引用本文:	黄锦炉,汪开毓,肖丹,刘贝贝,王均,黄凌远,付希,王浩丞.无乳链球菌(Streptococcus agalactiae) 三重PCR 快速检测方法的建立与应用.海洋与湖沼,2012,43(2):254-261.

【打印本页】【HTML】【下载PDF全文】【查看/发表评论】【下载PDF阅读器】【关闭】

过刊浏览高级检索

本文已被：浏览 3065次下载 4082次	码上扫一扫！
分享到：微信更多字体:加大+\|默认\|缩小-
*无乳链球菌(Streptococcus agalactiae) 三重PCR 快速检测方法的建立与应用*
黄锦炉¹, 汪开毓^1,2, 肖丹³, 刘贝贝¹, 王均¹, 黄凌远¹, 付希¹, 王浩丞¹
1.四川农业大学鱼病研究中心;2.动物疫病与人类健康四川省重点实验室;3.通威股份有限公司

摘要:

参照GenBank 发表的无乳链球菌sip、cpsE 这两个高度保守基因设计两组特异性引物, 应用已报道的无乳链球菌cpsL 基因高度保守序列的引物作为阳性对照引物, 经反应条件和反应体系参数优化, 建立一种检测无乳链球菌的三重PCR 方法, 并应用本三重PCR 方法检测40尾人工感染罗非鱼样本和22尾临床上收集的疑似无乳链球菌感染鱼样本。结果表明, 所建立的三重PCR 方法具有良好特异性, 检测无乳链球菌DNA样本时出现三条扩增条带, 检测其他7 种供试菌株DNA则不出现出任何扩增条带, 对无乳链球菌DNA 样本的最低检测浓度为 0.32ng/μ l, 最适Mg²⁺浓度为37.5mmol/L, 整个检测过程耗时100min左右。40尾人工感染罗非鱼的肝脏、肾脏组织DNA样本阳性检出率分别为100%, 22尾疑似无乳链球菌感染鱼的肝脏、肾脏组织DNA样本阳性检出率分别为72.7%, 以上两批样本检测结果与常规细菌鉴定方法结果一致。

关键词: 无乳链球菌, 三重PCR, 检测方法

DOI：10.11693/hyhz201202009009

分类号:

基金项目:教育部“长江学者和创新团队发展计划”创新团队项目, IRT0848 号; 通威股份有限公司重点资助项目, 2006 —2009

附件

THE DEVELOPMENT AND APPLICATION OF A TRIPLE PCR METHOD FOR RAPID DETECTION OF STREPTOCOCCUS AGALACTIAE

HUANG Jin-Lu¹, WANG Kai-Yu^1,2, XIAO Dan³, LIU Bei-Bei¹, WANG Jun¹, HUANG Ling-Yuan¹, FU Xi¹, WANG Hao-Cheng¹

1.Fish Disease Research Center of Sichuan Agricultural University;2.Key Laboratory of Animal Disease and Human Health of Sichuan Province, Sichuan Agricultural University;3.Tongwei Co. Ltd .

Abstract:

A pair of specific primers were designed based on the two well conserved genes of sip and cpsE of Strepto-coccus agalactiae published on the GenBank, respectively. The primer of cpsL gene well conserved in S. agalactiae was chosen to be the positive control. After the optimization of the reaction conditions and reaction system parameters, the triple PCR method for S. agalactiae detection was developed. The method was evaluated by examining samples of forty tilapia with artificial infection and twenty two suspected fish collected clinically. Results showed that the triple PCR method was well specific. The detection result of S. agalactiae DNA showed three bands, and those of other seven strains showed no bands. The minimum detection concentration of the S. agalactiae DNA was 0.32ng/μl, the optimization value of Mg²⁺ concentration was 37.5mmol/L, and it took about 100min to perform the examination. The positive rates of forty liver DNA samples and forty kidney DNA samples from the tilapia with artificial infection were 100%, respectively, and those of the twenty two liver DNA samples and twenty two kidney DNA samples from the suspected fish were 72.7%, respec-tively. Detection results of the two groups of samples were consistent with the results using general bacterial identification method.

Key words: Streptococcus agalactiae, Triple PCR, Detection method