绵羊DRA基因外显子2酵母表面展示库的构建及鉴定

doi:10.16431/j.cnki.1671-7236.2016.03.002

›› 2016, Vol. 43 ›› Issue (3): 568-576.doi: 10.16431/j.cnki.1671-7236.2016.03.002

绵羊DRA基因外显子2酵母表面展示库的构建及鉴定

许万云, 王会敏, 汪文伦, 胡梦薇, 严国, 李建华, 高剑峰

石河子大学生命科学学院, 石河子 832003

收稿日期:2015-08-26 出版日期:2016-03-20 发布日期:2016-03-30
通讯作者: 高剑峰 E-mail:jianfengg@shzu.edu.cn
作者简介:许万云(1991-),女,山东青岛人,硕士生,研究方向:动物基因工程,E-mail:502981634@qq.com
基金资助:
国家重点基础研究发展计划(973计划)(2010CB530200)

Construction and Identification of Yeast Surface Display Libraries of Ovis aries DRA Gene Exon 2

XU Wan-yun, WANG Hui-min, WANG Wen-lun, HU Meng-wei, YAN Guo, LI Jian-hua, GAO Jian-feng

College of Life Science, Shihezi University, Shihezi 832003, China

Received:2015-08-26 Online:2016-03-20 Published:2016-03-30

摘要/Abstract

摘要： 根据绵羊DRA基因序列和酿酒酵母表面展示载体pYD1上的多克隆位点设计特异性引物,从绵羊组织中提取总RNA并逆转录,利用PCR技术扩增得到DRA基因,克隆获得762 bp目的片段,并提交GenBank,登录号:KR422362。将该基因通过双酶切连接到表面展示载体pYD1 上,成功构建了酿酒酵母表面展示重组质粒pYD1-DRA。将DRA基因外显子2两端进行基因点突变,形成新的酶切位点,继而对外显子2设计特异性引物,对绵羊大样本进行DNA池化,并将外显子2扩增产物测序,分析其多态性获得多态位点。重组质粒双酶切得到246 bp具有多态性的外显子2,将其连接到经同样酶双酶切的表面展示重组突变载体pYD1-DRA-TB上,成功构建了酿酒酵母表面展示库。将其转化用于表面展示的酿酒酵母EBY100感受态细胞中,得到酵母转化子,挑取酵母菌的单克隆通过PCR 扩增及序列测定证实了DRA基因库已成功整合到酿酒酵母基因组中。经半乳糖诱导后,通过免疫荧光法在荧光显微镜下检测得到DRA基因库已成功展示在酵母细胞表面。

关键词: 绵羊; DRA; 外显子2; 点突变; 酵母表面展示库; 免疫荧光法

Abstract: The specific primers were designed according to Ovis aries DRA gene sequence deposited in GenBank and the multiple cloning site of the plasmid pYD1,which was a vector used for protein surface display on Saccharomyces cerevisiae.The gene encoding DRA was amplified by PCR using the genomic RNA of Ovis aries.The 762 bp fragment was cloned and released in GenBank and registration number was KR422362.The PCR product was inserted into the yeast surface display plasmid vector pYD1 by double enzyme digestion.It was indicated that DRA gene was successfully integrated into the genome.Dot mutation was made at both ends of exon 2 in DRA gene for making restriction enzyme cutting site and design the exon 2 specific primers according to mutated Ovis aries DRA gene sequence.Sequenced exon 2 amplification products based on DNA pooling of sheep large sample template was analyzed the polymorphic loci.The polymorphic exon 2 246 bp fragment was obtained by double enzyme digestion and connected to surface display restructuring mutation carriers pYD1-DRA by the same double enzyme digestion,and then we successfully constructed yeast surface display libraries.We transformed it into Saccharomyces cerevisiae EBY100 cell.Yeast monoclone was identified by PCR amplification and sequencing,and we confirmed that DRA gene had been integrated into Saccharomyces cerevisiae genome.After galactose induced,it was detected that DRA gene library had been successfully demonstrated on the yeast cell surface under the fluorescence microscope by immunofluorescence method.

Key words: Ovis arise; DRA; exon 2; point mutation; yeast surface display libraries; immunofluorescence assay

中图分类号:

许万云, 王会敏, 汪文伦, 胡梦薇, 严国, 李建华, 高剑峰. 绵羊DRA基因外显子2酵母表面展示库的构建及鉴定[J]. , 2016, 43(3): 568-576.

XU Wan-yun, WANG Hui-min, WANG Wen-lun, HU Meng-wei, YAN Guo, LI Jian-hua, GAO Jian-feng. Construction and Identification of Yeast Surface Display Libraries of Ovis aries DRA Gene Exon 2[J]. , 2016, 43(3): 568-576.

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绵羊DRA基因外显子2酵母表面展示库的构建及鉴定

Construction and Identification of Yeast Surface Display Libraries of Ovis aries DRA Gene Exon 2

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