旋毛虫肌幼虫p43cDNA的克隆及鉴定

中国寄生虫学与寄生虫病杂志 ›› 2005, Vol. 23 ›› Issue (6): 12-436.

旋毛虫肌幼虫p43cDNA的克隆及鉴定

郭恒¹,李莲瑞¹,刘明远¹*,吴秀萍¹,孙树民¹,付宝权¹,高长玲¹,卢强¹,陈启军³,P. Boireau²

1 吉林大学人兽共患病研究所,长春 130062; 2 法国食品卫生安全局,巴黎 94703;3 瑞典微生物与肿瘤研究中心,斯德哥尔摩 S-17177

收稿日期:1900-01-01 修回日期:1900-01-01 出版日期:2005-12-30 发布日期:2005-12-30

Cloning and Characterization of p43 cDNA from Trichinella spiralis

GUO Heng,LI Lian-rui,LIU Ming-yuan*, WU Xiu-ping,SUN Shu-min,FU Bao-quan,GAO Chang-ling,LU Qiang,CHEN Qi-jun,P. Boireau

Institute of Zoonoses,College of Animal Science and Veterinary Medicineof Jilin University,Changchun 130062,China

Received:1900-01-01 Revised:1900-01-01 Online:2005-12-30 Published:2005-12-30

摘要/Abstract

摘要： 目的克隆旋毛虫肌幼虫p43cDNA并对其表达的融合蛋白酶活性进行鉴定与分析。方法用PCR技术从旋毛虫肌幼虫cDNA文库中扩增靶基因，克隆到pMD?鄄18T载体，转化至大肠埃希菌NovaBlue，序列测定后克隆到原核表达载体pET28a并转入表达菌DE3中。经异丙基-β-D-硫代半乳糖苷（IPTG）诱导表达后提取包涵体并复性，通过降解双链λDNA测定其融合蛋白脱氧核糖核酸酶II（DNase II）活性。结果成功克隆到p43 cDNA序列，该cDNA序列与美国发表的存在两个核苷酸的变异，分别为第210位的C变为T，第604位的A变为G。基于3名研究者从旋毛虫T. spiralis美国分离株获得的序列相同、6名国内研究者（含本课题组）从T. spiralis中国分离株获得的序列也相同，由此可以确定这两个核苷酸的变异为T. spiralis中国分离株特异性和特征性单核苷酸多态性（SNP）标记。p43重组蛋白能够降解双链λDNA，表明其有DNase II酶活性。结论成功克隆到p43cDNA，T. spiralis中国分离株的p43cDNA具有两个SNP标记，其表达的重组蛋白具有DNase II酶活性。

关键词: 旋毛虫, p43cDNA, 克隆, 表达, 脱氧核糖核酸酶II

Abstract: Objective To clone and characterize the p43 cDNA from muscle larvae cDNA library of Trichinella spiralis (Ts） Chinese isolate. Methods PCR technique was used to amplify the target cDNA from muscle larvae cDNA library. After cloned in pMD18T vector， it was transformed into E. coli NovaBlue. The positive clones were sequenced and the cDNA was cloned into pET28a expression vector. After induced by IPTG， the inclusion body of the recombinant protein was purified and re-natured. The deoxyribonuclease II (DNase II ） activity of the recombinant protein was tested by hydrolyzing λDNA. Results Open reading frame （ORF） of the p43 cDNA was successfully cloned from the muscle larvae cDNA library of the Chinese Ts， there were mutations of two nucleotides in the ORF of the Chinese Ts p43 cDNA comparing with that from USA isolate at the positions 210 and 604， namely， C and A in the USA isolate but T and G in the Chinese isolate. Considering that three authors had cloned the same p43 cDNA from the USA isolate and six groups (including this team） had also obtained the same sequence from the Chinese isolate， the mutation of the two nucleotides was considered as the single nucleotide polymorphic (SNP） marker of the Chinese Ts isolate. The DNase II activity of the recombinant protein was successfully detected by hydrolyzing λDNA. Conclusion The p43 cDNA was successfully cloned from the muscle larvae cDNA library of the Ts Chinese isolate. Two SNPs were found in the nucleotide sequence. The DNase II activity was proved.

Key words: Trichinella spiralis, p43 cDNA, Cloning, Characterization, Deoxyribonuclease II

郭恒;李莲瑞;刘明远;吴秀萍;孙树民;付宝权;高长玲;卢强;陈启军;P.Boireau. 旋毛虫肌幼虫p43cDNA的克隆及鉴定[J]. 中国寄生虫学与寄生虫病杂志, 2005, 23(6): 12-436.

GUOHeng;LILian-rui;LIUMing-yuan*;WUXiu-ping;SUNShu-min;FUBao-quan;GAOChang-ling;LUQiang;CHENQi-jun;P.Boireau. Cloning and Characterization of p43 cDNA from Trichinella spiralis[J]. Chinese Journal of Parasitology and Parasitic Diseases, 2005, 23(6): 12-436.

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