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应用基于分类单元的 PCR 和变性高效液相色谱(PCR-DHPLC)技术对热带湖泊沉积物中的硅藻组合进行分子特征分析。

Molecular profiling of diatom assemblages in tropical lake sediments using taxon-specific PCR and Denaturing High-Performance Liquid Chromatography (PCR-DHPLC).

机构信息

Unit of Evolutionary Biology/Systematic Zoology, Institute of Biochemistry and Biology, University of Potsdam, Karl-Liebknecht-Strasse 24-25, Haus 26, D-14476 Potsdam, Germany.

出版信息

Mol Ecol Resour. 2011 Sep;11(5):842-53. doi: 10.1111/j.1755-0998.2011.03022.x. Epub 2011 May 19.

DOI:10.1111/j.1755-0998.2011.03022.x
PMID:21592311
Abstract

Here we present a protocol to genetically detect diatoms in sediments of the Kenyan tropical Lake Naivasha, based on taxon-specific PCR amplification of short fragments (approximately 100 bp) of the small subunit ribosomal (SSU) gene and subsequent separation of species-specific PCR products by PCR-based denaturing high-performance liquid chromatography (DHPLC). An evaluation of amplicons differing in primer specificity to diatoms and length of the fragments amplified demonstrated that the number of different diatom sequence types detected after cloning of the PCR products critically depended on the specificity of the primers to diatoms and the length of the amplified fragments whereby shorter fragments yielded more species of diatoms. The DHPLC was able to discriminate between very short amplicons based on the sequence difference, even if the fragments were of identical length and if the amplicons differed only in a small number of nucleotides. Generally, the method identified the dominant sequence types from mixed amplifications. A comparison with microscopic analysis of the sediment samples revealed that the sequence types identified in the molecular assessment corresponded well with the most dominant species. In summary, the PCR-based DHPLC protocol offers a fast, reliable and cost-efficient possibility to study DNA from sediments and other environmental samples with unknown organismic content, even for very short DNA fragments.

摘要

在这里,我们提出了一种基于特定于分类群的 PCR 扩增小亚基核糖体 (SSU) 基因的短片段(约 100bp),并随后通过基于 PCR 的变性高效液相色谱 (DHPLC) 分离物种特异性 PCR 产物的方法,从肯尼亚热带纳瓦沙湖沉积物中遗传检测硅藻的方案。对针对硅藻的引物特异性和扩增片段长度不同的扩增子的评估表明,在克隆 PCR 产物后检测到的不同硅藻序列类型的数量取决于硅藻的引物特异性和扩增片段的长度,其中较短的片段产生更多的硅藻物种。DHPLC 能够根据序列差异区分非常短的扩增子,即使片段长度相同,并且扩增子仅在少数核苷酸上存在差异。通常,该方法可从混合扩增中鉴定出主要序列类型。与沉积物样本的显微镜分析进行比较表明,分子评估中鉴定的序列类型与最主要的物种非常吻合。总之,基于 PCR 的 DHPLC 方案为研究沉积物和其他具有未知生物含量的环境样本中的 DNA 提供了一种快速、可靠且具有成本效益的可能性,即使是对于非常短的 DNA 片段也是如此。

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