Experiments with primary chick Mitral VICs and NIH3T3 cells, pIRES-GFP and pSV-b-galactosidase (Promega #E1081) vectors were co-transfected to determine transfection efficiency (pIRES-GFP) and to normalize the relative light units from the luciferase assay measurements. Transfections were performed using the Fugene reagent (Roche, #11-815-091-001) with a Fugene:DNA ratio of 6:2. After 48 hours, transfected mitral VIC extracts were prepared using reporter lysis buffer (Promega #E3971). To measure the luciferase activity, 20 mL of cell extract was added to 100 mL of Luciferase Assay Reagent (Promega #E1500) and the light produced was measured on a Monolight 2010 luminometer. Measurement of b-galactosidase activity in cell extracts was performed using the Promega b-galactosidase Enzyme Assay (Promega #E2000), and the A420 nm readings were used to standardize the luciferase assay values. Three replicates were used in each experiment and two independent experiments were performed. In the result section, the data obtained are represented as the average fold change for all replicates (n = 6) relative to controls. The error bars represent the standard error of the mean. An unpaired, two-tailed, Student’s Ttest was used to test for significance.JI-101 site PlasmidsThe mouse Crtl1 promoter (Crtl1) from 2979 to +26 was PCR amplified from genomic mouse DNA using the forward primer (59ccaaaccccttggctactcaaggc-39) and the reverse primer (59-cacttagctgggagctggag-39). The promoter was then cloned into a pGL3-Basic luciferase reporter vector (Promega, #E1751) between the KpnI and HindIII restriction enzyme sites. MedChemExpress Anlotinib Mutations were made to the Crtl1 construct at each Mef2 binding site using PCR Site-directed Mutagenesis and then cloned into pGL3Basic.The Mef2 consensus site from 2707 to 18055761 2698 was mutated from 59-ctataaataa-39 to 59-ctatagcgaa-39 (Crtl1-Mutant1) and the Mef2 consensus site from -922 to -913 was mutated from 59ttataaataa-39 to 59-ttatagcgaa-39 (Crtl1-Mutant2).The mouse Mef2c expression construct and Mef2-Engrailed dominant negative construct were provided by Dr. Eric Olson, University of Texas Southwestern Medical Center [15].Mitral VIC IsolationMitral valves from HH40 chick embryos were removed and digested with 400 mL of trypsin for 30 minutes. Mitral VICs were cultured in 100 mm cell culture dishes at 37uC with 5 CO2 in M199 medium (Gibco, #11150-059) with 1 chick serum, 1 penicillin/streptomycin, and 0.1 Insulin/Transferrin/Selenium (ITS).Results The Cartilage Link Protein Promoter Contains Two Highly Conserved Mef2 Binding SitesPrevious investigations by others into the regulation of the rat Crtl1 gene have shown that the upstream promoter region contains an A-T rich element that is conserved between mouse,Mef2c Regulates Crtl1 Transcriptionrat, and human and has a high degree of similarity to A-T rich elements found in the muscle creatine kinase promoter [27]. This A-T rich element is able to activate Crtl1 transcription in response to serum and can bind to an unidentified 32 kDa protein in electromobility shift assays using chondrocyte cell nuclear extracts [27]. It has been hypothesized that this protein could be a homeodomain containing protein or a MADS domain transcription factor [27]. The Mef2 transcription factors are members of the MADS domain family of transcription factors that bind to A-T rich sequences and regulate expression of multiple cardiac and skeletal muscle specific genes [28]. To determine whether Mef2 transcription factor b.Experiments with primary chick Mitral VICs and NIH3T3 cells, pIRES-GFP and pSV-b-galactosidase (Promega #E1081) vectors were co-transfected to determine transfection efficiency (pIRES-GFP) and to normalize the relative light units from the luciferase assay measurements. Transfections were performed using the Fugene reagent (Roche, #11-815-091-001) with a Fugene:DNA ratio of 6:2. After 48 hours, transfected mitral VIC extracts were prepared using reporter lysis buffer (Promega #E3971). To measure the luciferase activity, 20 mL of cell extract was added to 100 mL of Luciferase Assay Reagent (Promega #E1500) and the light produced was measured on a Monolight 2010 luminometer. Measurement of b-galactosidase activity in cell extracts was performed using the Promega b-galactosidase Enzyme Assay (Promega #E2000), and the A420 nm readings were used to standardize the luciferase assay values. Three replicates were used in each experiment and two independent experiments were performed. In the result section, the data obtained are represented as the average fold change for all replicates (n = 6) relative to controls. The error bars represent the standard error of the mean. An unpaired, two-tailed, Student’s Ttest was used to test for significance.PlasmidsThe mouse Crtl1 promoter (Crtl1) from 2979 to +26 was PCR amplified from genomic mouse DNA using the forward primer (59ccaaaccccttggctactcaaggc-39) and the reverse primer (59-cacttagctgggagctggag-39). The promoter was then cloned into a pGL3-Basic luciferase reporter vector (Promega, #E1751) between the KpnI and HindIII restriction enzyme sites. Mutations were made to the Crtl1 construct at each Mef2 binding site using PCR Site-directed Mutagenesis and then cloned into pGL3Basic.The Mef2 consensus site from 2707 to 18055761 2698 was mutated from 59-ctataaataa-39 to 59-ctatagcgaa-39 (Crtl1-Mutant1) and the Mef2 consensus site from -922 to -913 was mutated from 59ttataaataa-39 to 59-ttatagcgaa-39 (Crtl1-Mutant2).The mouse Mef2c expression construct and Mef2-Engrailed dominant negative construct were provided by Dr. Eric Olson, University of Texas Southwestern Medical Center [15].Mitral VIC IsolationMitral valves from HH40 chick embryos were removed and digested with 400 mL of trypsin for 30 minutes. Mitral VICs were cultured in 100 mm cell culture dishes at 37uC with 5 CO2 in M199 medium (Gibco, #11150-059) with 1 chick serum, 1 penicillin/streptomycin, and 0.1 Insulin/Transferrin/Selenium (ITS).Results The Cartilage Link Protein Promoter Contains Two Highly Conserved Mef2 Binding SitesPrevious investigations by others into the regulation of the rat Crtl1 gene have shown that the upstream promoter region contains an A-T rich element that is conserved between mouse,Mef2c Regulates Crtl1 Transcriptionrat, and human and has a high degree of similarity to A-T rich elements found in the muscle creatine kinase promoter [27]. This A-T rich element is able to activate Crtl1 transcription in response to serum and can bind to an unidentified 32 kDa protein in electromobility shift assays using chondrocyte cell nuclear extracts [27]. It has been hypothesized that this protein could be a homeodomain containing protein or a MADS domain transcription factor [27]. The Mef2 transcription factors are members of the MADS domain family of transcription factors that bind to A-T rich sequences and regulate expression of multiple cardiac and skeletal muscle specific genes [28]. To determine whether Mef2 transcription factor b.