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通过 454 焦磷酸测序分析环境水样中的细菌群落中活细胞与死细胞的区分。

Discrimination between live and dead cellsin bacterial communities from environmental water samples analyzed by 454 pyrosequencing.

机构信息

TNO Quality of Life, Business Unit Food and Biotechnology Innovations, Microbial Genomics Group, Zeist, Netherlands.

出版信息

Int Microbiol. 2010 Jun;13(2):59-65. doi: 10.2436/20.1501.01.111.

Abstract

The preferential detection of cells with intact membranes by sample treatment with propidium monoazide (PMA) in combination with PCR amplification is gaining in popularity. This study evaluates the effect of PMA on 454 pyrosequencing profiles of environmental water samples from a canal in Amsterdam and seawater (with sediment) left untreated or exposed to elevated temperatures (50, 60, or 85 °C) for 10 min. Community analysis was based on the extraction of genomic DNA followed by PCR amplification of 16S rRNA genes using universal bacterial primers. Whereas the highest temperature in combination with PMA treatment completely suppressed PCR amplification, PCR products from the other samples were subjected to massively parallel tag sequencing. PMA treatment did not substantially affect the sequence profiles of non-heated samples, but heat exposure resulted in a clear difference in the relative proportions of certain groups. This difference was significantly more pronounced in heated seawater than in heated canal water. The effect of the chosen experimental conditions on the membrane integrity of cells was supported by BacLight LIVE/DEAD staining in combination with flow cytometry, which confirmed an increase in the uptake of propidium iodide in samples exposed to high temperatures.

摘要

吖啶橙(PMA)与聚合酶链反应(PCR)联合应用于样本处理,可优先检测到完整细胞膜的细胞,该方法的应用日益广泛。本研究评估了吖啶橙对阿姆斯特丹运河环境水样和未经处理海水(含沉积物)以及经高温(50、60 或 85°C)处理 10 分钟海水的 454 焦磷酸测序图谱的影响。基于提取基因组 DNA,采用通用细菌引物对 16S rRNA 基因进行 PCR 扩增,然后进行群落分析。虽然高温联合吖啶橙处理完全抑制了 PCR 扩增,但其他样品的 PCR 产物进行了大规模平行标签测序。吖啶橙处理对未加热样本的序列图谱没有显著影响,但热暴露导致某些群体的相对比例明显不同。与加热后的运河水相比,加热后的海水差异更为显著。BacLight LIVE/DEAD 染色结合流式细胞术证实了高温暴露样本中碘化丙啶摄取量的增加,这支持了所选实验条件对细胞膜完整性的影响。

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