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利用针对血凝素编码基因vlhA的聚合酶链反应(PCR)和DNA序列分析对家禽滑液支原体菌株进行特异性检测和分型

Specific detection and typing of Mycoplasma synoviae strains in poultry with PCR and DNA sequence analysis targeting the hemagglutinin encoding gene vlhA.

作者信息

Hong Yang, García Maricarmen, Leiting Victoria, Bencina Dulan, Dufour-Zavala Louise, Zavala Guillermo, Kleven Stanley H

机构信息

Department of Avian Medicine, College of Veterinary Medicine, The University of Georgia, Athens, GA 30602-4875, USA.

出版信息

Avian Dis. 2004 Sep;48(3):606-16. doi: 10.1637/7156-011504R.

DOI:10.1637/7156-011504R
PMID:15529983
Abstract

Mycoplasma synoviae is a major pathogen of chickens and turkeys, causing economic losses to the poultry industry worldwide. In this study, we validated and applied polymerase chain reaction (PCR) and DNA sequence analysis on the N-terminal end of the hemagglutinin encoding gene vlhA as an alternative for the detection and initial typing of field strains of M. synoviae in commercial poultry. PCR primers were tested against isolates of M. synoviae from various sources along with other avian mycoplasma and other bacterial species. The vlhA gene-targeted PCR assay was highly specific in the identification of M. synoviae, with a detection limit of 4.7 x 10(2) color changing units/ml. DNA sequence analysis of amplified products was also conducted to validate the potential for typing M. synoviae strains using the N-terminal region of the vlhA gene. To evaluate the test, we applied the PCR assay to tracheal swabs collected from chickens challenged with M. synoviae strain K1968 and compared the results to the serologic detection. The PCR assay was also evaluated directly on tracheal samples collected from commercial layers. Overall, this vlhA gene-targeted PCR is a useful tool for detection and initial typing of M. synoviae and can be applied in the preliminary identification of M. synoviae isolates directly from clinical samples.

摘要

滑膜支原体是鸡和火鸡的主要病原体,给全球家禽业造成经济损失。在本研究中,我们验证并应用聚合酶链反应(PCR)以及对血凝素编码基因vlhA的N端进行DNA序列分析,作为检测和初步分型商业化家禽中滑膜支原体田间菌株的替代方法。针对来自各种来源的滑膜支原体分离株以及其他禽支原体和其他细菌物种对PCR引物进行了测试。以vlhA基因为靶点的PCR检测在鉴定滑膜支原体方面具有高度特异性,检测限为4.7×10² 个颜色变化单位/毫升。还对扩增产物进行了DNA序列分析,以验证使用vlhA基因的N端区域对滑膜支原体菌株进行分型的潜力。为了评估该检测方法,我们将PCR检测应用于从感染滑膜支原体K1968株的鸡采集的气管拭子,并将结果与血清学检测结果进行比较。还直接对从商业蛋鸡采集的气管样本进行了PCR检测评估。总体而言,这种以vlhA基因为靶点的PCR是检测和初步分型滑膜支原体的有用工具,可用于直接从临床样本中对滑膜支原体分离株进行初步鉴定。

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