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Estimating High-Affinity Methanotrophic Bacterial Biomass, Growth, and Turnover in Soil by Phospholipid Fatty Acid 13C Labeling

机译:通过磷脂脂肪酸13C标记估算土壤中的高亲和力甲烷营养细菌生物量,生长和周转

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摘要

A time series phospholipid fatty acid (PLFA) 13C-labeling study was undertaken to determine methanotrophic taxon, calculate methanotrophic biomass, and assess carbon recycling in an upland brown earth soil from Bronydd Mawr (Wales, United Kingdom). Laboratory incubations of soils were performed at ambient CH4 concentrations using synthetic air containing 2 parts per million of volume of 13CH4. Flowthrough chambers maintained a stable CH4 concentration throughout the 11-week incubation. Soils were analyzed at weekly intervals by gas chromatography (GC), GC-mass spectrometry, and GC-combustion-isotope ratio mass spectrometry to identify and quantify individual PLFAs and trace the incorporation of 13C label into the microbial biomass. Incorporation of the 13C label was seen throughout the experiment, with the rate of incorporation decreasing after 9 weeks. The δ13C values of individual PLFAs showed that 13C label was incorporated into different components to various extents and at various rates, reflecting the diversity of PLFA sources. Quantitative assessments of 13C-labeled PLFAs showed that the methanotrophic population was of constant structure throughout the experiment. The dominant 13C-labeled PLFA was 18:1ω7c, with 16:1ω5 present at lower abundance, suggesting the presence of novel type II methanotrophs. The biomass of methane-oxidizing bacteria at optimum labeling was estimated to be about 7.2 × 106 cells g−1 of soil (dry weight). While recycling of 13C label from the methanotrophic biomass must occur, it is a slower process than initial 13CH4 incorporation, with only about 5 to 10% of 13C-labeled PLFAs reflecting this process. Thus, 13C-labeled PLFA distributions determined at any time point during 13CH4 incubation can be used for chemotaxonomic assessments, although extended incubations are required to achieve optimum 13C labeling for methanotrophic biomass determinations.
机译:进行了时间序列磷脂脂肪酸(PLFA)13C标记研究,以确定甲烷营养类群,计算甲烷营养生物量,并评估了来自Bronydd Mawr(英国威尔士)的山地棕壤土壤中的碳再循环。使用环境空气中CH4浓度的土壤进行实验室温育,使用的空气中含有百万分之二的13CH4。在整个11周的温育过程中,流通室均保持稳定的CH4浓度。通过气相色谱(GC),GC-质谱和GC-燃烧-同位素比质谱法每周对土壤进行分析,以鉴定和定量各个PLFA,并跟踪将13C标签掺入微生物生物量中。在整个实验过程中均观察到13C标签的掺入,掺入率在9周后下降。单个PLFA的δ13C值表明13C标签以不同的程度和速率掺入了不同的组分,反映了PLFA来源的多样性。对13 C标记的PLFA进行定量评估表明,甲烷营养型种群在整个实验过程中具有恒定的结构。占优势的13C标记的PLFA为18:1ω7c,而16:1ω5的丰度较低,表明存在新的II型甲烷营养生物。在最佳标记条件下,甲烷氧化细菌的生物量估计约为7.2×106细胞g-1(干重)。虽然必须从甲烷营养型生物质中回收13C标签,但该过程比初始13CH4掺入的过程要慢,只有大约5%至10%的13C标记的PLFA反映了这一过程。因此,在13CH4孵育过程中的任何时间点确定的13C标记PLFA分布都可用于化学分类评估,尽管需要进行长时间孵育才能获得用于甲烷营养生物质测定的最佳13C标记。

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