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对六个水生态环境的宏蛋白质组学调查:发现参与生物地球化学循环的微生物种群的身份。

Metaproteomic survey of six aquatic habitats: discovering the identities of microbial populations active in biogeochemical cycling.

机构信息

Department of Microbiology, B57A Wing Hall, Cornell University, Ithaca, NY, 14853, USA.

出版信息

Microb Ecol. 2014 Apr;67(3):520-39. doi: 10.1007/s00248-013-0346-5. Epub 2014 Jan 15.

Abstract

Our goal is to strengthen the foundations of metaproteomics as a microbial community analysis tool that links the functional identity of actively expressed gene products with host phylogeny. We used shotgun metaproteomics to survey waters in six disparate aquatic habitats (Cayuga Lake, NY; Oneida Lake, NY; Gulf of Maine; Chesapeake Bay, MD; Gulf of Mexico; and the South Pacific). Peptide pools prepared from filter-gathered microbial biomass, analyzed by nano-liquid chromatography-mass spectrometry (MS/MS) generating 9,693 ± 1,073 mass spectra identified 326 ± 107 bacterial proteins per sample. Distribution of proteobacterial (Alpha and Beta) and cyanobacterial (Prochlorococcus and Synechococcus spp.) protein hosts across all six samples was consistent with the previously published biogeography for these microorganisms. Marine samples were enriched in transport proteins (TRAP-type for dicarboxylates and ATP binding cassette (ABC)-type for amino acids and carbohydrates) compared with the freshwater samples. We were able to match in situ expression of many key proteins catalyzing C-, N-, and S-cycle processes with their bacterial hosts across all six habitats. Pelagibacter was identified as the host of ABC-type sugar-, organic polyanion-, and glycine betaine-transport proteins; this extends previously published studies of Pelagibacter's in situ biogeochemical role in marine C- and N-metabolism. Proteins matched to Ruegeria confirmed these organism's role in marine waters oxidizing both carbon monoxide and sulfide. By documenting both processes expressed in situ and the identity of host cells, metaproteomics tested several existing hypotheses about ecophysiological processes and provided fodder for new ones.

摘要

我们的目标是加强宏蛋白质组学作为一种微生物群落分析工具的基础,将功能明确的活跃表达基因产物与宿主系统发育联系起来。我们使用鸟枪法宏蛋白质组学调查了六个不同水生栖息地(纽约州的卡尤加湖、纽约州的奥奈达湖、缅因湾、切萨皮克湾、墨西哥湾和南太平洋)的水。从过滤收集的微生物生物量中制备肽池,通过纳升液相色谱-质谱(MS/MS)分析,生成 9693±1073 个质谱,每个样品鉴定出 326±107 种细菌蛋白。所有六个样品中变形菌(α和β)和蓝细菌(聚球藻和聚球藻属)蛋白宿主的分布与这些微生物的先前发表的生物地理学一致。与淡水样本相比,海洋样本富含转运蛋白(二羧酸的 TRAP 型和氨基酸和碳水化合物的 ABC 型)。我们能够将许多催化 C、N 和 S 循环过程的关键蛋白与它们在所有六个栖息地的细菌宿主进行原位表达相匹配。与 ABC 型糖、有机多阴离子和甘氨酸甜菜碱转运蛋白的宿主是 Pelagibacter;这扩展了 Pelagibacter 在海洋 C 和 N 代谢中原位生物地球化学作用的先前发表研究。与 Ruegeria 匹配的蛋白证实了这些生物体在海洋水中氧化一氧化碳和硫化物的作用。通过记录原位表达的两种过程和宿主细胞的身份,宏蛋白质组学检验了一些关于生态生理过程的现有假设,并为新的假设提供了依据。

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