The establishment of PCR amplification, cloning, and sequencing of bovine herpesvirus 1 (BHV-1) glycoprotein D gene isolated in Indonesia

Q4 Environmental Science

Indonesian Journal of Biotechnology Pub Date : 2019-06-18 DOI:10.22146/IJBIOTECH.44298

D. Hidayati, E. A. Srihanto, T. Untari, M. H. Wibowo, Koichi Akiyama, W. Asmara

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Abstract

Considering the increasing incidence of infectious bovine rhinotracheitis (IBR) in Indonesia, it was necessary to conduct a more in-depth study of bovine herpesvirus-1 (BHV-1) as the causative agent of IBR disease. Previous research reports indicate that the BHV-1 subtypes found in Indonesia are subtype 1.1. Currently, IBR field case detection in Indonesia still uses the serological method (ELISA), which has the potential to give false positive results and cannot explain the virus subtype. Other detection methods, such as viral isolation, take longer and require adequate resources. This study aimed to determine the BHV-1 subtypes of Indonesian isolates using molecular techniques. Nested PCR using two pairs of primers was successfully used to amplify the glycoprotein D (gD) gene. The gD gene fragment was cloned into the pGEM-T plasmid. Analysis of the gD gene sequence was subsequently carried out to determine the BHV-1 character of the Indonesian isolates. The results indicated that the isolates were different from the previous isolates, and had similarities (100%) with subtype 1.2 strain SP1777 and SM023.

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印度尼西亚牛疱疹病毒1型糖蛋白D基因的PCR扩增、克隆和序列测定

考虑到传染性牛鼻气管炎（IBR）在印度尼西亚的发病率不断上升，有必要对牛疱疹病毒-1（BHV-1）作为IBR疾病的病原体进行更深入的研究。先前的研究报告表明，在印度尼西亚发现的BHV-1亚型为1.1亚型。目前，印尼的IBR现场病例检测仍使用血清学方法（ELISA），该方法有可能给出假阳性结果，无法解释病毒亚型。其他检测方法，如病毒分离，需要更长的时间，并且需要足够的资源。本研究旨在利用分子技术确定印尼分离株的BHV-1亚型。采用两对引物的套式聚合酶链式反应成功地扩增了糖蛋白D（gD）基因。将gD基因片段克隆到pGEM-T质粒中。随后对gD基因序列进行分析，以确定印尼分离株的BHV-1特征。结果表明，这些分离株与以前的分离株不同，与1.2亚型菌株SP1777和SM023有100%的相似性。

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