Recently, an rRNA-based polymerase chain reaction (PCR) has been developed for the detection of murine mycoplasmas at both the genus and species level (F. J. M. van Kuppeveld, J. T. M. van der Logt, A. F. Angulo, M. J. van Zoest, W. G. V. Quint, H. G. Niesters, J. M. D. Galama, and W. J. G. Melchers, Appl. Environ. Microbiol. 58:2606-2615, 1992). In this study, the diagnostic value of this PCR assay for the detection of Mycoplasma pulmonis in infected rats was studied. For this purpose, 25 Wistar rats were infected intranasally with M. pulmonis strain M72-138 and investigated for the presence of this pathogen by both in vitro isolation and PCR. Five rats were monitored longitudinally by screening of throat swabs at several time points for up to 248 days postinfection. The remaining 20 rats were killed between 3 and 87 days postinfection, and organism recovery from both throat and urogenital tract specimens was attempted. M. pulmonis could be detected in the throat for up to 248 days postinfection but not in the urogenital tract, either by culture or by PCR. PCR proved to be the optimal method for testing throat samples. All samples in which M. pulmonis was detected by culture were also positive by PCR. By PCR, M. pulmonis was also detected in 3.7% of the samples which were culture negative and in 9.9% of the samples from which cultures were overgrown with bacteria. The results of this study demonstrate the suitability of PCR for the detection of mycoplasmal infection in rodents.
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机译:最近,已开发出一种基于rRNA的聚合酶链反应(PCR),用于检测属和种水平的鼠类支原体(FJM van Kuppeveld,JTM van der Logt,AF Angulo,MJ van Zoest,WGV Quint,HG Niesters ,JMD Galama和WJG Melchers,Appl.Environ.Microbiol。58:2606-2615,1992)。在这项研究中,研究了该PCR检测对检测感染鼠肺炎支原体的诊断价值。为此,将25只Wistar大鼠经鼻内感染肺炎支原体菌株M72-138,并通过体外分离和PCR研究该病原体的存在。通过在几个时间点筛查咽拭子进行纵向监测,对五只大鼠进行感染后长达248天的监测。其余20只大鼠在感染后3至87天之间被杀死,并尝试从喉咙和泌尿生殖道标本中恢复细菌。通过培养或PCR,可以在感染后长达248天的喉咙中检测到肺炎支原体,而在泌尿生殖道中则不能。 PCR被证明是检测喉咙样品的最佳方法。通过培养检测到肺炎支原体的所有样品也通过PCR均为阳性。通过PCR,在3.7%培养阴性的样本中和9.9%细菌过度繁殖的样本中也检测到肺炎支原体。这项研究的结果证明了PCR在检测啮齿类动物支原体感染方面的适用性。
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