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De Novo Assembly of a Field Isolate Genome Reveals Novel Plasmodium vivax Erythrocyte Invasion Genes

机译:De Novo大会的现场隔离基因组揭示了新的间日疟原虫间质红细胞入侵基因。

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摘要

Recent sequencing of Plasmodium vivax field isolates and monkey-adapted strains enabled characterization of SNPs throughout the genome. These analyses relied on mapping short reads onto the P. vivax reference genome that was generated using DNA from the monkey-adapted strain Salvador I. Any genomic locus deleted in this strain would be lacking in the reference genome sequence and missed in previous analyses. Here, we report de novo assembly of a P. vivax field isolate genome. Out of 2,857 assembled contigs, we identify 362 contigs, each containing more than 5 kb of contiguous DNA sequences absent from the reference genome sequence. These novel P. vivax DNA sequences account for 3.8 million nucleotides and contain 792 predicted genes. Most of these contigs contain members of multigene families and likely originate from telomeric regions. Interestingly, we identify two contigs containing predicted protein coding genes similar to known Plasmodium red blood cell invasion proteins. One gene encodes the reticulocyte-binding protein gene orthologous to P. cynomolgi RBP2e and P. knowlesi NBPXb. The second gene harbors all the hallmarks of a Plasmodium erythrocyte-binding protein, including conserved Duffy-binding like and C-terminus cysteine-rich domains. Phylogenetic analysis shows that this novel gene clusters separately from all known Plasmodium Duffy-binding protein genes. Additional analyses showing that this gene is present in most P. vivax genomes and transcribed in blood-stage parasites suggest that P. vivax red blood cell invasion mechanisms may be more complex than currently understood. The strategy employed here complements previous genomic analyses and takes full advantage of next-generation sequencing data to provide a comprehensive characterization of genetic variations in this important malaria parasite. Further analyses of the novel protein coding genes discovered through de novo assembly have the potential to identify genes that influence key aspects of P. vivax biology, including alternative mechanisms of human erythrocyte invasion.
机译:间日疟原虫田间分离株和猴子适应株的最新测序使整个基因组中的SNPs的表征。这些分析依赖于将短读段映射到间日疟原虫参考基因组上,该基因组是使用来自猴子适应株萨尔瓦多I的DNA产生的。在该菌株中缺失的任何基因组位点都将缺少参考基因组序列,并且在先前的分析中会丢失。在这里,我们报道了间日疟原虫田间分离基因组的从头组装。在2857个已装配的重叠群中,我们确定了362个重叠群,每个重叠群均包含参考基因组序列中不存在的5 kb以上的连续DNA序列。这些新的间日疟原虫DNA序列占380万个核苷酸,并包含792个预测基因。这些重叠群大多数都包含多基因家族的成员,可能起源于端粒区域。有趣的是,我们确定了两个重叠群,它们包含与已知的疟原虫红细胞入侵蛋白相似的预测蛋白编码基因。一个基因编码与食蟹猴RBP2e和诺氏假单胞菌NBPXb同源的网状细胞结合蛋白基因。第二个基因带有疟原虫红细胞结合蛋白的所有特征,包括保守的Duffy结合样和富含C端半胱氨酸的结构域。系统发育分析表明,该新基因与所有已知的疟原虫Duffy结合蛋白基因分别簇集。其他分析表明,该基因存在于大多数间日疟原虫基因组中,并在血阶段寄生虫中转录,这表明间日疟原虫红细胞入侵机制可能比目前理解的更为复杂。这里采用的策略是对以前的基因组分析的补充,并充分利用了下一代测序数据的优势,可以对这种重要的疟原虫的遗传变异提供全面的表征。通过从头组装发现的新型蛋白质编码基因的进一步分析,有可能识别出影响间日疟原虫生物学关键方面的基因,包括人类红细胞入侵的其他机制。

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