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使用针对微卫星和简单重复DNA序列的单引物对真菌进行聚合酶链反应指纹分析:新型隐球菌的菌株变异

Polymerase chain reaction fingerprinting in fungi using single primers specific to minisatellites and simple repetitive DNA sequences: strain variation in Cryptococcus neoformans.

作者信息

Meyer W, Mitchell T G

机构信息

Department of Microbiology, Duke University Medical Center, Durham, NC 27710, USA.

出版信息

Electrophoresis. 1995 Sep;16(9):1648-56. doi: 10.1002/elps.11501601273.

DOI:10.1002/elps.11501601273
PMID:8582350
Abstract

Minisatellites and simple repetitive DNA sequence motifs are used as conventional oligonucleotide probes in DNA-hybridization-based fingerprinting. The same oligonucleotides can be used as single primers in the polymerase chain reaction (PCR) to generate individual PCR fingerprints. In this study, the simple repetitive sequences, (CA)8, (CT)8, (CAC)5, (GTG)5, (GACA)4 and (GATA)4, and a minisatellite core sequence derived from the wild-type phage M13 (5' GAGGGTGGCGGTTCT 3') were used as specific, single primers to amplify hypervariable repetitive DNA sequences during PCR analysis. The potential applications of this techniques are demonstrated with clinical isolates of the human pathogenic yeast, Cryptococcus neoformans. PCR fingerprint patterns have remained stable after long-term in vitro passage ( > 2 1/2 years to date). Hybridization of the primers to blots of electrophorectically separated chromosomes demonstrated that the target sequences recognized by most of the primers are dispersed through the entire yeast genome. Sequence analysis of the cloned bands obtained by PCR fingerprinting indicated that if the same or extremely similar, inversely oriented tandem repeats are located close to each other, when only one repeat-specific primer is used in the PCR, the region between these repeats is amplified. PCR fingerprinting has a wide range of current and potential applications to fungi, such as clarifying taxonomic questions, facilitating epidemiological studies and improving the diagnosis of mycotic diseases.

摘要

小卫星和简单重复DNA序列基序在基于DNA杂交的指纹分析中用作传统的寡核苷酸探针。相同的寡核苷酸可在聚合酶链反应(PCR)中用作单引物,以生成个体PCR指纹。在本研究中,简单重复序列(CA)8、(CT)8、(CAC)5、(GTG)5、(GACA)4和(GATA)4,以及源自野生型噬菌体M13的小卫星核心序列(5' GAGGGTGGCGGTTCT 3')被用作特异性单引物,在PCR分析期间扩增高变重复DNA序列。该技术的潜在应用通过人类致病酵母新型隐球菌的临床分离株得到了证明。长期体外传代(至今超过2.5年)后,PCR指纹图谱保持稳定。引物与电泳分离的染色体印迹杂交表明,大多数引物识别的靶序列分散在整个酵母基因组中。对通过PCR指纹分析获得的克隆条带进行序列分析表明,如果相同或极其相似、反向排列的串联重复序列彼此靠近,当在PCR中仅使用一种重复特异性引物时,这些重复序列之间的区域会被扩增。PCR指纹分析在真菌领域有广泛的当前和潜在应用,如阐明分类学问题、促进流行病学研究以及改善真菌病的诊断。

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