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使用聚合酶链反应检测儿童临床标本中的结核分枝杆菌。

Detection of Mycobacterium tuberculosis in clinical specimens from children using a polymerase chain reaction.

作者信息

Smith K C, Starke J R, Eisenach K, Ong L T, Denby M

机构信息

Department of Pediatrics, University of Texas-Houston Health Science Center 77030, USA.

出版信息

Pediatrics. 1996 Feb;97(2):155-60.

PMID:8584370
Abstract

OBJECTIVE

We evaluated the usefulness of the polymerase chain reaction (PCR) using the insertion sequence IS6110 as the target for DNA to detect Mycobacterium tuberculosis in clinical specimens from children.

STUDY DESIGN

This was a prospective, controlled, blinded study comparing PCR on clinical specimens, mycobacterial culture, and clinical diagnosis.

PATIENTS

Sixty-five hospitalized children were evaluated, 35 with tuberculosis disease and 30 controls. Cases were defined by culture and/or specific clinical criteria. Controls included patients with tuberculosis infection but no detectable disease as well as patients free of tuberculosis infection and disease.

RESULTS

Polymerase chain reaction had a sensitivity of 40% and a specificity of 80% compared with clinical diagnosis. Mycobacterial culture had a sensitivity of 37%. The combination of culture and PCR identified 19 of 35 children (54%) with clinically diagnosed tuberculosis. There were six children with false-positive PCR results: One had tuberculosis infection without disease, two had Mycobacterium avium lymphadenitis, and three had diagnoses unrelated to tuberculosis.

CONCLUSIONS

The sensitivity of PCR is comparable to that of culture for detecting M tuberculosis in children, and may strengthen and hasten the clinical diagnosis in culture-negative patients. However, because of the limitations in specificity, the results of PCR alone are insufficient to diagnose tuberculosis in children. Although ongoing refinements in PCR techniques should improve the specificity of this test, epidemiologic and clinical information continue to be the most important consideration in the diagnosis of tuberculosis in culture-negative children.

摘要

目的

我们评估了以插入序列IS6110为DNA靶点的聚合酶链反应(PCR)在检测儿童临床标本中结核分枝杆菌的实用性。

研究设计

这是一项前瞻性、对照、盲法研究,比较了临床标本的PCR、分枝杆菌培养和临床诊断。

患者

对65名住院儿童进行了评估,其中35名患有结核病,30名作为对照。病例由培养和/或特定临床标准定义。对照包括结核感染但无明显疾病的患者以及无结核感染和疾病的患者。

结果

与临床诊断相比,聚合酶链反应的敏感性为40%,特异性为80%。分枝杆菌培养的敏感性为37%。培养和PCR相结合,在35名临床诊断为结核病的儿童中识别出19名(54%)。有6名儿童PCR结果为假阳性:1名有结核感染但无疾病,2名有鸟分枝杆菌淋巴结炎,3名诊断与结核无关。

结论

PCR检测儿童结核分枝杆菌的敏感性与培养相当,可能会加强和加快对培养阴性患者的临床诊断。然而,由于特异性的局限性,仅PCR结果不足以诊断儿童结核病。尽管PCR技术的不断改进应会提高该检测的特异性,但流行病学和临床信息仍然是培养阴性儿童结核病诊断中最重要的考虑因素。

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