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首页> 外文期刊>African Journal of Microbiology Research >Choice of DNA extraction protocols from Gram negative and positive bacteria and directly from the soil
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Choice of DNA extraction protocols from Gram negative and positive bacteria and directly from the soil

机译:从革兰氏阴性和阳性细菌以及直接从土壤中提取DNA的方法

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DNA extraction is a fundamentally important step for the implementation of genotypic techniques in microbial identification, and the use of such techniques has become essential for the analysis of soil microbial diversity. Considering culture independent methodologies, it is still necessary to ensure that DNA is extracted in appropriate amounts and that extracted DNA is inhibitor-free. This study aimed at selecting a single protocol suitable for the extraction of total DNA from Gram positive and negative bacteria isolated from different sources, as well as a protocol for the direct extraction of DNA from soil. Four experimental protocols and a commercial kit were tested for the extraction of total DNA from isolated bacteria. Among the protocols, the detergent + salt + thermal incubation method (based on Harju et al., 2004) was considered the most promising because it produced satisfactory yields of DNA, with adequate quality for all isolates studied, especially Staphylococcus aureus, without the need to use enzymes and glass beads which can make the extraction process more expensive. Three experimental protocols and the commercial kit were tested for the direct extraction of DNA from soil. Regarding PCR amplification, the amount of total DNA extracted is less limiting than its quality. Thus, commercial kit PowerMax? Soil DNA Isolation (MoBio) offered more promising results, because although this provided low yields of DNA, it was sufficient for polymerase chain reaction (PCR) amplification.
机译:DNA提取是在微生物鉴定中实施基因型技术的根本重要步骤,而使用此类技术已成为分析土壤微生物多样性必不可少的步骤。考虑到与培养无关的方法,仍然有必要确保以适当的量提取DNA,并且所提取的DNA不含抑制剂。这项研究旨在选择一种适用于从不同来源分离的革兰氏阳性和阴性细菌中提取总DNA的方案,以及直接从土壤中提取DNA的方案。测试了四个实验方案和一个商业试剂盒,用于从分离的细菌中提取总DNA。在方案中,去污剂+盐+热孵育方法(基于Harju等,2004)被认为是最有前途的,因为它可以产生令人满意的DNA产量,并且对于所有研究的分离物(尤其是金黄色葡萄球菌)都具有足够的质量,而无需使用酶和玻璃珠会使提取过程更加昂贵。测试了三种实验方案和商业试剂盒,用于从土壤中直接提取DNA。关于PCR扩增,提取的总DNA量比其质量要少。因此,商业套件PowerMax?土壤DNA分离(MoBio)提供了更可观的结果,因为尽管这提供了低DNA产量,但足以用于聚合酶链反应(PCR)扩增。

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