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利用多重 PCR 技术直接从培养物中快速鉴定荚膜组织胞浆菌。

Rapid identification of Histoplasma capsulatum directly from cultures by multiplex PCR.

机构信息

Departamento de Microbiología, Parasitología e Inmunología, Facultad de Medicina, Universidad de Buenos Aires, Paraguay 2155 piso 11, 1121 Buenos Aires, Argentina.

出版信息

Mycopathologia. 2012 Dec;174(5-6):451-6. doi: 10.1007/s11046-012-9567-2. Epub 2012 Jul 21.

DOI:10.1007/s11046-012-9567-2
PMID:22821346
Abstract

The multiplex PCR developed from a suspension of the yeast fungi correctly identified fifty-one clinical of H. capsulatum var. capsulatum strains isolated from clinical samples and soil specimens. The multiplex PCR was developed by combining two pairs of primers, one of them was specific to the H. capsulatum and the other one, universal for fungi, turned out to be specific to H. capsulatum, regardless of the fungus isolate studied. Primers designed to amplify a region of about 390-bp (Hc I-Hc II) and a region of approximately 600-bp (ITS1-ITS4) were used to identify a yeast isolated as H. capsulatum when both regions could be amplified. Absolute agreement (100 % sensitivity) could be shown between this assay and the cultures of H. capsulatum according to their morphological characteristics. Failure to amplify the target DNA sequence by PCR with primers Hc I-Hc II in the presence of the ITS1-ITS4 amplicon in isolates of P. brasiliensis, Cryptococcus neoformans, Trichosporon spp, Candida glabrata, C. albicans, C. tropicalis, C. parapsilosis, C. krusei, or Penicillium marneffei was an unequivocal sign of the high specificity of this assay. The assay specificity was also found to be 100 %. Incipient yeast forms obtained from clinical samples were identified as H. capsulatum by the PCR assay described before the morphological characteristics were registered shortening the time of diagnosis.

摘要

从酵母真菌混悬液中开发的多重 PCR 正确鉴定了从临床样本和土壤标本中分离出的五十一株荚膜组织胞浆菌荚膜变种临床株。该多重 PCR 是通过结合两对引物开发的,其中一对引物特异性针对荚膜组织胞浆菌,另一对引物通用,对真菌具有特异性,且无论研究的真菌分离株如何,结果均特异性针对荚膜组织胞浆菌。设计用于扩增约 390-bp 区域(Hc I-Hc II)和约 600-bp 区域(ITS1-ITS4)的引物用于鉴定被鉴定为荚膜组织胞浆菌的酵母分离株,当可以扩增这两个区域时。根据其形态特征,该检测方法与荚膜组织胞浆菌培养物之间可以显示出绝对一致性(100%敏感性)。在用引物 Hc I-Hc II 进行 PCR 时,如果在 P. brasiliensis、Cryptococcus neoformans、Trichosporon spp、Candida glabrata、C. albicans、C. tropicalis、C. parapsilosis、C. krusei 或 Penicillium marneffei 的分离物中未能扩增目标 DNA 序列,则这是该检测方法高度特异性的明确标志。该检测方法的特异性也为 100%。从临床样本中获得的初始酵母形式通过描述的 PCR 检测方法鉴定为荚膜组织胞浆菌,然后再记录形态特征,从而缩短了诊断时间。

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