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Use of Field-Based Stable Isotope Probing To Identify Adapted Populations and Track Carbon Flow through a Phenol-Degrading Soil Microbial Community

机译:使用基于场的稳定同位素探测来识别适应的种群并追踪通过苯酚降解土壤微生物群落的碳流

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摘要

The goal of this field study was to provide insight into three distinct populations of microorganisms involved in in situ metabolism of phenol. Our approach measured 13CO2 respired from [13C]phenol and stable isotope probing (SIP) of soil DNA at an agricultural field site. Traditionally, SIP-based investigations have been subject to the uncertainties posed by carbon cross-feeding. By altering our field-based, substrate-dosing methodologies, experiments were designed to look beyond primary degraders to detect trophically related populations in the food chain. Using gas chromatography-mass spectrometry (GC/MS), it was shown that 13C-labeled biomass, derived from primary phenol degraders in soil, was a suitable growth substrate for other members of the soil microbial community. Next, three dosing regimes were designed to examine active members of the microbial community involved in phenol metabolism in situ: (i) 1 dose of [13C]phenol, (ii) 11 daily doses of unlabeled phenol followed by 1 dose of [13C]phenol, and (iii) 12 daily doses of [13C]phenol. GC/MS analysis demonstrated that prior exposure to phenol boosted 13CO2 evolution by a factor of 10. Furthermore, imaging of 13C-treated soil using secondary ion mass spectrometry (SIMS) verified that individual bacteria incorporated 13C into their biomass. PCR amplification and 16S rRNA gene sequencing of 13C-labeled soil DNA from the 3 dosing regimes revealed three distinct clone libraries: (i) unenriched, primary phenol degraders were most diverse, consisting of α-, β-, and γ-proteobacteria and high-G+C-content gram-positive bacteria, (ii) enriched primary phenol degraders were dominated by members of the genera Kocuria and Staphylococcus, and (iii) trophically related (carbon cross-feeders) were dominated by members of the genus Pseudomonas. These data show that SIP has the potential to document population shifts caused by substrate preexposure and to follow the flow of carbon through terrestrial microbial food chains.
机译:这项实地研究的目的是深入了解参与苯酚原位代谢的三种微生物。我们的方法测量了在农田现场从[13C]苯酚呼吸的13CO2和土壤DNA的稳定同位素探测(SIP)。传统上,基于SIP的调查受到碳交叉喂入带来的不确定性的影响。通过改变我们基于现场的底物计量方法,设计了一些实验,以超越主要降解菌的范围,以检测食物链中与营养相关的种群。使用气相色谱-质谱法(GC / MS),表明13C标记的生物质源自土壤中的主要酚降解物,是土壤微生物群落其他成员的合适生长底物。接下来,设计了三种给药方案以检查参与原位酚代谢的微生物群落的活跃成员:(i)1剂量的[13C]苯酚,(ii)11剂量的未标记苯酚,然后是1剂量的[13C]苯酚和(iii)12每日剂量的[13C]苯酚。 GC / MS分析表明,事先暴露于苯酚会使13CO2的释放增加10倍。此外,使用二次离子质谱(SIMS)对13C处理过的土壤成像的结果证实,个别细菌将13C掺入了生物量。从3种给药方案对13C标记的土壤DNA进行的PCR扩增和16S rRNA基因测序显示了三个不同的克隆文库:(i)未富集的初级酚降解物种类最多,由α-,β-和γ变形杆菌组成,并且-G + C含量的革兰氏阳性细菌,(ii)富集的一级酚降解剂由Kocuria和葡萄球菌属的成员主导,(iii)与营养相关的(碳交叉供体)由假单胞菌属的成员主导。这些数据表明,SIP有潜力记录底物预暴露引起的种群转移,并追踪碳通过陆地微生物食物链的流动。

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