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Intraspecific genetic variation in complex assemblages from mitochondrial metagenomics: comparison with DNA barcodes

机译:线粒体宏基因组学中复杂组合的种内遗传变异:与DNA条码的比较

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摘要

Metagenomic shotgun sequencing, using Illumina technology, and de novo genome assembly of mixed field-collected amples of invertebrates readily produce mitochondrial genome sequences, allowing rapid identification and quantification of species diversity. However, intraspecific genetic variability present in the specimen pools is lost during mitogenome assembly, which limits the utility of ‘mitochondrial metagenomics’ for studies of population diversity.ud2. Using 10 natural communities (>2600 individuals) of leaf beetles (Chrysomelidae), DNA variation in the mitochondrial cox1-5’ ‘barcode’ was compared for Sanger sequenced individuals and Illumina shotgun sequenced specimen pools. ud3. Generally, only a single mitochondrial contig was assembled per species, even in the presence of intraspecific variation. Ignoring ambiguity from the use of two different assemblers, the cox1 barcode regions from these assemblies were exact nucleotide matches of a Sanger sequenced barcode in 90.7% of cases, which dropped to 76.0% in assemblies from samples with large intra and interspecific variability. Nucleotide differences between barcodes from both data types were almost exclusively in synonymous 3rd codon position, although the number of affected sites was very low, and the greatest discrepancies were correlated with poor quality of Sanger sequences.ud4. Unassembled shotgun reads were also used to score single nucleotide polymorphisms and to calculate intraspecific nucleotide diversity (pi) for all available populations at each site. These values correlated with Sanger sequenced cox1 variation but were significantly higher.ud5. Overall, the assemblage-focused shotgun sequencing of pooled samples produced nucleotide variation data comparable to the well-established specimen-focused Sanger approach. The findings thus extend the application of mitochondrial metagenomics of complex biodiversity samples to the estimation of diversity below the species level.
机译:使用Illumina技术进行元基因组shot弹枪测序,以及从野外采集的无脊椎动物混合样本从头进行基因组组装,可轻松产生线粒体基因组序列,从而可以快速识别和定量物种多样性。但是,在有丝分裂基因组组装过程中,标本库中存在的种内遗传变异性消失了,这限制了“线粒体宏基因组学”在种群多样性研究中的应用。 ud2。利用10个叶甲虫(金眼科)的自然群落(> 2600个个体),比较了Sanger测序个体和Illumina shot弹枪测序标本库的线粒体cox1-5’“条形码”中的DNA变异。 ud3。通常,即使存在种内变异,每个物种也只能装配一个线粒体重叠群。忽略使用两种不同的装配体的歧义性,来自这些装配体的cox1条形码区域是Sanger测序条形码的精确核苷酸匹配,在90.7%的情况下,在具有较大的种内和种间变异性的样品的装配体中降至76.0%。来自两种数据类型的条形码之间的核苷酸差异几乎都在同义的第三个密码子位置,尽管受影响位点的数量非常少,并且最大的差异与Sanger序列质量差有关。 ud4。还使用未组装的shot弹枪读数对单个核苷酸多态性进行评分,并计算每个位点所有可用种群的种内核苷酸多样性(pi)。这些值与Sanger测序的cox1变异相关,但明显更高。 ud5。总体而言,以集合体为重点的shot弹枪测序汇集的样本所产生的核苷酸变异数据可与公认的以样本为中心的Sanger方法媲美。因此,这些发现将复杂生物多样性样品的线粒体宏基因组学的应用扩展到物种水平以下的多样性估计。

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