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Hypervariability within the Rifin, Stevor and Pfmc-2TM superfamilies in Plasmodium falciparum

机译:恶性疟原虫Rifin,Stevor和Pfmc-2TM超家族内的高变异性

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摘要

The human malaria parasite, Plasmodium falciparum, possesses a broad repertoire of proteins that are proposed to be trafficked to the erythrocyte cytoplasm or surface, based upon the presence within these proteins of a Pexel/VTS erythrocyte-trafficking motif. This catalog includes large families of predicted 2 transmembrane (2TM) proteins, including the Rifin, Stevor and Pfmc-2TM super-families, of which each possesses a region of extensive sequence diversity across paralogs and between isolates that is confined to a proposed surface-exposed loop on the infected erythrocyte. Here we express epitope-tagged versions of the 2TM proteins in transgenic NF54 parasites and present evidence that the Stevor and Pfmc-2TM families are exported to the erythrocyte membrane, thus supporting the hypothesis that host immune pressure drives antigenic diversity within the loop. An examination of multiple P.falciparum isolates demonstrates that the hypervariable loop within Stevor and Pfmc-2TM proteins possesses sequence diversity across isolate boundaries. The Pfmc-2TM genes are encoded within large amplified loci that share profound nucleotide identity, which in turn highlight the divergences observed within the hypervariable loop. The majority of Pexel/VTS proteins are organized together within sub-telomeric genome neighborhoods, and a mechanism must therefore exist to differentially generate sequence diversity within select genes, as well as within highly defined regions within these genes.
机译:人类疟疾寄生虫恶性疟原虫具有广泛的蛋白质库,根据这些蛋白质中存在Pexel / VTS红细胞贩运基序,这些蛋白质被提议转运至红细胞胞质或表面。该目录包括预测的2个跨膜(2TM)蛋白质的大家族,包括Rifin,Stevor和Pfmc-2TM超家族,其每个家族在跨同源物之间和分离株之间均具有广泛的序列多样性区域,该区域仅限于拟议的表面-感染的红细胞上的裸露环。在这里,我们在转基因NF54寄生虫中表达2TM蛋白的表位标记版本,并提供了Stevor和Pfmc-2TM家族输出到红细胞膜的证据,从而支持了宿主免疫压力驱动环内抗原多样性的假说。对多个恶性疟原虫分离株的检查表明,Stevor和Pfmc-2TM蛋白内的高变环在分离株边界上具有序列多样性。 Pfmc-2TM基因在具有深远核苷酸同一性的大型扩增基因座中编码,从而突显了在高变环中观察到的差异。大多数Pexel / VTS蛋白在亚端粒基因组邻域内一起组织,因此必须存在一种机制,以差异化地在所选基因内以及这些基因内的高清晰度区域内产生序列多样性。

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