Osaka Toshifumi, Yoshie Sachiko, Tsuneda Satoshi, Hirata Akira, Iwami Norio, Inamori Yuhei
Department of Chemical Engineering, Waseda University, 3-4-1 Ohkubo, Shinjuku-ku, Tokyo 169-8555, Japan.
Microb Ecol. 2006 Aug;52(2):253-66. doi: 10.1007/s00248-006-9071-7. Epub 2006 Aug 5.
Stable-isotope probing (SIP) was used to identify acetate- or methanol-assimilating bacteria under nitrate-reducing conditions in activated sludge. A sludge sample obtained from wastewater treatment systems was incubated in a denitrifying batch reactor fed with synthetic wastewater containing [(13)C]acetate or [(13)C]methanol as the main carbon source and nitrate as the electron acceptor. We analyzed how growth of bacterial populations was stimulated by acetate or methanol as the external carbon source in nitrogen-removal systems. Most of the acetate- or methanol-assimilating bacteria identified by SIP have been known as denitrifiers in wastewater treatment systems. When acetate was used as the carbon source, 16S rRNA gene sequences retrieved from (13)C-labeled DNA were closely related to the 16S rRNA genes of Comamonadaceae (e.g., Comamonas and Acidovorax) and Rhodocyclaceae (e.g., Thauera and Dechloromonas) of the Betaproteobacteria, and Rhodobacteraceae (e.g., Paracoccus and Rhodobacter) of the Alphaproteobacteria. When methanol was used as the carbon source, 16S rRNA gene sequences retrieved from (13)C-DNA were affiliated with Methylophilaceae (e.g., Methylophilus, Methylobacillus, and Aminomonas) and Hyphomicrobiaceae. Rarefaction curves for clones retrieved from (13)C-DNA showed that the diversity levels for methanol-assimilating bacteria were considerably lower than those for acetate-assimilating bacteria. Furthermore, we characterized nitrite reductase genes (nirS and nirK) as functional marker genes for denitrifier communities in acetate- or methanol-assimilating populations and detected the nirS or nirK sequence related to that of some known pure cultures, such as Alcaligenes, Hyphomicrobium, and Thauera. However, most of the nirS or nirK sequences retrieved from (13)C-DNA were clustered in some unidentified groups. On the basis of 16S rRNA gene clone libraries retrieved from (13)C-DNA, these unidentified nir sequences might be identified by examining the nir gene in candidates for true denitrifiers (e.g., the families Comamonadaceae, Hyphomicrobiaceae, Methylophilaceae, and Rhodobacteraceae).
采用稳定同位素探知技术(SIP),以识别活性污泥中在硝酸盐还原条件下同化乙酸盐或甲醇的细菌。从废水处理系统采集污泥样本,在一个反硝化间歇式反应器中进行培养,该反应器中加入含有[(13)C]乙酸盐或[(13)C]甲醇作为主要碳源以及硝酸盐作为电子受体的合成废水。我们分析了在脱氮系统中,作为外部碳源的乙酸盐或甲醇如何刺激细菌种群的生长。通过SIP识别出的大多数同化乙酸盐或甲醇的细菌在废水处理系统中被认为是反硝化菌。当使用乙酸盐作为碳源时,从(13)C标记的DNA中检索到的16S rRNA基因序列与β-变形菌纲的丛毛单胞菌科(如丛毛单胞菌属和嗜酸菌属)、红环菌科(如陶厄氏菌属和脱氯单胞菌属)以及α-变形菌纲的红杆菌科(如副球菌属和红杆菌属)的16S rRNA基因密切相关。当使用甲醇作为碳源时,从(13)C-DNA中检索到的16S rRNA基因序列隶属于嗜甲基菌科(如嗜甲基菌属、甲基芽孢杆菌属和氨基单胞菌属)和生丝微菌科。从(13)C-DNA中检索到的克隆的稀释曲线表明,同化甲醇的细菌的多样性水平显著低于同化乙酸盐的细菌。此外,我们将亚硝酸还原酶基因(nirS和nirK)作为反硝化菌群落中乙酸盐或甲醇同化菌群的功能标记基因进行表征,并检测到与一些已知纯培养物(如产碱菌属、生丝微菌属和陶厄氏菌属)相关的nirS或nirK序列。然而,从(13)C-DNA中检索到的大多数nirS或nirK序列聚集在一些未鉴定的组中。基于从(13)C-DNA中检索到的16S rRNA基因克隆文库,通过检测真正反硝化菌(如丛毛单胞菌科、生丝微菌科、嗜甲基菌科和红杆菌科)候选菌株中的nir基因,这些未鉴定的nir序列可能会被识别出来。
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