(i) and overexpression (j)–(k) were assessed by EdU incorporation (h) and (j) and cell counting (i) and (k), respectively, and normalized to values from hVSMCs treated with control siRNA on stiff hydrogels (h)–(i) or infected with GFP adenovirus (Adv) on soft hydrogels ( j)–(k). n = 5 (h), n = 3 (i), n = 4 (j), and n = 4 (k), independent experiments. Data are means + SEMs. * p < 0.05, ** p < 0.01, and *** p < 0.001.

    Article Snippet: The following survivin ( BIRC5 ), FAK ( PTK2 ), and cyclin D1 ( CCND1 ) siRNAs were obtained from Ambion: survivin siRNA #1 (ID no. 121294), 5′-CCACUUCCAGGGUUUAUUCtt-3′; survivin siRNA #2 (ID no. 121295), 5′-GCCAUUCUAAGUCAUUGGGtt-3′; FAK siRNA #1 (ID no. 157448), 5′-CCUAGCAGACUUUAACCAAtt-3′; FAK siRNA #2 (ID no. 61352), 5′-GGCAUGGAGAUGCUACUGAtt-3′; and cyclin D1 siRNA (ID no. 42828), 5′-GGAGAACAAACAGAUCAUCtt-3′.

    Techniques: Transfection, Quantitative RT-PCR, Western Blot, Expressing, Over Expression, Cell Counting, Infection

    Survivin is an upstream regulator of stiffness-induced cell cycle progression. (a) and (b) hVSMCs were transfected with control siRNA or siRNAs to cyclin D1, synchronized to G 0 via serum starvation, and plated on stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR to determine mRNA levels of cyclin D1 (CCND1) (a) and survivin (b). Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 3, independent experiments. (c) G 0 -synchronized hVSMCs were treated with either 5 or 30 μ M mitomycin C (MMC) and then cultured on soft or stiff hydrogels for 24 h. Survivin induction was analyzed by immunoblotting. Survivin protein levels were normalized to those in hVSMCs treated with DMSO on stiff hydrogels (d). n = 4–8, independent experiments.

    Journal: APL Bioengineering

    Article Title: Survivin as a mediator of stiffness-induced cell cycle progression and proliferation of vascular smooth muscle cells

    doi: 10.1063/5.0150532

    Figure Lengend Snippet: Survivin is an upstream regulator of stiffness-induced cell cycle progression. (a) and (b) hVSMCs were transfected with control siRNA or siRNAs to cyclin D1, synchronized to G 0 via serum starvation, and plated on stiff hydrogels with 10% FBS for 24 h. Total cell lysates were analyzed by RT-qPCR to determine mRNA levels of cyclin D1 (CCND1) (a) and survivin (b). Expression levels were normalized to those in hVSMCs treated with control siRNA on stiff hydrogels. n = 3, independent experiments. (c) G 0 -synchronized hVSMCs were treated with either 5 or 30 μ M mitomycin C (MMC) and then cultured on soft or stiff hydrogels for 24 h. Survivin induction was analyzed by immunoblotting. Survivin protein levels were normalized to those in hVSMCs treated with DMSO on stiff hydrogels (d). n = 4–8, independent experiments.

    Article Snippet: The following survivin ( BIRC5 ), FAK ( PTK2 ), and cyclin D1 ( CCND1 ) siRNAs were obtained from Ambion: survivin siRNA #1 (ID no. 121294), 5′-CCACUUCCAGGGUUUAUUCtt-3′; survivin siRNA #2 (ID no. 121295), 5′-GCCAUUCUAAGUCAUUGGGtt-3′; FAK siRNA #1 (ID no. 157448), 5′-CCUAGCAGACUUUAACCAAtt-3′; FAK siRNA #2 (ID no. 61352), 5′-GGCAUGGAGAUGCUACUGAtt-3′; and cyclin D1 siRNA (ID no. 42828), 5′-GGAGAACAAACAGAUCAUCtt-3′.

    Techniques: Transfection, Quantitative RT-PCR, Expressing, Cell Culture, Western Blot

    MYF5 target transcripts include mRNAs that encode proteins involved in myoblast proliferation and differentiation. ( A ) RIP assay using cytoplasmic lysates prepared from C2C12 cells using either anti-MYF5 antibody or IgG under conditions that preserved mRNA-RBP (mRNP) complexes. ( B ) Western blot analysis of MYF5 recovered in IP samples. ( C ) Following MYF5 RIP, MYF5-bound mRNAs were identified by microarray (RIP-chip) analysis in growing (GM) C2C12 cells. Data represent the Z -ratio of mRNAs in MYF5 RIP relative to IgG RIP. ( D ) RIP followed by RT-qPCR analysis to validate the association of MYF5 with mRNAs encoding myogenic proteins in proliferating C2C12 myoblasts; the levels of mRNAs in MYF5 IP were normalized to the levels of Gapdh mRNA and plotted as fold enrichment relative to the levels seen in control IgG IP samples. Discontinuous gray line: twofold enrichment in mRNAs bound to MYF5. ( E ) RIP analysis of Flag-MYF5 interaction with Ccnd1 mRNA. Forty-eight hours after C2C12 transfection with Flag-MYF5, RIP analysis was carried out using IgG or anti-Flag antibodies. Ccnd1 mRNA was detected by RT-qPCR analysis and its levels in Flag IP were compared with those in control IgG IP samples; Actn mRNA (encoding the housekeeping protein β-Actin) was measured to normalize sample input. Data in (D,E) represent the means and S.E.M. from three or more independent experiments. ( F ) Ingenuity pathway analysis (IPA) of mRNAs enriched in MYF5 IP relative to IgG in C2C12 growing myoblasts. *, P < 0.05 and **, P < 0.01 (Student's t -test).

    Journal: Nucleic Acids Research

    Article Title: Novel RNA-binding activity of MYF5 enhances Ccnd1 / Cyclin D1 mRNA translation during myogenesis

    doi: 10.1093/nar/gkw023

    Figure Lengend Snippet: MYF5 target transcripts include mRNAs that encode proteins involved in myoblast proliferation and differentiation. ( A ) RIP assay using cytoplasmic lysates prepared from C2C12 cells using either anti-MYF5 antibody or IgG under conditions that preserved mRNA-RBP (mRNP) complexes. ( B ) Western blot analysis of MYF5 recovered in IP samples. ( C ) Following MYF5 RIP, MYF5-bound mRNAs were identified by microarray (RIP-chip) analysis in growing (GM) C2C12 cells. Data represent the Z -ratio of mRNAs in MYF5 RIP relative to IgG RIP. ( D ) RIP followed by RT-qPCR analysis to validate the association of MYF5 with mRNAs encoding myogenic proteins in proliferating C2C12 myoblasts; the levels of mRNAs in MYF5 IP were normalized to the levels of Gapdh mRNA and plotted as fold enrichment relative to the levels seen in control IgG IP samples. Discontinuous gray line: twofold enrichment in mRNAs bound to MYF5. ( E ) RIP analysis of Flag-MYF5 interaction with Ccnd1 mRNA. Forty-eight hours after C2C12 transfection with Flag-MYF5, RIP analysis was carried out using IgG or anti-Flag antibodies. Ccnd1 mRNA was detected by RT-qPCR analysis and its levels in Flag IP were compared with those in control IgG IP samples; Actn mRNA (encoding the housekeeping protein β-Actin) was measured to normalize sample input. Data in (D,E) represent the means and S.E.M. from three or more independent experiments. ( F ) Ingenuity pathway analysis (IPA) of mRNAs enriched in MYF5 IP relative to IgG in C2C12 growing myoblasts. *, P < 0.05 and **, P < 0.01 (Student's t -test).

    Article Snippet: CCND1 siRNA (SR408533, Origene) was transfected 48 h before measuring cell number.

    Techniques: Western Blot, Microarray, Quantitative RT-PCR, Transfection

    MYF5 binds to specific sequences on the Ccnd1 mRNA. (A) Top , schematic showing biotinylated RNA fragments spanning the 5′UTR, coding region (CR), and 3′UTR of Ccnd1 mRNA used for pulldown. Bottom , biotinylated RNA fragments were incubated with cytoplasmic lysates from C2C12 cells (GM); after pulldown using streptavidin beads, the levels of MYF5 bound to the biotinylated RNA segments were detected by western blot analysis. (B) Recombinant purified His-MYF5 was incubated with biotinylated Ccnd1 RNA fragments followed by pulldown and detection of MYF5 by western blot analysis using anti-MYF5 antibody. (C) Schematic of biotinylated RNA fragments spanning the Ccnd1 3′UTR-C transcript ( top ), were tested for binding to His-MYF5 after pull-down using streptavidin beads; His-MYF5 interaction with RNA segments of fragment C ( middle ) and smaller RNAs after closer subdivision of fragments 9 through 11 ( bottom ) were assessed by western blot analysis using anti-MYF5 antibody. (D) GST or GST-MYF5 were incubated with radiolabeled Ccnd1 3′UTR-C10–1, then either resolved on native acrylamide gels ( left ) by RNA electrophoretic mobility shift assay (EMSA), or crosslinked by UV irradiation and resolved by SDS-PAGE ( right ). (E) The domain of MYF5 that interacts with the Ccnd1 3′-C fragment was mapped by creating GST-tagged truncations of MYF5 ( left ) and testing their interaction by biotin pulldown and western blot analysis using anti-GST antibody ( right ).

    Journal: Nucleic Acids Research

    Article Title: Novel RNA-binding activity of MYF5 enhances Ccnd1 / Cyclin D1 mRNA translation during myogenesis

    doi: 10.1093/nar/gkw023

    Figure Lengend Snippet: MYF5 binds to specific sequences on the Ccnd1 mRNA. (A) Top , schematic showing biotinylated RNA fragments spanning the 5′UTR, coding region (CR), and 3′UTR of Ccnd1 mRNA used for pulldown. Bottom , biotinylated RNA fragments were incubated with cytoplasmic lysates from C2C12 cells (GM); after pulldown using streptavidin beads, the levels of MYF5 bound to the biotinylated RNA segments were detected by western blot analysis. (B) Recombinant purified His-MYF5 was incubated with biotinylated Ccnd1 RNA fragments followed by pulldown and detection of MYF5 by western blot analysis using anti-MYF5 antibody. (C) Schematic of biotinylated RNA fragments spanning the Ccnd1 3′UTR-C transcript ( top ), were tested for binding to His-MYF5 after pull-down using streptavidin beads; His-MYF5 interaction with RNA segments of fragment C ( middle ) and smaller RNAs after closer subdivision of fragments 9 through 11 ( bottom ) were assessed by western blot analysis using anti-MYF5 antibody. (D) GST or GST-MYF5 were incubated with radiolabeled Ccnd1 3′UTR-C10–1, then either resolved on native acrylamide gels ( left ) by RNA electrophoretic mobility shift assay (EMSA), or crosslinked by UV irradiation and resolved by SDS-PAGE ( right ). (E) The domain of MYF5 that interacts with the Ccnd1 3′-C fragment was mapped by creating GST-tagged truncations of MYF5 ( left ) and testing their interaction by biotin pulldown and western blot analysis using anti-GST antibody ( right ).

    Article Snippet: CCND1 siRNA (SR408533, Origene) was transfected 48 h before measuring cell number.

    Techniques: Incubation, Western Blot, Recombinant, Purification, Binding Assay, Electrophoretic Mobility Shift Assay, Irradiation, SDS Page

    MYF5 regulates CCND1 expression in C2C12 myoblasts. (A) Western blot analysis of MYF5 and CCND1 expression during C2C12 differentiation; heat shock protein 90 (HSP90) was included as loading control. (B,C) Forty-eight hours after transfecting C2C12 cells with MYF5 siRNA or Ctrl siRNA, the levels of MYF5, CCND1 and loading control GAPDH were analyzed by western blot analysis (B) and the levels of Ccnd1 pre-mRNA and mRNA by RT-qPCR analysis (C). (D–F) Forty-eight hours after transfection of proliferating C2C12 myoblasts with Ctrl or CCND1 siRNAs, the levels of CCND1 and HSP90 were assessed by western blot analysis (D) and cell numbers were measured using a TC10 automated cell counter (BioRad) and represented as fold change in cell number after CCND1 silencing relative to those in the Ctrl siRNA group (E). At day 6 in differentiation medium (DM6) C2C12 differentiation was monitored by measuring creatine kinase activity (F). (G) Forty-eight hours after MYF5 was overexpressed using pFlag-MYF5 pcDNA3, the levels of MYF5, CCND1 and loading control HSP90 were studied by western blot analysis. Data in (B-F) represent the means and S.E.M. from three or four independent experiments. *, P < 0.05 and **, P < 0.01 (Student's t -test).

    Journal: Nucleic Acids Research

    Article Title: Novel RNA-binding activity of MYF5 enhances Ccnd1 / Cyclin D1 mRNA translation during myogenesis

    doi: 10.1093/nar/gkw023

    Figure Lengend Snippet: MYF5 regulates CCND1 expression in C2C12 myoblasts. (A) Western blot analysis of MYF5 and CCND1 expression during C2C12 differentiation; heat shock protein 90 (HSP90) was included as loading control. (B,C) Forty-eight hours after transfecting C2C12 cells with MYF5 siRNA or Ctrl siRNA, the levels of MYF5, CCND1 and loading control GAPDH were analyzed by western blot analysis (B) and the levels of Ccnd1 pre-mRNA and mRNA by RT-qPCR analysis (C). (D–F) Forty-eight hours after transfection of proliferating C2C12 myoblasts with Ctrl or CCND1 siRNAs, the levels of CCND1 and HSP90 were assessed by western blot analysis (D) and cell numbers were measured using a TC10 automated cell counter (BioRad) and represented as fold change in cell number after CCND1 silencing relative to those in the Ctrl siRNA group (E). At day 6 in differentiation medium (DM6) C2C12 differentiation was monitored by measuring creatine kinase activity (F). (G) Forty-eight hours after MYF5 was overexpressed using pFlag-MYF5 pcDNA3, the levels of MYF5, CCND1 and loading control HSP90 were studied by western blot analysis. Data in (B-F) represent the means and S.E.M. from three or four independent experiments. *, P < 0.05 and **, P < 0.01 (Student's t -test).

    Article Snippet: CCND1 siRNA (SR408533, Origene) was transfected 48 h before measuring cell number.

    Techniques: Expressing, Western Blot, Quantitative RT-PCR, Transfection, Activity Assay

    MYF5 promotes translation of Ccnd1 mRNA. (A,B) Forty-eight hours after Ctrl or MYF5 siRNA transfection of C2C12 cells, cytoplasmic extracts were fractionated through sucrose gradients to obtain cytoplasmic components of progressively larger weight: ribosomal subunits (40S, 60S), monosomes (80S) and low-molecular-weight (LMW) and high-molecular-weight (HMW) polysomes (A). The relative distribution of Gapdh mRNA, encoding a housekeeping protein, and Ccnd1 mRNA were measured by RT-qPCR analysis of RNA in each of the gradient fractions and represented as percentage of total RNA in the gradient (B). (C) Schematic of the dual luciferase reporter plasmids derived from the parent vector psiCHECK2 (psi), which expresses renilla luciferase (RL) and the internal control firefly luciferase (FL), and psiCHECK2-derived plasmids bearing the Ccnd1 fragments downstream of the RL coding region. (D) Top , Influence of MYF5 silencing on the expression of the reporter constructs. Twenty-four h after transfection of C2C12 cells with either MYF5 siRNA or Ctrl siRNA, each reporter plasmid was transfected, and 16 h later the ratio of RL activity to FL activity was measured. The decrease in relative RL/FL ratio of MYF5 siRNA-transfected cells relative to the RL/FL ratio of Ctrl siRNA-transfected cells is indicated. Bottom , RT-qPCR analysis of RL mRNA levels normalized to FL mRNA levels in each transfection group. Data represent the means and S.E.M. from 3 independent experiments. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).

    Journal: Nucleic Acids Research

    Article Title: Novel RNA-binding activity of MYF5 enhances Ccnd1 / Cyclin D1 mRNA translation during myogenesis

    doi: 10.1093/nar/gkw023

    Figure Lengend Snippet: MYF5 promotes translation of Ccnd1 mRNA. (A,B) Forty-eight hours after Ctrl or MYF5 siRNA transfection of C2C12 cells, cytoplasmic extracts were fractionated through sucrose gradients to obtain cytoplasmic components of progressively larger weight: ribosomal subunits (40S, 60S), monosomes (80S) and low-molecular-weight (LMW) and high-molecular-weight (HMW) polysomes (A). The relative distribution of Gapdh mRNA, encoding a housekeeping protein, and Ccnd1 mRNA were measured by RT-qPCR analysis of RNA in each of the gradient fractions and represented as percentage of total RNA in the gradient (B). (C) Schematic of the dual luciferase reporter plasmids derived from the parent vector psiCHECK2 (psi), which expresses renilla luciferase (RL) and the internal control firefly luciferase (FL), and psiCHECK2-derived plasmids bearing the Ccnd1 fragments downstream of the RL coding region. (D) Top , Influence of MYF5 silencing on the expression of the reporter constructs. Twenty-four h after transfection of C2C12 cells with either MYF5 siRNA or Ctrl siRNA, each reporter plasmid was transfected, and 16 h later the ratio of RL activity to FL activity was measured. The decrease in relative RL/FL ratio of MYF5 siRNA-transfected cells relative to the RL/FL ratio of Ctrl siRNA-transfected cells is indicated. Bottom , RT-qPCR analysis of RL mRNA levels normalized to FL mRNA levels in each transfection group. Data represent the means and S.E.M. from 3 independent experiments. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).

    Article Snippet: CCND1 siRNA (SR408533, Origene) was transfected 48 h before measuring cell number.

    Techniques: Transfection, Molecular Weight, Quantitative RT-PCR, Luciferase, Derivative Assay, Plasmid Preparation, Expressing, Construct, Activity Assay

    Influence of MYF5 on myogenesis via regulation of CCND1 expression. (A,B) C2C12 cells were transfected with MYF5 siRNA or Ctrl siRNA, along with a control vector [pcDNA3-Flag (pV)] or a plasmid vector that expressed Myc-tagged CCND1. Forty-eight hours later, the levels of CCND1 and MYF5 were analyzed by western blot analysis (A) and the degree of differentiation was analyzed by measuring creatine kinase activity at day 6 into differentiation (B). Data presented are the means and S.E.M. from four independent experiments; significance (P) is indicated. (C) Proposed model whereby MYF5 modulates myogenesis by acting upon CCND1 expression on two levels: first, MYF5 activates Ccnd1 transcription moderately, and second, MYF5 binds the Ccnd1 mRNA at the CR and 3′UTR, promoting Ccnd1 mRNA translation. The net effect is a CCND1-mediated increase in myoblast proliferation necessary at the initiation of myogenesis. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).

    Journal: Nucleic Acids Research

    Article Title: Novel RNA-binding activity of MYF5 enhances Ccnd1 / Cyclin D1 mRNA translation during myogenesis

    doi: 10.1093/nar/gkw023

    Figure Lengend Snippet: Influence of MYF5 on myogenesis via regulation of CCND1 expression. (A,B) C2C12 cells were transfected with MYF5 siRNA or Ctrl siRNA, along with a control vector [pcDNA3-Flag (pV)] or a plasmid vector that expressed Myc-tagged CCND1. Forty-eight hours later, the levels of CCND1 and MYF5 were analyzed by western blot analysis (A) and the degree of differentiation was analyzed by measuring creatine kinase activity at day 6 into differentiation (B). Data presented are the means and S.E.M. from four independent experiments; significance (P) is indicated. (C) Proposed model whereby MYF5 modulates myogenesis by acting upon CCND1 expression on two levels: first, MYF5 activates Ccnd1 transcription moderately, and second, MYF5 binds the Ccnd1 mRNA at the CR and 3′UTR, promoting Ccnd1 mRNA translation. The net effect is a CCND1-mediated increase in myoblast proliferation necessary at the initiation of myogenesis. N.S., not significant; *, P < 0.05; **, P < 0.01 (Student's t -test).

    Article Snippet: CCND1 siRNA (SR408533, Origene) was transfected 48 h before measuring cell number.

    Techniques: Expressing, Transfection, Plasmid Preparation, Western Blot, Activity Assay