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乙肝病毒突变核心蛋白基因的克隆及序列分析
引用本文:张洪勤,李佩珍,应俊. 乙肝病毒突变核心蛋白基因的克隆及序列分析[J]. 中国微生态学杂志, 2008, 20(6): 573-574
作者姓名:张洪勤  李佩珍  应俊
作者单位:温州医学院生物实验教学中心,浙江温州,325000
摘    要:目的克隆发生长片段缺失的乙肝病毒核心蛋白基因(HBV-C),并对其进行DNA序列和蛋白质结构分析。方法通过PCR从1株乙型肝炎病毒中扩增得到发生长片段缺失的HBV-C基因,利用TA克隆将PCR产物克隆人pUCm—T载体并进行测序、同源性比较和蛋白质结构分析。结果PCR扩增出的HBV-C基因经序列分析表明长度为454bp,其核苷酸序列缺失了220—317bp之间的98个碱基,造成从74个氨基酸起发生移码突变。结论成功克隆发生长片段缺失的HBV-C基因,为表达及功能研究奠定了基础。

关 键 词:乙肝病毒  核心蛋白基因  缺失  基因克隆

Cloning and analysis of the mutational core gene of the hepatitis B virus
ZHANG Hong-qin,LI Pei-zhen,YING Jun. Cloning and analysis of the mutational core gene of the hepatitis B virus[J]. Chinese Journal of Microecology, 2008, 20(6): 573-574
Authors:ZHANG Hong-qin  LI Pei-zhen  YING Jun
Affiliation:( Central Laboratory of Biology of Wenzhou Medical College, Wenzhou 325027, China)
Abstract:Objective To clone and analyze the deleted form of the hepatitis B virus core gene.Methods The deleted form of hepatitis B virus core gene was obtained by PCR from a hepatitis B virus genome.The PCR product was ligated into pUCm-T vector and sequenced.Result The cloned segment was 454 bp with 98 bp between 220 bp and 317 bp being lost.Conclusion The deleted form of hepatitis B virus core gene was cloned successfully which could be used for expression and function researches.
Keywords:Hepatitis B virus  Core gene  Deletion  Gene cloning
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