基于鞭毛蛋白基因的坚强芽孢杆菌特异性套式PCR和荧光定量PCR方法的建立

许彦芬; 王海亮; 陈大菾; 宋晓玲; 黄  倢

文章摘要

许彦芬,王海亮,陈大菾,宋晓玲,黄倢.基于鞭毛蛋白基因的坚强芽孢杆菌特异性套式PCR和荧光定量PCR方法的建立.渔业科学进展,2015,36(3):68-73

基于鞭毛蛋白基因的坚强芽孢杆菌特异性套式PCR和荧光定量PCR方法的建立

Establishment of Specific Detection Methods by Nested PCR and qPCR for Bacillus firmus Based on the hag Gene

投稿时间：2014-05-04 修订日期：2014-06-24

DOI：10.11758/yykxjz.20150311

中文关键词: 坚强芽孢杆菌鞭毛蛋白 hag基因套式PCR 荧光定量PCR

英文关键词: Bacillus firmus Flagellin hag gene Nested PCR Fluorescent quantitative PCR

基金项目:公益性行业科研专项经费项目(201103034)、现代农业产业技术体系(CARS-47)、山东省泰山学者建设工程专项经费和农业部科研杰出人才和创新团队专项经费共同资助

作者	单位
许彦芬	农业部海洋渔业可持续发展重点实验室中国水产科学研究院黄海水产研究所青岛 266071；上海海洋大学上海 201306
王海亮	农业部海洋渔业可持续发展重点实验室中国水产科学研究院黄海水产研究所青岛 266071
陈大菾	农业部海洋渔业可持续发展重点实验室中国水产科学研究院黄海水产研究所青岛 266071；上海海洋大学上海 201306
宋晓玲	农业部海洋渔业可持续发展重点实验室中国水产科学研究院黄海水产研究所青岛 266071；青岛海洋科学与技术国家重点实验室青岛 266071
黄倢	农业部海洋渔业可持续发展重点实验室中国水产科学研究院黄海水产研究所青岛 266071；上海海洋大学上海 201306；青岛海洋科学与技术国家重点实验室青岛 266071

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中文摘要:

细菌鞭毛蛋白编码基因hag具两端的保守序列及中间可变区域，在细菌的分类和鉴定中可作为分子标记。本研究克隆了坚强芽孢杆菌鞭毛蛋白编码基因hag部分序列，根据所得核酸序列设计套式引物Bfho和Bfhi，进行菌株的套式PCR特异性检测。此外，采用内引物Bfhi建立坚强芽孢杆菌荧光定量PCR特异性检测方法并确定该方法的检测限，对15个模拟样品进行检测并对阳性组中坚强芽孢杆菌的含量进行定量分析。结果显示，克隆得到的坚强芽孢杆菌hag基因长为1213 bp，经比对，与枯草芽孢杆菌hag基因相似性为13%−15%。荧光定量PCR方法对坚强芽孢杆菌菌株PC004和PC024的检测限分别为17.3×103和19.7×103 CFU/ml。模拟样品检测结果显示，15个样品中检测出7个阳性，并同时定量各样品中坚强芽孢杆菌的含量。本研究建立的坚强芽孢杆菌检测方法特异性强、操作时间短、灵敏度高，可为该菌的实际检测提供技术支持。

英文摘要:

Hag, a Flagellin coding gene, has conserved domains on the ends and a central domain that is highly variable in the length and the sequence, and hence has been used as a molecular marker in bacterial classification and identification. In this study, the hag gene was amplified from Bacillus firmus with the primer set Bhag, which was designed based on the conserved regions of the hag gene of B. subtilis and other bacteria. Two primer sets, Bfho and Bfhi, were designed based on the obtained sequence of hag of B. firmus and were used in the nested PCR for the species-specific detection of B. firmus. Furthermore we developed another specific detection method using fluorescent quantification PCR based on the inner primer set Bfhi, and tested the detection limit. Some simulated samples were tested with this FQ-PCR method and in the positive samples the concentrations of B. firmus were determined with the same method. The sequence of hag cloned from B. firmus had 1213 bp and was only 13%15% similar to that of B. subtilis according to NCBI BLAST, and most differences existed in the variable region. The detection limits of the FQ-PCR method were 17.3×103 CFU/ml and 19.7×103 CFU/ml for B. firmus strains PC004 and PC024 respectively. In 15 simulated samples, 7 were detected positive with the FQ-PCR method, and the concentrations of B. firmus in the samples were determined as well. The detection methods developed in our study have technical advantages such as high specificity, time-saving, and high sensitivity, and thus may become valuable tools in the practical application.

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