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昆虫细胞杆状病毒表达系统表达重组人类ZP3蛋白的研究

Expression of recombinant human ZP3 protein using the baculovirus expression system

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摘要目的：探讨利用重组表达系统制备重组人类ZP3（hZP3）蛋白的方法和技术难点,为hZP3蛋白的制备和应用打下技术基础。方法：构建hZP3的载体质粒pFASTBAC HTa-hZP3,在大肠杆菌宿主细胞中利用杆状病毒Bac-to-Bac系统同源重组构建重组的杆状病毒穿梭载体Bacmid,用重组的Bacmid转染Sf9细胞制备重组杆状病毒,分别表达带HIS标签的h ZP3全长蛋白（氨基酸1-424）和截短的hZP3蛋白（氨基酸23-348）。摸索重组hZP3蛋白的表达时间和纯化制备方法。结果：成功制备了表达重组人hZP3全长蛋白和截短体蛋白的Bacmid和杆状病毒颗粒,Western印迹检测表明,在Sf9细胞中较好的表达时间段为感染后72-96 h。重组表达的hZP3蛋白可以部分被钴柱亲和纯化,大量的重组hZP3蛋白不能结合到亲和介质而流穿,但确切的原因还未知。纯化得到的hZP3经荧光素Dylight Dye488标记,能与人精子结合。结论：利用昆虫细胞杆状病毒表达系统表达hZP3蛋白是可行的,可以进一步优化,但hZP3蛋白的有效富集和纯化方法是最大的瓶颈,还需要进一步摸索。 Objective： To investigate the methods and solve the technical bottlenecks in the preparation of recombinant human protein h ZP3 using the baculovirus expression system and pave the technical ground for the production and application of recombinant hZP3. Methods： The recombinant vector pFASTBAC HTa-hZP3 was constructed and transferred to competent E. coli cells carrying bacmid to produce recombinant bacmid by homologous recombination. Sf9 cells were transfected with the recombinant bacmid to produce recombinant baculovirus. Full-length recombinant h ZP3（ amino acids 1-424） and truncated recombinant hZP3（ amino acids 23-348） were expressed in the sf9 cells by infection with the recombinant baculovirus. The expression time of hZP3 was determined by Western blot and its purification was explored. Results： The recombinant bacmid and baculovirus were successfully constructed for expressing both the full-length and truncated hZP3. The maximal expression of recombinant hZP3 in the sf9 cells was achieved at 72-96 hours after baculovirus infection. Some of the recombinant h ZP3 with His-tag could bind affinity matrix and got purified but most of the solubilized h ZP3 passed through and the reasons remained unknown. Purified recombinant h ZP3 labeled with Dylight Dye488 was able to bind human sperm. Conclusion： It is feasible to express recombinant h ZP3 in insect cells using the baculovirus system though the yield of hZP3 needs to be optimized. The methods for efficient enrichment and purification of recombinant hZP3 require further exploration.

作者卢慧刁华肖玉芳于合国李铮施惠娟

机构地区上海交通大学医学院附属仁济医院泌尿外科上海市计划生育科学研究所

出处《中华男科学杂志》 CAS CSCD 2014年第11期978-983,共6页 National Journal of Andrology

基金国家重点基础研究发展计划973计划(2011CB944504) 上海市科委重点课题(10JC1409900)~~

关键词人ZP3 精子重组蛋白昆虫细胞杆状病毒表达系统 hZP3 sperm recombinant protein baculovirus expression system

分类号 Q786 [生物学—分子生物学]

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参考文献17

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中华男科学杂志

2014年第11期

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