Application of a simple and high-throughput DNA extraction method to real-time PCR quantification of target plant-parasitic nematodes in nematode communities

Nematological Research (Japanese Journal of Nematology) Pub Date : 2018-07-25 DOI:10.3725/JJN.48.1

Masanori Kawanobe, K. Toyota

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引用次数: 0

Abstract

Molecular techniques are prevailing in nematode identification and quantification, for which DNA extraction from nematodes is essential. However, the published DNA extraction methods are laborious and often require various expensive consumables and high-end equipment. In order to prepare DNA templates for a high-throughput real-time PCR assay, the present study modified a conventional DNA extraction method of Naklha et al. (2010) from nematode suspensions with ordinary lab equipment and achieved results and advantages comparable with two other conventional methods. The results of real-time PCR assays for quantifying Pratylenchus zeae, Tylenchorhynchus leviterminalis and Hoplolaimus sp. using the new protocol were highly correlated with those obtained by morphological counts and comparable to or more sensitive than those obtained by two conventional methods. Although the new protocol took over 100 min for DNA extraction, the manual processing took less than 10 min, i.e., half to one-fourth of the other methods. The running cost was less than half to one-tenth of the other methods. Nematol. Res. 48(1), 1–10 (2018).

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一种简单、高通量的DNA提取方法在线虫群落中目标植物-寄生线虫实时PCR定量中的应用

分子技术在线虫的鉴定和定量中很流行，其中提取线虫的DNA是必不可少的。然而，已发表的DNA提取方法是费力的，往往需要各种昂贵的耗材和高端设备。为了制备高通量实时PCR检测所需的DNA模板，本研究对Naklha et al.(2010)使用普通实验室设备从线虫悬浮液中提取DNA的传统方法进行了改进，取得了与其他两种传统方法相当的结果和优势。实时荧光定量PCR检测结果与形态学计数结果高度相关，灵敏度与两种常规方法相当或更高。虽然新方案需要100分钟以上的DNA提取，人工处理只需要不到10分钟，即其他方法的一半到四分之一。运行成本不到其他方法的一半到十分之一。Nematol。Res. 48(1)， 1 - 10(2018)。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Nematological Research (Japanese Journal of Nematology)

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