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对受污染土壤和地下水中蛋白质提取物进行的功能宏蛋白质组分析。

Functional metaproteome analysis of protein extracts from contaminated soil and groundwater.

作者信息

Benndorf Dirk, Balcke Gerd U, Harms Hauke, von Bergen Martin

机构信息

Department of Proteomics, UFZ-Helmholtz Centre for Environmental Research, Leipzig, Germany.

出版信息

ISME J. 2007 Jul;1(3):224-34. doi: 10.1038/ismej.2007.39. Epub 2007 May 31.

DOI:10.1038/ismej.2007.39
PMID:18043633
Abstract

Using proteins from soil or groundwater as functional biomarkers requires efficient extraction. We developed an extraction method in which the separation of proteins from the inorganic and organic constituents of the soil matrix was achieved by a combination of 0.1 M NaOH treatment and phenol extraction. Incubation with NaOH released humic acids and proteins from soil minerals, and simultaneously, disrupted microorganisms. The subsequent phenol extraction separated the proteins from the humic organic matter. Protein extracts were applied to sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and 2D-electrophoresis (2-DE). Spots and bands were excised and individual proteins identified by liquid chromatography online linked to mass spectrometry (MS) via electrospray ionization source (LC-ESI-MS). To assess the suitability of the method for the functional analysis of environmental metaproteomes, it was applied to soil that had been enriched in chlorophenoxy acid-degrading bacteria by incubation with 2,4-dichlorophenoxy acetic acid (2,4-D) for 22 days. The method was also used to analyze groundwater from the aquifer of a chlorobenzene-contaminated site. The identification of enzymes such as chlorocatechol dioxygenases was consistent with bacterial metabolic pathways expected to be expressed in these samples. The protocol enabled thus the analysis of the metaproteome of soil and groundwater samples. It thereby provides a means to study the diversity of environmental microbial communities while addressing functional aspects more directly than metagenome or even metatranscriptome analysis.

摘要

将土壤或地下水中的蛋白质用作功能生物标志物需要高效提取。我们开发了一种提取方法,通过0.1 M NaOH处理和苯酚提取相结合,实现了从土壤基质的无机和有机成分中分离蛋白质。用NaOH孵育可从土壤矿物质中释放腐殖酸和蛋白质,同时破坏微生物。随后的苯酚提取将蛋白质与腐殖有机物质分离。将蛋白质提取物应用于十二烷基硫酸钠聚丙烯酰胺凝胶电泳(SDS-PAGE)和二维电泳(2-DE)。切下斑点和条带,并通过液相色谱在线连接到通过电喷雾电离源(LC-ESI-MS)的质谱(MS)来鉴定单个蛋白质。为了评估该方法对环境宏蛋白质组功能分析的适用性,将其应用于通过与2,4-二氯苯氧基乙酸(2,4-D)孵育22天而富集了氯苯氧基酸降解细菌的土壤。该方法还用于分析来自氯苯污染场地含水层的地下水。对诸如氯儿茶酚双加氧酶等酶的鉴定与预期在这些样品中表达的细菌代谢途径一致。该方案因此能够分析土壤和地下水样品的宏蛋白质组。从而提供了一种研究环境微生物群落多样性的手段,同时比宏基因组甚至宏转录组分析更直接地解决功能方面的问题。

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