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不同电子供体对甲基营养型反硝化细菌分子微生物生态学和生物动力学的影响

Impact of varying electron donors on the molecular microbial ecology and biokinetics of methylotrophic denitrifying bacteria.

作者信息

Baytshtok Vladimir, Lu Huijie, Park Hongkeun, Kim Sungpyo, Yu Ran, Chandran Kartik

机构信息

Department of Earth and Environmental Engineering, Columbia University, New York, New York 10027, USA.

出版信息

Biotechnol Bioeng. 2009 Apr 15;102(6):1527-36. doi: 10.1002/bit.22213.

Abstract

The goal of this study was to identify bacterial populations that assimilated methanol in a denitrifying sequencing batch reactor (SBR), using stable isotope probing (SIP) of (13)C labeled DNA and quantitatively track changes in these populations upon changing the electron donor from methanol to ethanol in the SBR feed. Based on SIP derived (13)C 16S rRNA gene clone libraries, dominant SBR methylotrophic bacteria were related to Methyloversatilis spp. and Hyphomicrobium spp. These methylotrophic populations were quantified via newly developed real-time PCR assays. Upon switching the electron donor from methanol to ethanol, Hyphomicrobium spp. concentrations decreased significantly in accordance with their obligately methylotrophic nutritional mode. In contrast, Methyloversatilis spp. concentrations were relatively unchanged, in accordance with their ability to assimilate both methanol and ethanol. Direct assimilation of ethanol by Methyloversatilis spp. but not Hyphomicrobium spp. was also confirmed via SIP. The reduction in methylotrophic bacterial concentration upon switching to ethanol was paralleled by a significant decrease in the methanol supported denitrification biokinetics of the SBR on nitrate. In sum, the results of this study demonstrate that the metabolic capabilities (methanol assimilation and metabolism) and substrate specificity (obligately or facultatively methylotrophic) of two distinct methylotrophic bacterial populations contributed to their survival or washout in denitrifying bioreactors.

摘要

本研究的目标是在反硝化序批式反应器(SBR)中,利用对(13)C标记DNA的稳定同位素探测(SIP)来识别同化甲醇的细菌群落,并在SBR进料中将电子供体从甲醇改为乙醇时,定量追踪这些群落的变化。基于SIP衍生的(13)C 16S rRNA基因克隆文库,SBR中占主导地位的甲基营养细菌与嗜甲基菌属和生丝微菌属有关。这些甲基营养菌群落通过新开发的实时PCR测定法进行定量。当将电子供体从甲醇切换为乙醇时,生丝微菌属的浓度根据其专性甲基营养营养模式而显著下降。相比之下,嗜甲基菌属的浓度相对不变,这与其同化甲醇和乙醇的能力一致。通过SIP还证实了嗜甲基菌属可直接同化乙醇,而生丝微菌属则不能。切换到乙醇后甲基营养细菌浓度的降低与SBR对硝酸盐的甲醇支持反硝化生物动力学的显著下降同时发生。总之,本研究结果表明,两个不同甲基营养细菌群落的代谢能力(甲醇同化和代谢)和底物特异性(专性或兼性甲基营养)导致了它们在反硝化生物反应器中的存活或被冲刷掉。

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