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聚合酶链反应在人类伯氏疏螺旋体感染实验室诊断中的应用

PCR in laboratory diagnosis of human Borrelia burgdorferi infections.

作者信息

Schmidt B L

机构信息

Ludwig Boltzmann Institute for Dermato-Venerological Serodiagnosis, Hospital of Vienna-Lainz, Vienna, Austria.

出版信息

Clin Microbiol Rev. 1997 Jan;10(1):185-201. doi: 10.1128/CMR.10.1.185.

Abstract

The laboratory diagnosis of Lyme borreliosis, the most prevalent vector-borne disease in the United States and endemic in parts of Europe and Asia, is currently based on serology with known limitations. Direct demonstration of Borrelia burgdorferi by culture may require weeks, while enzyme-linked immunosorbent assays for antigen detection often lack sensitivity. The development of the PCR has offered a new dimension in the diagnosis. Capable of amplifying minute amounts of DNA into billions of copies in just a few hours, PCR facilitates the sensitive and specific detection of DNA or RNA of pathogenic organisms. This review is restricted to applications of PCR methods in the diagnosis of human B. burgdorferi infections. In the first section, methodological aspects, e.g., sample preparation, target selection, primers and PCR methods, and detection and control of inhibition and contamination, are highlighted. In the second part, emphasis is placed on diagnostic aspects, where PCR results in patients with dermatological, neurological, joint, and ocular manifestations of the disease are discussed. Here, special attention is given to monitoring treatment efficacy by PCR tests. Last, specific guidelines on how to interpret PCR results, together with the advantages and limitations of these new techniques, are presented.

摘要

莱姆病螺旋体病是美国最常见的媒介传播疾病,在欧洲和亚洲部分地区也有流行,目前其实验室诊断基于血清学,但存在已知局限性。通过培养直接证明伯氏疏螺旋体可能需要数周时间,而用于抗原检测的酶联免疫吸附测定通常缺乏敏感性。聚合酶链反应(PCR)的发展为诊断提供了新的维度。PCR能够在短短几小时内将微量DNA扩增成数十亿个拷贝,有助于灵敏且特异的检测致病生物的DNA或RNA。本综述局限于PCR方法在人类伯氏疏螺旋体感染诊断中的应用。在第一部分,重点介绍方法学方面,例如样品制备、靶标选择、引物和PCR方法,以及抑制和污染的检测与控制。在第二部分,重点放在诊断方面,讨论了患有该疾病皮肤、神经、关节和眼部表现患者的PCR结果。在此,特别关注通过PCR检测监测治疗效果。最后,给出了关于如何解释PCR结果的具体指南,以及这些新技术的优点和局限性。

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