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Evaluating levels of PCR efficiency and genotyping error in DNA extracted from engorged and non-engorged female Dermacentor variabilis ticks

机译:评估从饱食和不饱食的雌性Dermacentor variabilis s中提取的DNA的PCR效率和基因分型错误水平

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摘要

Polymerase chain reaction (PCR)-based methods are increasingly used to elucidate tick biology. However, DNA extracted from ticks may provide poor PCR templates as a result of PCR inhibition by mammalian blood or contamination by male DNA (in fertilized females). In this study, the effects of removing the bloodmeal and reproductive organs were evaluated through paired DNA extractions in engorged and non-engorged Dermacentor variabilis (Say) (Acari: Ixodidae), prior to PCR amplification at 12 microsatellites. The first extraction utilized only mouthparts and legs ('mouthpart' samples) and the second utilized tick bodies ('body' samples). The results indicated that contamination by male DNA was an unlikely source of genotyping error in mouthpart and body samples. Engorged females showed higher levels of PCR inhibition in body vs. mouthpart samples, with a 29% decrease in amplification success rates per PCR and a 10-fold increase in levels of missing genotypes in body samples. By contrast, non-engorged females showed little difference in amplification success rates or numbers of missing genotypes in body vs. mouthpart samples. We discuss analytical concerns related to this systematic bias in PCR problems and recommend the removal of the bloodmeal and reproductive organs prior to DNA extraction, especially in engorged female ticks.
机译:基于聚合酶链反应(PCR)的方法越来越多地用于阐明壁虱生物学。但是,由于哺乳动物血液对PCR的抑制作用或雄性DNA(受精的雌性)的污染,从tick中提取的DNA可能提供的PCR模板质量较差。在这项研究中,在12个微卫星上进行PCR扩增之前,先通过配对的DNA提取方法对膨大和未膨化的Dermacentor variabilis(Say)(Acari:Ixodidae)中的成对DNA进行了评估,以评估去除血粉和生殖器官的效果。第一次提取仅使用口部和腿部(“口部”样品),第二次使用壁虱体(“体部”样品)。结果表明,男性DNA的污染是口腔和身体样本中不太可能出现基因分型错误的来源。饱食的女性在身体样品中比在口部样品中显示出更高的PCR抑制水平,每次PCR扩增成功率降低29%,身体样品中缺失基因型水平升高10倍。相比之下,未充血的雌性在体检样本和口器样本中扩增成功率或缺失基因型的数量几乎没有差异。我们讨论了与PCR问题中这种系统偏见有关的分析问题,并建议在DNA提取之前,尤其是在饱腹的雌性壁虱中,去除血粉和生殖器官。

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