通过培养、直接免疫荧光和竞争性聚合酶链反应对沙眼衣原体进行定量分析。
Quantitation of Chlamydia trachomatis by culture, direct immunofluorescence and competitive polymerase chain reaction.
作者信息
Frost E H, Deslandes S, Bourgaux-Ramoisy D, Bourgaux P
机构信息
Département de microbiologie, Centre hospitalier universitaire de Sherbrooke, Quebec, Canada.
出版信息
Genitourin Med. 1995 Aug;71(4):239-43. doi: 10.1136/sti.71.4.239.
OBJECTIVES
Methods to quantitate Chlamydia trachomatis have never been compared although it would be relevant to periodically evaluate the sensitivity of a detection system. We compared the sensitivity and reproducibility of culture, direct immunofluorescence and the polymerase chain reaction (PCR) to quantitate C trachomatis.
METHODS
A competitive semiquantitative PCR procedure was developed. The number of inclusions in culture, particles by direct immunofluorescence and DNA copies by PCR were measured for 12 patient specimens. Variation was determined by measuring a sample 10 times for each method.
RESULTS
Patient C trachomatis major outer membrane protein gene DNA was measured semiquantitatively by amplifying together with reference DNA. DNA molecules, particles and infectious units were quantitated in clinical samples with, on average, 595 DNA molecules and 87 immunofluorescent particles observed per inclusion-forming-unit. Similar coefficients of variation (47-52%) were observed for the 3 procedures.
CONCLUSION
Competitive PCR and counting immunofluorescent particles provide reproducible and sensitive methods of quantitating C trachomatis.
目的
尽管定期评估检测系统的敏感性很有必要,但从未对沙眼衣原体定量方法进行过比较。我们比较了培养法、直接免疫荧光法和聚合酶链反应(PCR)定量沙眼衣原体的敏感性和可重复性。
方法
开发了一种竞争性半定量PCR方法。对12份患者标本测量了培养中的包涵体数量、直接免疫荧光法检测的颗粒数量以及PCR检测的DNA拷贝数。通过对每种方法的一个样本进行10次测量来确定变异情况。
结果
通过与参照DNA一起扩增对患者沙眼衣原体主要外膜蛋白基因DNA进行半定量测量。在临床样本中对DNA分子、颗粒和感染单位进行了定量,每个包涵体形成单位平均观察到595个DNA分子和87个免疫荧光颗粒。3种方法观察到相似的变异系数(47%-52%)。
结论
竞争性PCR和计数免疫荧光颗粒提供了可重复且敏感的沙眼衣原体定量方法。
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