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通过广谱实时聚合酶链反应检测感染人类和动物的衣原体种类。

Detection by broad-range real-time PCR assay of Chlamydia species infecting human and animals.

作者信息

Goldschmidt P, Rostane H, Sow M, Goépogui A, Batellier L, Chaumeil C

机构信息

Laboratoire du Centre Hospitalier National d'Ophtalmologie des Quinze Vingts, 28 rue de Charenton, 75012 Paris, France.

出版信息

Br J Ophthalmol. 2006 Nov;90(11):1425-9. doi: 10.1136/bjo.2006.096420. Epub 2006 Aug 9.

Abstract

BACKGROUND

Tests available for molecular diagnosis of chlamydial infections detect Chlamydiatrachomatis, but do not find other Chlamydia species associated with genital, ophthalmic, cardiovascular, respiratory or neurological diseases. The routine detection of all Chlamydia species would improve the prognosis of infected people and guide therapeutic choices.

AIM

To design and validate a sensitive, specific, reproducible, inexpensive and easy-to-perform assay to quantify most Chlamydia species.

METHODS

Primers and probe were selected using the gene coding for the 16S rRNA. The detection limits were assessed for suspensions of Chlamydia trachomatis, Chlamydia psittaci and Chlamydia pneumoniae. The performance of this test was compared with that of two commercial kits (Amplicor-Roche and Artus) on 100 samples obtained from children with trachoma.

RESULTS

The detection capacities for Chlamydia trachomatis of the broad-range real-time polymerase chain reaction (PCR) were similar or slightly better than those obtained with commercial kits (0.2 copies of DNA/microl). Only the broad-range PCR identified specimens containing Chlamydia psittaci and Chlamydia pneumoniae. The commercial kits and the broad-range assay detected Chlamydia species in 5% and in 11%, respectively, of samples from children with trachoma.

CONCLUSIONS

This new real-time PCR offers a sensitive, reproducible assay that produces results in <3 h. With panels of quantified Chlamydia species, this real-time PCR can be run with all real-time PCR equipment. Larger trials are needed to confirm the utility of this test in diagnosis and for therapeutic follow-up.

摘要

背景

现有的用于衣原体感染分子诊断的检测方法可检测沙眼衣原体,但无法检测出与生殖器、眼科、心血管、呼吸道或神经系统疾病相关的其他衣原体物种。对所有衣原体物种进行常规检测将改善感染者的预后并指导治疗选择。

目的

设计并验证一种灵敏、特异、可重复、廉价且易于操作的检测方法,以对大多数衣原体物种进行定量。

方法

使用编码16S rRNA的基因选择引物和探针。评估沙眼衣原体、鹦鹉热衣原体和肺炎衣原体悬液的检测限。将该检测方法的性能与两种商业试剂盒(Amplicor - Roche和Artus)对100份沙眼患儿样本的检测性能进行比较。

结果

广谱实时聚合酶链反应(PCR)对沙眼衣原体的检测能力与商业试剂盒相似或略好(DNA/微升0.2拷贝)。只有广谱PCR能鉴定出含有鹦鹉热衣原体和肺炎衣原体的标本。商业试剂盒和广谱检测分别在11%和5%的沙眼患儿样本中检测到衣原体物种。

结论

这种新的实时PCR提供了一种灵敏、可重复的检测方法,能在3小时内得出结果。通过对衣原体物种进行定量分析,这种实时PCR可在所有实时PCR设备上运行。需要进行更大规模的试验来证实该检测方法在诊断和治疗随访中的实用性。

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