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Microbial community of a mesophilic propionate-degrading methanogenic consortium in chemostat cultivation analyzed based on 16S rRNA and acetate kinase genes

机译:基于16S rRNA和乙酸激酶基因分析的常温降解嗜温丙酸产甲烷菌群的微生物群落。

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We constructed a mesophilic anaerobic chemostat that was continuously fed with synthetic wastewater containing propionate as the sole source of carbon and energy. Steady-state conditions were achieved below the critical dilution rate of 0.3 d(-1) supercript stop with almost complete substrate degradation. The propionate-degrading methanogenic communities in the chemostat at dilution rates of 0.01, 0.08, and 0.3 d(-1) supercript stop were analyzed using molecular biological techniques. Fluorescence in situ hybridization with archaeal and bacterial domain-specific probes showed that archaeal cells predominated throughout the three dilution rates. Archaeal-16S rRNA gene clone library analysis and quantitative real-time polymerase chain reaction studies showed that hydrogenotrophic methanogen rRNA genes closely related to Methanoculleus was detected at a dilution rate of 0.01 d(-1) supercript stop , whereas rRNA genes closely related to the Methanoculleus and Methanospirillum genera were detected at dilution rates of 0.08 and 0.3 d(-1) supercript stop . The aceticlastic methanogen, Methanosaeta , was detected throughout the three dilution rates. Bacterial-rRNA gene clone library analysis and denaturing gradient gel electrophoresis demonstrated that rRNA genes affiliated with the genus Syntrophobacter predominated at the low dilution rate, whereas rRNA genes affiliated with the phylum Firmicutes predominated at the higher dilution rates. A significant number of rRNA genes affiliated with the genus Pelotomaculum were detected at dilution rate of 0.3 d(-1) supercript stop . The diversity of genes encoding acetate kinase agreed closely with the results of the rRNA gene analysis. The dilution rates significantly altered the archaeal and bacterial communities in the propionate-fed chemostat.
机译:我们构建了一个中温厌氧型化学恒温器,该恒温器连续供入含有丙酸酯作为唯一碳和能源的合成废水。在几乎完全降解底物的0.3 d(-1)超临界停止临界稀释速率以下,实现了稳态条件。使用分子生物学技术分析了稀释度为0.01、0.08和0.3 d(-1)的超临界点在恒化器中降解丙酸的产甲烷菌群落。与古细菌和细菌域特异性探针的荧光原位杂交表明,古细菌细胞在三种稀释率中均占主导。 Archaeal-16S rRNA基因克隆文库分析和定量实时聚合酶链反应研究表明,在0.01 d(-1)的超临界点稀释率下检测到与甲烷菌密切相关的氢营养型产甲烷菌rRNA基因,而与该酶密切相关的rRNA基因。以0.08和0.3 d(-1)的超临界点稀释率检测到甲烷菌属和甲烷螺旋菌属。在三个稀释率中均检测到了乙腈产甲烷菌Methanosaeta。细菌rRNA基因克隆文库分析和变性梯度凝胶电泳表明,与滑膜菌属有关的rRNA基因在较低的稀释率下占优势,而与Firmicutes门属有关的rRNA基因在较高的稀释率下占优势。在稀释倍数为0.3 d(-1)的超临界点稀释液中检测到大量与Pelotomaculum属有关的rRNA基因。编码乙酸激酶的基因的多样性与rRNA基因分析的结果非常吻合。稀释率显着改变了丙酸盐喂养的恒化器中的古细菌和细菌群落。

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