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首页> 外文期刊>Journal of Clinical Microbiology >Multiplex PCR Assays for Simultaneous Detection of Six Major Serotypes and Two Virulence-Associated Phenotypes of Streptococcus suis in Tonsillar Specimens from Pigs
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Multiplex PCR Assays for Simultaneous Detection of Six Major Serotypes and Two Virulence-Associated Phenotypes of Streptococcus suis in Tonsillar Specimens from Pigs

机译:同时检测猪扁桃体样本中猪链球菌的六种主要血清型和两种与毒力相关的表型的多重PCR方法

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Multiplex PCR assays for the detection and identification of various Streptococcus suis strains in tonsillar specimens from pigs were developed and evaluated. In two separate reactions, five distinct DNA targets were amplified. Three targets, based on the S. suis capsular polysaccharide (cps) genes specific for serotypes 1 (and 14), 7, and 9, were amplified in multiplex PCR I. Two other targets, based on the serotype 2- (and 1/2-) specific cps gene and the epf gene, encoding the EF proteins of virulent serotype 2 and highly virulent serotype 1 strains, were amplified in multiplex PCR II. To identify false-negative results, firefly luciferase (luc) DNA and primers based on the luc gene were included in the assay. The multiplex PCR assays were evaluated with tonsillar specimens from pigs infected with S. suis strains. The results obtained with the PCR assays were compared with the results obtained with a bacteriological examination. Most (94%) of the results obtained with multiplex PCR assays were confirmed by the bacteriological examination. The PCR method seems to be more sensitive compared to the bacteriological method, since the remaining 6% of the samples were positive by PCR and negative by bacteriological examination. These results indicate that the PCR method is highly specific for the detection of S. suis strains most frequently involved in clinical disease in infected pig herds. The serotypes found by PCR in tonsillar specimens from diseased pigs were compared with the serotypes of the strains isolated from the affected tissues of the same pigs. The results showed that there is significant association between carriership and clinical illness for S. suis serotype 9 and EF-positive serotype 2 strains and not for serotype 7 and EF-negative serotype 2 (or 1/2) strains.
机译:建立并评估了用于检测和鉴定猪扁桃体标本中各种猪链球菌的多重PCR检测方法。在两个单独的反应中,扩增了五个不同的DNA靶标。基于 S的三个目标。对血清型1(和14),7和9特异的suis 荚膜多糖( cps )基因在多重PCR I中进行了扩增。另外两个基于血清型2-(多重PCR II扩增了编码有毒血清型2和高毒血清型1的EF蛋白的1 / 2-)特异的 cps 基因和 epf 基因。为了鉴定假阴性结果,测定中包括萤火虫荧光素酶( luc )DNA和基于 luc 基因的引物。用感染了 S的猪的扁桃体样本评估了多重PCR分析。 suis 菌株。将通过PCR测定获得的结果与通过细菌学检查获得的结果进行比较。通过多重PCR分析获得的大多数结果(94%)已通过细菌学检查得到证实。与细菌学方法相比,PCR方法似乎更为灵敏,因为其余6%的样品在PCR中为阳性,而在细菌学检查中为阴性。这些结果表明PCR方法对 S的检测具有高度特异性。猪群中最常与临床疾病有关的suis 菌株。通过PCR在患病猪的扁桃体样本中发现的血清型与从相同猪的受影响组织中分离出的菌株的血清型进行了比较。结果表明, S的携带者与临床疾病之间存在显着关联。 suis 血清型9和EF阳性血清型2菌株,而不适用于血清型7和EF阴性血清型2(或1/2)菌株。

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