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高通量DNA测序在抗原变异研究中的应用:应用于奈瑟菌属物种。

The use of high-throughput DNA sequencing in the investigation of antigenic variation: application to Neisseria species.

作者信息

Davies John K, Harrison Paul F, Lin Ya-Hsun, Bartley Stephanie, Khoo Chen Ai, Seemann Torsten, Ryan Catherine S, Kahler Charlene M, Hill Stuart A

机构信息

Department of Microbiology, Monash University, Clayton, Victoria, Australia.

Victorian Bioinformatics Consortium, Monash University, Clayton, Victoria, Australia.

出版信息

PLoS One. 2014 Jan 22;9(1):e86704. doi: 10.1371/journal.pone.0086704. eCollection 2014.

Abstract

Antigenic variation occurs in a broad range of species. This process resembles gene conversion in that variant DNA is unidirectionally transferred from partial gene copies (or silent loci) into an expression locus. Previous studies of antigenic variation have involved the amplification and sequencing of individual genes from hundreds of colonies. Using the pilE gene from Neisseria gonorrhoeae we have demonstrated that it is possible to use PCR amplification, followed by high-throughput DNA sequencing and a novel assembly process, to detect individual antigenic variation events. The ability to detect these events was much greater than has previously been possible. In N. gonorrhoeae most silent loci contain multiple partial gene copies. Here we show that there is a bias towards using the copy at the 3' end of the silent loci (copy 1) as the donor sequence. The pilE gene of N. gonorrhoeae and some strains of Neisseria meningitidis encode class I pilin, but strains of N. meningitidis from clonal complexes 8 and 11 encode a class II pilin. We have confirmed that the class II pili of meningococcal strain FAM18 (clonal complex 11) are non-variable, and this is also true for the class II pili of strain NMB from clonal complex 8. In addition when a gene encoding class I pilin was moved into the meningococcal strain NMB background there was no evidence of antigenic variation. Finally we investigated several members of the opa gene family of N. gonorrhoeae, where it has been suggested that limited variation occurs. Variation was detected in the opaK gene that is located close to pilE, but not at the opaJ gene located elsewhere on the genome. The approach described here promises to dramatically improve studies of the extent and nature of antigenic variation systems in a variety of species.

摘要

抗原变异发生在广泛的物种中。这个过程类似于基因转换,即变异的DNA从部分基因拷贝(或沉默位点)单向转移到表达位点。以前对抗原变异的研究涉及从数百个菌落中对单个基因进行扩增和测序。利用淋病奈瑟菌的pilE基因,我们已经证明,通过PCR扩增,然后进行高通量DNA测序和一种新颖的组装过程,可以检测到个体抗原变异事件。检测这些事件的能力比以前有了很大提高。在淋病奈瑟菌中,大多数沉默位点包含多个部分基因拷贝。在这里我们表明,存在一种偏向,即使用沉默位点3'端的拷贝(拷贝1)作为供体序列。淋病奈瑟菌和一些脑膜炎奈瑟菌菌株的pilE基因编码I类菌毛蛋白,但来自克隆复合体8和11的脑膜炎奈瑟菌菌株编码II类菌毛蛋白。我们已经证实,脑膜炎球菌菌株FAM18(克隆复合体11)的II类菌毛是不变异的,克隆复合体8的菌株NMB的II类菌毛也是如此。此外,当一个编码I类菌毛蛋白的基因转入脑膜炎球菌菌株NMB背景时,没有抗原变异的证据。最后,我们研究了淋病奈瑟菌opa基因家族的几个成员,有人认为该家族存在有限的变异。在靠近pilE的opaK基因中检测到变异,但在基因组其他位置的opaJ基因中未检测到变异。这里描述的方法有望显著改善对各种物种中抗原变异系统的范围和性质的研究。

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