首页> 外文期刊>Journal of Clinical Microbiology >Concordance of clinical and environmental isolates of Cryptococcus neoformans var. gattii by random amplification of polymorphic DNA analysis and PCR fingerprinting.
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Concordance of clinical and environmental isolates of Cryptococcus neoformans var. gattii by random amplification of polymorphic DNA analysis and PCR fingerprinting.

机译:新型隐球菌变种临床和环境分离物的一致性。加蒂通过随机扩增的多态性DNA分析和PCR指纹图谱。

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Sixty-one clinical and forty-nine environmental isolates of Cryptococcus neoformans var. gattii from Australia and the United States were analyzed by random amplification of polymorphic DNA (RAPD), using 12- to 22-mer primers in pairs, and/or PCR fingerprinting with a single primer derived from the microsatellite core sequence of the wild-type phage M13 (5' GAGGGTGGCGGTTCT 3'). Three major genetic profiles were identified by both typing techniques. A single RAPD profile (VGI) predominated among clinical isolates (44 of 48, 92%) and isolates from host eucalypts (45 of 45, 100%) from Australia. Of the 94 Australian isolates, 4 (3 clinical and 1 environmental) were assigned to profile VGII; 2 of these were recovered from patients and one was recovered from plant debris from Western Australia. Only one Australian clinical isolate was assigned to profile VGIII. A different distribution of RAPD profiles (four VGIII, two VGII, and one VGI) was found among four clinical and three environmental isolates from the United States. RAPD profiles of 8 of the 101 isolates studied revealed minor genetic variants, 4 of profile VGI and 4 of profile VGII. Genetic concordance between the majority of clinical and environmental isolates in Australia is consistent with the hypothesis that human disease is acquired from exposure to host eucalypts. Profiles of clinical isolates were independent of body site of infection, and profiles of all isolates were stable over time. Analysis by PCR fingerprinting confirmed the RAPD results. A second RAPD profile (VGII) was associated with infection in southwest Western Australia, where the two host eucalypts do not occur naturally. This raises the possibility of an alternative and as yet unidentified natural habitat of C. neoformans var. gattii. Our results indicate that RAPD analysis is a sensitive and useful method for investigating environmental sources of human infection with this biotype.
机译:新变形隐球菌的六十一种临床和四十九种环境分离株。通过随机扩增多态性DNA(RAPD),使用12至22个mer引物对和/或使用源自野生型微卫星核心序列的单个引物进行PCR指纹图谱分析来分析来自澳大利亚和美国的gattii噬菌体M13(5'GAGGGTGGCGGTTCT 3')。通过两种打字技术鉴定出三个主要的遗传概况。在澳大利亚的临床分离株(48个中的44个,占92%)和寄主桉树分离株(45个中的45个,占100%)中,单一的RAPD谱(VGI)占主导地位。在94种澳大利亚分离株中,有4种(3种临床和1种环境)被归类为VGII;其中2例是从患者身上回收的,1例是从西澳大利亚州的植物残渣中回收的。仅将一个澳大利亚临床隔离株分配给VGIII谱。在来自美国的四个临床分离株和三个环境分离株中发现了不同的RAPD分布(四个VGIII,两个VGII和一个VGI)。研究的101个分离株中有8个的RAPD图谱显示较小的遗传变异,VGI图谱中的4个和VGII图谱中的4个。澳大利亚大多数临床和环境分离株之间的遗传一致性符合以下假设:人类疾病是通过暴露于宿主桉树而获得的。临床分离株的概况与感染的身体部位无关,并且所有分离株的概况随时间稳定。 PCR指纹图谱分析证实了RAPD结果。第二个RAPD图谱(VGII)与西澳大利亚州西南部的感染有关,在该处,两个寄主桉不是自然发生的。这就提出了新的C. neoformans var替代和尚未确定的自然栖息地的可能性。加蒂。我们的结果表明,RAPD分析是调查这种生物型人类感染的环境来源的灵敏且有用的方法。

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