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重组蓖麻、相思子毒素A链嵌合突变体的制备与分析
引用本文:韩艳辉,张弢,康琳,高姗,辛文文,王景林. 重组蓖麻、相思子毒素A链嵌合突变体的制备与分析[J]. 生物技术通讯, 2011, 22(4): 453-457. DOI: 10.3969/j.issn.1009-0002.2011.04.001
作者姓名:韩艳辉  张弢  康琳  高姗  辛文文  王景林
作者单位:军事医学科学院微生物流行病研究所,病原微生物生物安全国家重点实验室,北京,100071
基金项目:军队"十一五"计划专题
摘    要:目的:构建蓖麻毒素(RIC)、相思子毒素(ABR)A链突变体的嵌合体蛋白,实现嵌合体蛋白的可溶性表达、纯化及抗原性分析。方法:采用柔性linker连接RIC A链突变体(mRICAD75AV76MY80A)和ABR A链突变体(mABRAE164AR167L),构建嵌合体基因mRICA/mABRA,将该嵌合体基因亚克隆至原核载体pQE80L构建表达质粒pQE80L-mRICA/mABRA,再转化至大肠杆菌M15获得表达工程菌株M15/pQE80L-mRICA/mABRA,工程菌在18℃经0.1 mmol/L的IPTG诱导14 h,表达的嵌合体蛋白经Ni-NTA亲和层析柱纯化,通过ELISA和Western印迹检测嵌合体蛋白的抗原性。结果:所获得的mRICA/mABRA嵌合体基因经一致性比对分析,与预计嵌合基因的序列一致性为100%,其开放读框全长1572 bp,编码524个氨基酸残基;重组表达质粒pQE80L-mRICA/mABRA经PCR及双酶切鉴定证明构建正确,嵌合体蛋白相对分子质量约为62×103,与预测相符,可溶性的嵌合体蛋白经Ni-NTA亲和层析柱纯化,纯度可达99%;间接ELISA和Western印迹结果表明,嵌合体蛋白能同时与抗RIC多克隆抗体和抗ABR多克隆抗体发生特异的抗原抗体反应。结论:得到的mRICA/mABRA嵌合体蛋白具有良好的抗原性,为研制新型RIC和ABR双价疫苗奠定了重要基础。

关 键 词:蓖麻毒素  相思子毒素  突变体  嵌合体  抗原性

Production and Characterization of a Recombinant Chimeric Protein Consisting Mutant Ricin A Chain and Abrin A Chain
HAN Yan-Hui,ZHANG Tao,KANG Lin,GAO Shan,XIN Wen-Wen,WANG Jing-Lin. Production and Characterization of a Recombinant Chimeric Protein Consisting Mutant Ricin A Chain and Abrin A Chain[J]. Letters in Biotechnology, 2011, 22(4): 453-457. DOI: 10.3969/j.issn.1009-0002.2011.04.001
Authors:HAN Yan-Hui  ZHANG Tao  KANG Lin  GAO Shan  XIN Wen-Wen  WANG Jing-Lin
Affiliation:HAN Yan-Hui,ZHANG Tao,KANG Lin,GAO Shan,XIN Wen-Wen,WANG Jing-Lin State Key Laboratory of Pathogen and Biosecurity,Institute of Microbiology and Epidemiology,Academy of Military Medical Sciences,Beijing 100071,China
Abstract:Objective: To construct the chimeric protein mRICA/mABRA consisting mutant ricin(RIC) A chain and abrin(ABR) A chain,express it in the cytoplasm of Escherichia coli M15,and evaluate its antigenicity.Methods: The chimeric gene mRICA/mABRA was produced by connecting the genes of mutant ricin A chain(mRICAD75AV76MY80A) and mutant abrin A chain(mABRAE164AR167L) via linker.The recombinant expression vector pQE80L-mRICA/mABRA was transformed into E.coli M15 for expression under induction of IPTG at 18℃.The product was purified using chelating nickel-nitrilotriacetic acid(Ni-NTA) affinity chromatography,and then its antigenicity was determined by ELISA and Western blot.Results: Both PCR and sequencing analysis proved that recombinant plasmid pQE80L-mRICA/mABRA was produced correctly,the sequence of chimeric gene mRICA/mABRA had a 100% homology with the sequence of designed gene,with an open reading frame of 1572 bp,which could encode the chimeric protein mRICA/mABRA with 524 amino acid residues.The Mr of soluble expressed protein mRICA/mABRA was approximately 62×103.The protein reached a purity of about 99% after purification,and showed specific affinity with both polyclonal antibodies against native ricin and abrin.Conclusion: This study describes the generation of a substantial amount of chimeric protein mRICA/mABRA from E.coli and the potential application of mRICA/mABRA as an effective chimeric vaccine candidate that can protect against ricin and abrin simultaneously.
Keywords:ricin A chain  abrin A chain  mutant  chimeric protein  antigenicity  
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