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Multiple-Locus Variable Number Tandem Repeat Analysis for Streptococcus pneumoniae: Comparison with PFGE and MLST

机译:肺炎链球菌的多位点可变数目串联重复分析:与PFGE和MLST的比较

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摘要

In the era of pneumococcal conjugate vaccines, surveillance of pneumococcal disease and carriage remains of utmost importance as important changes may occur in the population. To monitor these alterations reliable genotyping methods are required for large-scale applications. We introduced a high throughput multiple-locus variable number tandem repeat analysis (MLVA) and compared this method with pulsed-field gel electrophoresis (PFGE) and multilocus sequence typing (MLST). The MLVA described here is based on 8 BOX loci that are amplified in two multiplex PCRs. The labeled PCR products are sized on an automated DNA sequencer to accurately determine the number of tandem repeats. The composite of the number of repeats of the BOX loci makes up a numerical profile that is used for identification and clustering. In this study, MLVA was performed on 263 carriage isolates that were previously characterized by MLST and PFGE. MLVA, MLST and PFGE (cut-off of 80%) yielded 164, 120, and 87 types, respectively. The three typing methods had Simpson's diversity indices of 98.5% or higher. Congruence between MLST and MLVA was high. The Wallace of MLVA to MLST was 0.874, meaning that if two strains had the same MLVA type they had an 88% chance of having the same MLST type. Furthermore, the Wallace of MLVA to clonal complex of MLST was even higher: 99.5%. For some isolates belonging to a single MLST clonal complex although displaying different serotypes, MLVA was more discriminatory, generating groups according to serotype or serogroup. Overall, MLVA is a promising genotyping method that is easy to perform and a relatively cheap alternative to PFGE and MLST. In the companion paper published simultaneously in this issue we applied the MLVA to assess the pneumococcal population structure of isolates causing invasive disease in the Netherlands before the introduction of the 7-valent conjugate vaccine.
机译:在肺炎球菌结合疫苗时代,对肺炎球菌疾病和运输的监测仍然至关重要,因为人群中可能发生重要变化。为了监测这些变化,大规模应用需要可靠的基因分型方法。我们引入了高通量多位点可变数目串联重复分析(MLVA),并将此方法与脉冲场凝胶电泳(PFGE)和多位点序列分型(MLST)进行了比较。此处描述的MLVA基于8个BOX位点,它们在两个多重PCR中被扩增。标记的PCR产物在自动DNA测序仪上确定大小,以准确确定串联重复序列的数量。 BOX基因座的重复数的组合构成了用于识别和聚类的数字配置文件。在这项研究中,对263个先前由MLST和PFGE表征的运载体分离株进行了MLVA。 MLVA,MLST和PFGE(截止80%)分别产生164、120和87种类型。三种打字方法的辛普森多样性指数为98.5%或更高。 MLST和MLVA之间的一致性很高。 MLVA对MLST的华莱士指数为0.874,这意味着如果两个菌株具有相同的MLVA类型,则它们具有88%的机会具有相同的MLST类型。此外,MLVA对MLST的克隆复合物的华莱士甚至更高:99.5%。对于一些属于单个MLST克隆复合体的分离株,尽管它们显示出不同的血清型,但MLVA具有更大的歧视性,可根据血清型或血清群产生组。总体而言,MLVA是一种有前途的基因分型方法,易于执行,并且是PFGE和MLST的相对便宜的替代品。在本期同时发表的同行论文中,我们应用MLVA评估了引入7价结合疫苗之前在荷兰引起侵袭性疾病的分离株的肺炎球菌种群结构。

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