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[戊型肝炎病毒4型开放阅读框2蛋白在多形汉逊酵母中的表达]

[Expression of ORF2 protein of HEV genotype IV in Hansenula polymorpha].

作者信息

Su Cai-Xia, Gu Mei-Rong, Zhang Ping, Jin Zhen-Ji, Meng Fan-Hong, Chen Er-Jia, Yang Zhe, Liu Yong, Wang You-Chun

机构信息

Department of R&D, Dalian Hissen Bio-Pharmaceutical INC., 116600, China.

出版信息

Sheng Wu Gong Cheng Xue Bao. 2007 Jan;23(1):73-8.

Abstract

Hepatitis E, an acute infectious disease transmitted via the fecal-oral route, is caused by hepatitis E virus. However, no effective treatment currently exists for hepatitis E, and the only epidemic control approach is vaccination. But so for there are no commercial vaccine for hepatitis E available in the world. To find a new expression system to develop recombinant hepatitis E vaccine, in this study the expression system of methylotrophic yeast Hansenula polymorpha was used to express the gene encoding amino acid 112 - 607 of the open reading frame 2 (ORF2) of hepatitis E virus (HEV) genotype IV. In order to achieve high expression level, the coding sequence was optimized according to codon usage bias of Hansenula polymorpha and synthesized through overlapping PCR. Subsequently the gene was subcloned into the multi-copy expression vectors of Hansenula polymorpha, which include pDGXHP1.0 (MOX promotor), pDGXHP2.0 (MOX promotor) and pDGXHP2.1 ( FMD promotor). The series of one-copy and multi-copy recombinant plasmids were transformed into ATCC26012(Ura3-) by electroporation. The transformants were cultured in selection media MDL and screened for the existence of foreign gene by PCR. Then the strains were induced in MM media and the expression products were detected by SDS-PAGE, ELISA and Western blot assays to select the high-level expression strains. The result of SDS-PAGE showed that the HEV ORF2 expression product was accumulated up to 12% of total cellular protein and its molecular weight is 56kD. The expression product showed high immunoreactivity detected by ELISA and the highest titer is 1:2048. The result of Western blot demonstrated that the expression product could be specifically recognized by the polyclonal antibody against HEV. The successful expression of HEV ORF2 protein in Hansenula polymorpha provides foundation for the further development of recombinant subunit vaccine against hepatitis E.

摘要

戊型肝炎是一种通过粪-口途径传播的急性传染病,由戊型肝炎病毒引起。然而,目前尚无针对戊型肝炎的有效治疗方法,唯一的疫情控制手段是接种疫苗。但迄今为止,世界上尚无戊型肝炎的商用疫苗。为了找到一种新的表达系统来开发重组戊型肝炎疫苗,本研究利用甲基营养型酵母多形汉逊酵母的表达系统来表达戊型肝炎病毒(HEV)基因型IV开放阅读框2(ORF2)的112 - 607位氨基酸的编码基因。为了实现高表达水平,根据多形汉逊酵母的密码子使用偏好对编码序列进行优化,并通过重叠PCR合成。随后将该基因亚克隆到多形汉逊酵母的多拷贝表达载体中,这些载体包括pDGXHP1.0(甲醇氧化酶启动子)、pDGXHP2.0(甲醇氧化酶启动子)和pDGXHP2.1(口蹄疫病毒启动子)。通过电穿孔将一系列单拷贝和多拷贝重组质粒转化到ATCC26012(Ura3-)中。将转化体在选择培养基MDL中培养,并通过PCR筛选外源基因的存在。然后在MM培养基中诱导菌株,并通过SDS-PAGE、ELISA和Western blot分析检测表达产物,以筛选高表达菌株。SDS-PAGE结果显示,HEV ORF2表达产物积累量高达细胞总蛋白的12%,其分子量为56kD。ELISA检测显示表达产物具有高免疫反应性,最高效价为1:2048。Western blot结果表明,该表达产物能被抗HEV多克隆抗体特异性识别。HEV ORF2蛋白在多形汉逊酵母中的成功表达为进一步开发重组戊型肝炎亚单位疫苗奠定了基础。

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