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采用聚合酶链反应/杂交技术对马尔尼菲青霉进行特异性鉴定。

Specific identification of Penicillium marneffei by a polymerase chain reaction/hybridization technique.

作者信息

Vanittanakom N, Merz W G, Sittisombut N, Khamwan C, Nelson K E, Sirisanthana T

机构信息

Department of Microbiology, Faculty of Medicine, Chiang Mai University, Chiang Mai, Thailand.

出版信息

Med Mycol. 1998 Jun;36(3):169-75.

PMID:9776830
Abstract

Penicillium marneffei has been described recently as a cause of an emerging mycotic infection in HIV-infected patients. A PCR/hybridization assay was developed to rapidly identify this pathogen. The nucleotide sequence of the 631-bp region of 18S ribosomal DNA of P. marneffei was determined using the standard dideoxy chain termination method. An oligonucleotide probe was designed on the basis of the analysed sequences of P. marneffei and 18S rDNA sequences of other fungi in the GenBank database. A 631-bp PCR product was amplified using primers RRF1 and RRH1 from P. marneffei and seven other fungi, Penicillium spp., Aspergillus fumigatus, A. flavus, Histoplasma capsulatum, Cryptococcus neoformans, Candida albicans and C. krusei. A 15 oligonucleotide segment (Pm3) which was specific for P. marneffei was synthesized and used as a probe. Only the PCR products of P. marneffei isolates hybridized with the Pm3 oligonucleotide probe. The sensitivity of the assay was approximately 0.5 pg/microl and 0.1 pg/microl of DNA by PCR and Southern hybridization, respectively. The usefulness of this method as a diagnostic tool will require further studies.

摘要

马尔尼菲青霉最近被描述为人类免疫缺陷病毒(HIV)感染患者中新出现的真菌性感染的病因。已开发出一种聚合酶链反应/杂交检测法来快速鉴定这种病原体。使用标准双脱氧链终止法测定了马尔尼菲青霉18S核糖体DNA 631 bp区域的核苷酸序列。根据马尔尼菲青霉的分析序列以及GenBank数据库中其他真菌的18S rDNA序列设计了一种寡核苷酸探针。使用引物RRF1和RRH1从马尔尼菲青霉以及其他七种真菌(青霉属、烟曲霉、黄曲霉、荚膜组织胞浆菌、新型隐球菌、白色念珠菌和克柔念珠菌)中扩增出631 bp的PCR产物。合成了一段对马尔尼菲青霉具有特异性的15个寡核苷酸片段(Pm3)并用作探针。只有马尔尼菲青霉分离株的PCR产物与Pm3寡核苷酸探针杂交。该检测法的灵敏度通过PCR和Southern杂交分别约为0.5 pg/微升和0.1 pg/微升的DNA。作为一种诊断工具,该方法的实用性还需要进一步研究。

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