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利用聚合酶链反应中的单引物鉴定利什曼原虫属内物种和菌株的关系并确定其相关性。

Identification and determination of the relationships of species and strains within the genus Leishmania using single primers in the polymerase chain reaction.

作者信息

Schönian G, Schweynoch C, Zlateva K, Oskam L, Kroon N, Gräser Y, Presber W

机构信息

Institut für Mikrobiologie und Hygiene, Universitätsklinikum Charité, Humboldt-Universität zu Berlin, Germany.

出版信息

Mol Biochem Parasitol. 1996 Apr;77(1):19-29. doi: 10.1016/0166-6851(96)02572-8.

Abstract

DNA polymorphisms were assessed in different species and strains within the genus Leishmania by amplifying genomic DNA with single non-specific primers. This polymerase chain reaction (PCR) method employed non-random primers which anneal to mini- and microsatellite DNA sequences like the M13 core sequence and the simple repeat sequences (GTG)5 and (GACA)4, and the T3B primer derived from an intergenic spacer for tRNA genes. Distinctive and reproducible sets of amplified DNA fragments were obtained for all Leishmania isolates tested. The number and size of amplification products were found to be characteristic for a given taxon. Highly similar PCR profiles were observed when genomic DNA of representatives of the L. donovani, L. mexicana or L. braziliensis complexes was amplified. By comparing PCR patterns of unidentified Leishmania isolates with those obtained from reference strains it was possible to identify these isolates at the species level. The information of the amplification patterns was used for the construction of phylogenetic trees to measure the genetic relatedness within the genus Leishmania.

摘要

通过使用单一非特异性引物扩增基因组DNA,对利什曼原虫属内的不同物种和菌株的DNA多态性进行了评估。这种聚合酶链反应(PCR)方法使用非随机引物,这些引物可与微卫星和小卫星DNA序列退火,如M13核心序列、简单重复序列(GTG)5和(GACA)4,以及源自tRNA基因基因间隔区的T3B引物。对于所有测试的利什曼原虫分离株,均获得了独特且可重复的扩增DNA片段组。发现扩增产物的数量和大小是特定分类单元的特征。当扩增杜氏利什曼原虫、墨西哥利什曼原虫或巴西利什曼原虫复合体代表的基因组DNA时,观察到高度相似的PCR图谱。通过将未鉴定的利什曼原虫分离株的PCR模式与从参考菌株获得的模式进行比较,可以在物种水平上鉴定这些分离株。扩增模式的信息用于构建系统发育树,以衡量利什曼原虫属内的遗传相关性。

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