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通过聚合酶链反应(PCR)测定法评估为犬巴贝斯虫、维氏巴贝斯虫和罗氏巴贝斯虫亚种特异性鉴别设计的引物。

Assessment of primers designed for the subspecies-specific discrimination among Babesia canis canis, Babesia canis vogeli and Babesia canis rossi by PCR assay.

作者信息

Duarte Sabrina Castilho, Linhares Guido Fontgalland Coelho, Romanowsky Tatiana Nunes, da Silveira Neto Osvaldo José, Borges Ligia Miranda Ferreira

机构信息

Veterinary School, Federal University of Goiás, Brazil.

出版信息

Vet Parasitol. 2008 Mar 25;152(1-2):16-20. doi: 10.1016/j.vetpar.2007.12.013. Epub 2007 Dec 23.

DOI:10.1016/j.vetpar.2007.12.013
PMID:18242863
Abstract

Canine babesiosis is an infectious disease caused by either Babesia gibsoni or Babesia canis protozoans. The latter is also classified under three different phylogenetic groups, referred to as subspecies B. canis canis, B. canis vogeli and B. canis rossi. The objective of the present study was to validate and standardize a PCR assay to discriminate the organisms at the subspecies level. First, the reference sequences of the 18S rRNA, 5.8S rRNA and 28S rRNA genes, including the internal transcribed spacer 1 (ITS1) and 2 (ITS2) of the most common species and subspecies of the genus Babesia were retrieved from the GenBank database. Subspecies-specific primers (BAB3, BAB4 and BAB5) and one genus-specific primer were designed from the alignment of the sequences. The PCR assays were evaluated in three different combinations of primer pairs in order to assure complete specificity for each reaction. The results of the tests had demonstrated effectiveness of the novel primer pairs BAB1/BAB3, BAB1/BAB4 and BAB1/BAB5 for the amplification of the subspecies-specific target fragments of 746 bp (B. c. canis), 546 bp (B. c. vogeli) and 342 bp (B. c. rossi) by PCR. The original enzymatic amplification assays with novel primers reported in this paper were confirmed to be a reliable tool for the specific discrimination among B. canis subspecies by single-step PCR assays.

摘要

犬巴贝斯虫病是一种由吉氏巴贝斯虫或犬巴贝斯虫原生动物引起的传染病。后者也被归类为三个不同的系统发育组,称为犬巴贝斯虫犬亚种、犬巴贝斯虫韦氏亚种和犬巴贝斯虫罗氏亚种。本研究的目的是验证和标准化一种PCR检测方法,以便在亚种水平上鉴别这些病原体。首先,从GenBank数据库中检索巴贝斯虫属最常见的物种和亚种的18S rRNA、5.8S rRNA和28S rRNA基因的参考序列,包括内部转录间隔区1(ITS1)和2(ITS2)。根据序列比对设计了亚种特异性引物(BAB3、BAB4和BAB5)和一个属特异性引物。为确保每个反应的完全特异性,对引物对的三种不同组合进行了PCR检测评估。测试结果表明,新型引物对BAB1/BAB3、BAB1/BAB4和BAB1/BAB5可通过PCR扩增出746 bp(犬巴贝斯虫犬亚种)、546 bp(犬巴贝斯虫韦氏亚种)和342 bp(犬巴贝斯虫罗氏亚种)的亚种特异性目标片段。本文报道的用新型引物进行的原始酶促扩增检测被证实是一种通过单步PCR检测对犬巴贝斯虫亚种进行特异性鉴别的可靠工具。

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