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作 者:曲哲会[1] 唐雪峰[1] 赵聘[1] 赵云焕[1] 李建柱 郭晓秋[1]
机构地区:[1]信阳农林学院动物科学系,河南信阳464000
出 处:《中国畜牧杂志》2014年第1期6-10,共5页Chinese Journal of Animal Science
基 金:河南省科技攻关项目(112102110061);信阳农专青年教师科研基金项目(2009ZRKX020)
摘 要:本研究旨在分析淮南麻鸭IGF-Ⅰ基因的结构特点以及获得编码的蛋白。根据GenBank数据库中鹅、鸡和鸭的IGF-Ⅰ基因序列,设计1对引物P1/P2,利用RT-PCR方法克隆了淮南麻鸭的包含有编码区的部分IGF-Ⅰ基因。将IGF-Ⅰ编码区基因连接到原核表达载体pPROEXTMHTb,然后转化到感受态菌DH5α中,经终浓度为1.0 mmol/L的IPTG诱导表达IGF-Ⅰ融合蛋白。结果表明:获得了534 bp的淮南麻鸭IGF-Ⅰ部分基因,经过生物信息进行序列分析,包括1个462 bp的开放阅读框,可编码153个氨基酸,与鸭、鸡、人、绵羊、牛、野猪和大鼠的同源性分别达到99%、99%、84%、81%、83%、84%和78%;经SDS蛋白质电泳结果表明,成功获得分子量约27 ku的IGF-Ⅰ融合蛋白,纯化后经Western-blotting鉴定,可与兔抗人IGF-Ⅰ抗体发生特异性免疫反应。The research aimed to study the structural characteristics of IGF- I gene in Huainan duck and the functional production and analysis of its encoding proteins. According to the published sequence of IGF- I in GenBank, a pair of primers P1/P2 was designed to clone and analyze cDNA sequence of IGF-I gene in Huainan duck using RT-PCR and bioinformaties technique. The recombinant expression vector was constructed by cloning IGF- I gene in Huainan duck into the prokaryotie expression plasmid pPROEXTMHTb. The resulted showed that a eDNA sequence with the size of 534 bp was obtained, which included a 462 bp whole ORF and encoded 153 amino acid residuals, has an overall similarity with comparable region of domestic duck (99%), chicken (99%), coturnix (99%), human(84%), sheep(81%), bovine(83%), pig (84%) and rat(78%). The recombinant vector was transformed into the E. coli DH5 ( strain. The fusion protein is 27ku in size and it can affect specific reaction with the antibody through Western-blotting.
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