1. 您所在位置:
  2. 网站首页
  3. 文档分类
  4. 学术论文
  5. 自然科学论文

EGFP融合蛋白基因的构建、表达及活性分析.docxVIP

EGFP融合蛋白基因的构建、表达及活性分析.docx

    1. 1、本文档共13页,可阅读全部内容。
    2. 2、有哪些信誉好的足球投注网站(book118)网站文档一经付费(服务费),不意味着购买了该文档的版权,仅供个人/单位学习、研究之用,不得用于商业用途,未经授权,严禁复制、发行、汇编、翻译或者网络传播等,侵权必究。
    3. 3、本站所有内容均由合作方或网友上传,本站不对文档的完整性、权威性及其观点立场正确性做任何保证或承诺!文档内容仅供研究参考,付费前请自行鉴别。如您付费,意味着您自己接受本站规则且自行承担风险,本站不退款、不进行额外附加服务;查看《如何避免下载的几个坑》。如果您已付费下载过本站文档,您可以点击 这里二次下载
    4. 4、如文档侵犯商业秘密、侵犯著作权、侵犯人身权等,请点击“版权申诉”(推荐),也可以打举报电话:400-050-0827(电话支持时间:9:00-18:30)。
    5. 5、该文档为VIP文档,如果想要下载,成为VIP会员后,下载免费。
    6. 6、成为VIP后,下载本文档将扣除1次下载权益。下载后,不支持退款、换文档。如有疑问请联系我们
    7. 7、成为VIP后,您将拥有八大权益,权益包括:VIP文档下载权益、阅读免打扰、文档格式转换、高级专利检索、专属身份标志、高级客服、多端互通、版权登记。
    8. 8、VIP文档为合作方或网友上传,每下载1次, 网站将根据用户上传文档的质量评分、类型等,对文档贡献者给予高额补贴、流量扶持。如果你也想贡献VIP文档。上传文档
    查看更多
    EGFP融合蛋白基因的构建、表达及活性分析

    Arg9/人抗HBsAg单链抗体/ EGFP融合蛋白基因的构建、表达及活性分析 作者:薛茜,温伟红,孟艳玲,张勇,张巍,王涛,张瑞,杨安钢 【关键词】 肝炎,乙型;肝炎表面抗原,乙型;ScFv;Arg9 【Abstract】 AIM: To construct R9/ScFv14/EGFP fusion genes and to analyze the binding activity of the fusion proteins after they were expressed in E.coli BL21. METHODS: A series of oligonucleotide primers were designed and used to amplify the genes of ScFv14 and R9/ScFv14. The PCR products were cloned into pMD18T vector, followed by DNA sequencing. R9/ScFv14 gene and ScFv14 gene were ligated with EGFP gene respectively before they were recombined into the expression vector pET32a. After induced in E.coli BL21 by IPTG, the expressed fusion proteins named R9/ScFv14/EGFP and ScFv14/EGFP were detected by SDSPAGE and the binding activity of them were analyzed by indirect ELISA. RESULTS: Restriction endonuclease digestion and DNA sequencing proved that the two fusion genes were correctly constructed. SDSPAGE analysis showed that they were successfully expressed in E.coli BL21 and the percentages of them were 20% and 25% of total bacteria proteins respectively. Indirect ELISA confirmed that the expressed products had antigen specific binding activity. CONCLUSION: The two fusion genes were constructed successfully. And the products of them expressed in E.coli BL21 maintained the binding activity to HBsAg. 【Keywords】 hepatitis B; hepatitis B surface antigens; ScFv; Arg9 【摘要】 目的: 构建带有转膜结构域Arg9编码序列的R9/ScFv14/EGFP融合基因,将其转化入大肠杆菌中进行表达,并分析表达产物与HBsAg的结合活性. 方法: 设计引物,将Arg9的编码序列引入单链抗体基因的5′端,PCR扩增后获得带有Arg9编码序列的ScFv14基因,将PCR产物连入pMD18T载体,进行序列测定. 将测序正确的ScFv14基因和R9/ScFv14基因分别与EGFP基因连接后转化入原核表达载体pET32a,获得ScFv14/EGFP和R9/ScFv14/EGFP两种融合基因的表达载体,转化大肠杆菌BL21(DE3)LysS,以IPTG诱导表达,对表达产物进行SDSPAGE分析,并用间接ELISA方法检测其与HBsAg的亲和活性. 结果: 经酶切鉴定及测序证实ScFv14/EGFP融合基因和R9/ScFv14/EGFP融合基因序列完全正确.SDSPAGE分析表明两种融合基因在大肠杆菌BL21中成功获得表达,表达量分别占菌体总蛋白的20% 和25%.间接ELISA检测证实所表达的ScFv14/EGFP融合蛋白和R9/ScFv14/EGFP融合蛋白均具有HBsAg结合活性. 结论: 成功构建了带有转膜结构域Arg9编码序列的R9/ScFv14/EGFP融合基因,并在大肠杆菌BL21中成功表达,表达产物ScFv14/EGFP和R9/ScFv

    您可能关注的文档

    最近下载

    文档评论(0)

    zsmfjh + 关注
    实名认证
    文档贡献者

    该用户很懒,什么也没介绍

    咨询Ta 进入空间

    1亿VIP精品文档

    更多 >

    相关文档

    更多 >