非洲猪瘟病毒P30蛋白的表达及抗体液相芯片检测方法的建立  

作　　者：张芳源 杨大为 仇德洋 姜国骞 李桂梅 单虎 ZHANG Fangyuan;YANG Dawei;QIU Deyang;JIANG Guoqian;LI Guimei;SHAN Hu(College of Veterinary Medicine,Qingdao Agricultural University,Qingdao 266109,China;Novel Veterinary Pharmacy Innovation Center of Shandong Province,Qingdao 266109,China;Research Center for Engineering Technology in Veterinary Medicine and Veterinary Diagnostic Reagent of Shandong Province,Qingdao 266109,China)

机构地区：[1]青岛农业大学动物医学院,青岛266109 [2]山东省新兽药创制协同创新中心,青岛266109 [3]山东省兽药诊断试剂工程技术研究中心,青岛266109

出　　处：《畜牧兽医学报》2023年第10期4300-4310,共11页ACTA VETERINARIA ET ZOOTECHNICA SINICA

基　　金：山东省重点研发计划(2020CXGC010801-02);山东省农业重大应用技术创新项目(SD2019XM003)。

摘　　要：本研究旨在为建立高效、快速、准确检测非洲猪瘟病毒(African swine fever virus,ASFV)的抗体液相芯片检测方法。首先构建pET-28a-p30表达载体,利用大肠杆菌(Escherichia coli)原核表达系统表达ASFV重组P30蛋白,然后将重组P30蛋白与羧基化的荧光微球偶联,建立ASFV P30抗体液相芯片检测方法。经鉴定,重组质粒成功转入大肠杆菌BL21感受态细胞,并以包涵体形式表达,Western blot结果显示重组P30蛋白可以与ASFV阳性血清产生特异性反应,证明其具有良好的反应原性。建立的ASFV抗体液相芯片检测方法检测中值荧光强度(median fluorescent intensity,MFI)阈值为1575.7,最佳结合蛋白浓度为每1.25×10^(6)个微球6μg,最佳血清稀释度为1∶600,最佳二抗浓度为1μg·mL^(-1),该方法具有良好的特异性、灵敏性和重复性。用建立的方法和商品化ELISA试剂盒同时对92份临床采集的猪血清样本进行检测,结果显示二者符合率为92.39%。本研究成功表达重组P30蛋白,并建立了ASFV P30抗体液相芯片检测方法,为ASFV感染早期的血清学检测提供了新的方法,也为多种病原体的抗体检测奠定了基础。This study was conducted to develop a rapid and accurate method for detection of African swine fever virus(ASFV)antibody based on x-MAP technology.In this our study,pET-28a-p30 expression plasmid was constructed,and ASFV recombinant P30 protein was expressed in Escherichia coli.Then the recombinant P30 protein was coupled with carboxylated fluorescent microspheres and an x-MAP multiple bead-based technology was developed for detection of ASFV P30 antibody.The recombinant plasmid was successfully expressed in inclusion body form in Escherichia coli BL21.Western blot ting analysis showed that recombinant P30 protein could react specifically with ASFV positive serum,indicating that it had good reactivity.The detection threshold of the x-MAP based ASFV antibody detection method is MFI 1575.7,and the optimal binding protein concentration is 6μg per 1.25×10^(6) microspheres,the optimal serum dilution is 1:600,and the optimal concentration of secondary antibody is 1μg·mL^(-1),the method has good specificity,sensitivity and repeatability.Ninety-two clinical pig serum samples were tested by x-MAP analysis and compared with the result tested by a commercial ELISA kit.The results showed that the consistency was 92.39%.The recombinant P30 protein was successfully expressed,and the ASFV antibody detection method based on x-MAP technology was established,which provides a new method for the early serological detection of ASFV infection.

关 键 词：非洲猪瘟病毒 P30蛋白 原核表达 液相芯片技术 抗体检测 

分 类 号：S852.659.1[农业科学—基础兽医学]