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使用单一引物对通过聚合酶链反应鉴定四种医学上重要的念珠菌属物种。

PCR identification of four medically important Candida species by using a single primer pair.

作者信息

Jordan J A

机构信息

Department of Pathology, School of Medicine, Magee-Womens Research Institute, University of Pittsburgh, Pennsylvania 15213.

出版信息

J Clin Microbiol. 1994 Dec;32(12):2962-7. doi: 10.1128/jcm.32.12.2962-2967.1994.

DOI:10.1128/jcm.32.12.2962-2967.1994
PMID:7883883
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC264208/
Abstract

A single pair of primers was used in a PCR assay to amplify and identify the DNAs from four medically important Candida species: C. albicans, C. parapsilosis, C. tropicalis, and C. (Torulopsis) glabrata. The report describes the first successful amplification of a chitin synthase-specific fragment from the four Candida species responsible for more than 90% of all cases of neonatal candidemia. The primer pair sequence was based on that from the C. albicans chitin synthase gene, CHS1 (J. Au-Young and P.W. Robbins, Mol. Microbiol. 4:197-207, 1990). Each of the four amplified products is a single band of a different size. The DNA sequence of each PCR product was determined, and four species-specific probes were synthesized. The DNAs from as few as 10 organisms in 100 microliters of plasma could be detected after amplification and Southern blot analysis. In a retrospective study of 27 paired blood samples from 16 patients with culture-proven candidemia, PCR analysis was successful at detecting and correctly identifying to the species level 26 of the 27 Candida isolates. The speed and accuracy of this PCR-based technology make it a very powerful tool for detecting and diagnosing candidemia. Implementation of this assay for analyzing blood samples should result in the more timely treatment of neonatal candidemia, thereby reducing morbidity and mortality.

摘要

在聚合酶链反应(PCR)检测中使用一对引物来扩增和鉴定来自四种医学上重要的念珠菌属物种的DNA:白色念珠菌、近平滑念珠菌、热带念珠菌和光滑念珠菌(Torulopsis光滑念珠菌)。该报告描述了首次成功从这四种念珠菌物种中扩增出几丁质合酶特异性片段,这四种念珠菌导致了超过90%的新生儿念珠菌血症病例。引物对序列基于白色念珠菌几丁质合酶基因CHS1(J. Au-Young和P.W. Robbins,《分子微生物学》4:197 - 207,1990)。四个扩增产物中的每一个都是一条大小不同的单带。测定了每个PCR产物的DNA序列,并合成了四种物种特异性探针。在扩增和Southern印迹分析后,可以检测到100微升血浆中低至10个生物体的DNA。在一项对16例经培养证实为念珠菌血症患者的27对血液样本的回顾性研究中,PCR分析成功地检测并在物种水平上正确鉴定了27株念珠菌分离株中的26株。这种基于PCR的技术的速度和准确性使其成为检测和诊断念珠菌血症的非常强大的工具。实施这种用于分析血液样本的检测方法应能使新生儿念珠菌血症得到更及时的治疗,从而降低发病率和死亡率。

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