畜牧兽医学报
畜牧獸醫學報
축목수의학보
2009年
11期
1588-1593
,共6页
张晓玮%崔文涛%伍晓雄%杨述林%牟玉莲%唐中林%李奎
張曉瑋%崔文濤%伍曉雄%楊述林%牟玉蓮%唐中林%李奎
장효위%최문도%오효웅%양술림%모옥련%당중림%리규
猪%MSTN前肽基因%定点诱变%真核表达
豬%MSTN前肽基因%定點誘變%真覈錶達
저%MSTN전태기인%정점유변%진핵표체
pig%MSTN propeptide gene%site-directed mutagenesis%eukaryotic expression
本研究旨在克隆通城猪含有第1个内含子的MSTN前肽基因,构建真核定点诱变载体,并通过转染C2C12细胞验证载体表达的有效性.以通城猪血液样品中提取的DNA作为模板,PCR扩增得到含第1个内含子的MSTN前肽基因,扩增产物进行克隆、测序.再将目的片段定向克隆到去除了EGFP基因的pEGFP-N1表达载体上.通过定点诱变方法将前肽编码序列第76位天冬氨酸突变为丙氨酸,获得定点诱变载体pEGFP(-)-N1-ProMstnD76A,并瞬时转染C2C12细胞.转染48 h后,通过RT-PCR和Real-time PCR方法检测目的基因的表达情况.结果表明:本研究成功克隆了通城猪含第1个内含子的MSTN前肽基因,并对该基因进行定点诱变修饰,构建了真核表达载体,转染后其前体mRNA能在C2C12细胞中进行正确剪接,目的基因mRNA表达水平较高.这为猪MSTN前肽基因在体内表达的研究奠定基础,并为制备转基因猪提供有用的分子材料.
本研究旨在剋隆通城豬含有第1箇內含子的MSTN前肽基因,構建真覈定點誘變載體,併通過轉染C2C12細胞驗證載體錶達的有效性.以通城豬血液樣品中提取的DNA作為模闆,PCR擴增得到含第1箇內含子的MSTN前肽基因,擴增產物進行剋隆、測序.再將目的片段定嚮剋隆到去除瞭EGFP基因的pEGFP-N1錶達載體上.通過定點誘變方法將前肽編碼序列第76位天鼕氨痠突變為丙氨痠,穫得定點誘變載體pEGFP(-)-N1-ProMstnD76A,併瞬時轉染C2C12細胞.轉染48 h後,通過RT-PCR和Real-time PCR方法檢測目的基因的錶達情況.結果錶明:本研究成功剋隆瞭通城豬含第1箇內含子的MSTN前肽基因,併對該基因進行定點誘變脩飾,構建瞭真覈錶達載體,轉染後其前體mRNA能在C2C12細胞中進行正確剪接,目的基因mRNA錶達水平較高.這為豬MSTN前肽基因在體內錶達的研究奠定基礎,併為製備轉基因豬提供有用的分子材料.
본연구지재극륭통성저함유제1개내함자적MSTN전태기인,구건진핵정점유변재체,병통과전염C2C12세포험증재체표체적유효성.이통성저혈액양품중제취적DNA작위모판,PCR확증득도함제1개내함자적MSTN전태기인,확증산물진행극륭、측서.재장목적편단정향극륭도거제료EGFP기인적pEGFP-N1표체재체상.통과정점유변방법장전태편마서렬제76위천동안산돌변위병안산,획득정점유변재체pEGFP(-)-N1-ProMstnD76A,병순시전염C2C12세포.전염48 h후,통과RT-PCR화Real-time PCR방법검측목적기인적표체정황.결과표명:본연구성공극륭료통성저함제1개내함자적MSTN전태기인,병대해기인진행정점유변수식,구건료진핵표체재체,전염후기전체mRNA능재C2C12세포중진행정학전접,목적기인mRNA표체수평교고.저위저MSTN전태기인재체내표체적연구전정기출,병위제비전기인저제공유용적분자재료.
This research intended to construct eukaryotic expression vector with a site-directed mu-tation of porcine MSTN propeptide gene, and verify its expression efficacy in C2C12 cells. By means of PCR amplification with DNA extracted from blood samples of Tongcheng pigs as tem-plates, MSTN propeptide gene containing the first intron was cloned and then suquenced. It was then subcloned into vector pEGFP-N1 without EGFP fragment and site-directed mutagenesis was perfomed which successfully converted Asp into Ala at the 76th amino acid site in propeptide se-quence. After being confirmed by R. E digestion and sequencing, the recombinant plasmid pEGFP (-)-N1-ProMstnD76A was transferred into C2C12 cells. After 48 h, the expression of target gene was detected at transcriptional level using RT-PCR and Real-time PCR. The results showed that the recombinant expression plasmid pEGFP(-)-N1-ProMstnD76A was constructed successfully. After being transiently transfected into C2C12 cells, the high expression level of target mRNA was detected and the primary mRNA transcript was found spliced correctly. The present research will lay a good foundation for further studying the functions of porcine MSTN propeptide gene in vivo and provide useful molecular materials for preparation of transgenic pigs.
