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Validation of Heavy-Water Stable Isotope Probing for the Characterization of Rapidly Responding Soil Bacteria

机译:重水稳定同位素探查用于快速响应土壤细菌特征的验证

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摘要

Rapid responses of bacteria to sudden changes in their environment can have important implications for the structure and function of microbial communities. In this study, we used heavy-water stable isotope probing (H218O-SIP) to identify bacteria that respond to soil rewetting. First, we conducted experiments to address uncertainties regarding the H218O-SIP method. Using liquid chromatography-mass spectroscopy (LC-MS), we determined that oxygen from H218O was incorporated into all structural components of DNA. Although this incorporation was uneven, we could effectively separate 18O-labeled and unlabeled DNAs derived from laboratory cultures and environmental samples that were incubated with H218O. We found no evidence for ex vivo exchange of oxygen atoms between DNA and extracellular H2O, suggesting that 18O incorporation into DNA is relatively stable. Furthermore, the rate of 18O incorporation into bacterial DNA was high (within 48 to 72 h), coinciding with pulses of CO2 generated from soil rewetting. Second, we examined shifts in the bacterial composition of grassland soils following rewetting, using H218O-SIP and bar-coded pyrosequencing of 16S rRNA genes. For some groups of soil bacteria, we observed coherent responses at a relatively course taxonomic resolution. Following rewetting, the relative recovery of Alphaproteobacteria, Betaproteobacteria, and Gammaproteobacteria increased, while the relative recovery of Chloroflexi and Deltaproteobacteria decreased. Together, our results suggest that H218O-SIP is effective at identifying metabolically active bacteria that influence soil carbon dynamics. Our results contribute to the ecological classification of soil bacteria while providing insight into some of the functional traits that influence the structure and function of microbial communities under dynamic soil moisture regimes.
机译:细菌对环境突然变化的快速响应可能会对微生物群落的结构和功能产生重要影响。在这项研究中,我们使用重水稳定同位素探测(H2 18 O-SIP)来识别对土壤重新润湿有反应的细菌。首先,我们进行了实验,以解决有关H2 18 O-SIP方法的不确定性。使用液相色谱-质谱法(LC-MS),我们确定来自H2 18 O的氧已被掺入DNA的所有结构成分中。尽管掺入不均匀,但我们可以有效地分离由实验室培养物和与H2 18 O孵育的环境样品得到的 18 O标记和未标记的DNA。我们发现没有证据表明DNA与细胞外H2O之间存在氧原子的离体交换,这表明 18 O掺入DNA相对稳定。此外, 18 O掺入细菌DNA的速率很高(在48至72小时内),这与土壤重新湿润产生的CO2脉冲一致。其次,我们使用H2 18 O-SIP和条形码16S rRNA基因的焦磷酸测序技术,研究了再润湿后草原土壤细菌组成的变化。对于某些类型的土壤细菌,我们在相对分类的分辨率下观察到相干响应。重新润湿后,α-变形杆菌,β-变形杆菌和γ-变形杆菌的相对恢复增加,而绿弯曲菌和δ变形杆菌的相对恢复则下降。总之,我们的结果表明,H2 18 O-SIP可有效识别影响土壤碳动态的代谢活性细菌。我们的结果有助于土壤细菌的生态学分类,同时提供洞察力在动态土壤水分条件下影响微生物群落结构和功能的某些功能性状。

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