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淡水真核微藻 DNA 提取方法的评估。

Evaluation of DNA extraction methods for freshwater eukaryotic microalgae.

机构信息

Newcastle University, School of Civil Engineering of Geosciences, Newcastle upon Tyne NE1 7RU, United Kingdom.

出版信息

Water Res. 2012 Oct 15;46(16):5355-64. doi: 10.1016/j.watres.2012.07.023. Epub 2012 Jul 24.

Abstract

The use of molecular methods to investigate microalgal communities of natural and engineered freshwater resources is in its infancy, with the majority of previous studies carried out by microscopy. Inefficient or differential DNA extraction of microalgal community members can lead to bias in downstream community analysis. Three commercially available DNA extraction kits have been tested on a range of pure culture freshwater algal species with diverse cell walls and mixed algal cultures taken from eutrophic waste stabilization ponds (WSP). DNA yield and quality were evaluated, along with DNA suitability for amplification of 18S rRNA gene fragments by polymerase chain reaction (PCR). QiagenDNeasy(®) Blood and Tissue kit (QBT), was found to give the highest DNA yields and quality. Denaturant Gradient Gel Electrophoresis (DGGE) was used to assess the diversity of communities from which DNA was extracted. No significant differences were found among kits when assessing diversity. QBT is recommended for use with WSP samples, a conclusion confirmed by further testing on communities from two tropical WSP systems. The fixation of microalgal samples with ethanol prior to DNA extraction was found to reduce yields as well as diversity and is not recommended.

摘要

利用分子方法研究天然和人工淡水资源中的微藻群落尚处于起步阶段,大多数先前的研究都是通过显微镜进行的。微藻群落成员的 DNA 提取效率低下或存在差异,可能会导致下游群落分析出现偏差。本研究测试了三种市售的 DNA 提取试剂盒,分别对具有不同细胞壁的一系列纯培养淡水藻类物种以及富营养化废水稳定塘(WSP)中的混合藻类培养物进行了测试。评估了 DNA 的产量和质量,以及聚合酶链反应(PCR)扩增 18S rRNA 基因片段的适用性。研究发现,QiagenDNeasy(®) Blood and Tissue kit(QBT)试剂盒可获得最高的 DNA 产量和质量。变性梯度凝胶电泳(DGGE)用于评估提取 DNA 的群落多样性。在评估多样性时,三种试剂盒之间没有发现显著差异。建议在使用 WSP 样品时使用 QBT,这一结论通过对来自两个热带 WSP 系统的群落的进一步测试得到了证实。研究发现,在提取 DNA 之前用乙醇固定微藻样品会降低产量和多样性,因此不建议这样做。

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