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Nucleotide-resolution profiling of RNA recombination in the encapsidated genome of a eukaryotic RNA virus by next-generation sequencing

机译:下一代测序技术在真核RNA病毒衣壳化基因组中重组RNA的核苷酸分辨率分析

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摘要

Next-generation sequencing has been used in numerous investigations to characterize and quantify the genetic diversity of a virus sample through the mapping of polymorphisms and measurement of mutation frequencies. Next-generation sequencing has also been employed to identify recombination events occurring within the genomes of higher organisms, for example, detecting alternative RNA splicing events and oncogenic chromosomal rearrangements. Here, we combine these two approaches to profile RNA recombination within the encapsidated genome of a eukaryotic RNA virus, flock house virus. We detect hundreds of thousands of recombination events, with single-nucleotide resolution, which result in diversity in the encapsidated genome rivaling that due to mismatch mutation. We detect previously identified defective RNAs as well as many other abundant and novel defective RNAs. Our approach is exceptionally sensitive and unbiased and requires no prior knowledge beyond the virus genome sequence. RNA recombination is a powerful driving force behind the evolution and adaptation of RNA viruses. The strategy implemented here is widely applicable and provides a highly detailed description of the complex mutational landscape of the transmissible viral genome.
机译:下一代测序已用于众多研究中,通过绘制多态性图谱和测量突变频率来表征和量化病毒样品的遗传多样性。下一代测序也已用于鉴定在高等生物的基因组内发生的重组事件,例如,检测替代性的RNA剪接事件和致癌的染色体重排。在这里,我们结合这两种方法来在真核RNA病毒鸡群病毒的衣壳化基因组中分析RNA重组。我们以单核苷酸分辨率检测到成千上万的重组事件,这导致衣壳化基因组中的多样性与错配突变相匹配。我们检测到先前发现的缺陷RNA以及许多其他丰富而新颖的缺陷RNA。我们的方法异常敏感且无偏见,不需要病毒基因组序列以外的任何先验知识。 RNA重组是RNA病毒进化和适应背后的强大动力。此处实施的策略可广泛应用,并对可传播病毒基因组的复杂突变情况提供了高度详细的描述。

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