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作 者:马晓林[1] 刘晨曦[2] 牛志刚[1] 唐森[1] 罗淑萍[2] 刘磊[2] 刘明军[1]
机构地区:[1]新疆畜牧科学院农业部家畜繁育生物技术重点开放实验室,新疆乌鲁木齐830000 [2]新疆农业大学,新疆乌鲁木齐830052
出 处:《草食家畜》2008年第2期15-18,共4页Grass-Feeding Livestock
基 金:新疆高技术研究发展计划;编号:20061106
摘 要:肌肉生长抑制素是肌肉生长的负调控因子。本研究为了得到有效抑制绵羊MSTN基因的siRNA分子,设计8对siRNA寡聚核苷酸引物,经退火与pSilencerTM4.1-CMV neo连接构建siRNA真核表达载体,转染C2C12细胞后,利用RT-PCR及real time PCR检测干扰效果。结果显示,8条siRNA分子中有3条对MSTN基因有显著的抑制作用,其中psi-mstn-717和psi-mstn-986分子对MSTN mRNA抑制效率分别达到61%和53%。本研究证实载体表达siRNA能有效抑制细胞MSTN mRNA的表达,下一步筛选的siRNA将用于体内实验。To construct the expression vector of siRNA targeting myostatin gene of ovis, and to observe the inhibitory effect of the vector on myostatin gene expression in C2C12 cells ,Methods: 55 base-pair oligonucleotide for small interfering RNA expression targeting MSTN gene was designed and chemically synthesized. After annealing, double oligonucleotide were inserted into the down-stream of CMV promotor of pSilencer4.1 to recombine pSilencer-mstn-siRNA plasmids. Eight siRNA expression vectors were transiently transfected into mouse fibroblast cell line C2C12 with lipofectamine-mediated transfection. RT-PCR and real time PCR was used to detect the expression levels of MSTN gene. Results: The recombined psi-mstn-717 and psi-mstn-986 vector significantly suppressed the expression of MSTN mRNA by 61% and 53% in cells. Conclusion: The constructed siRNA expression vector of MSTN gene can block the expression of MSTN gene in cell.
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