在高稀释率下,用抗性淀粉对人粪便进行恒化器富集培养,对黏附性产丁酸梭菌具有选择性。
Chemostat enrichments of human feces with resistant starch are selective for adherent butyrate-producing clostridia at high dilution rates.
作者信息
Sharp R, Macfarlane G T
机构信息
School of Applied Sciences, South Bank University, London, United Kingdom.
出版信息
Appl Environ Microbiol. 2000 Oct;66(10):4212-21. doi: 10.1128/AEM.66.10.4212-4221.2000.
Resistant starch (RS) enrichments were made using chemostats inoculated with human feces from two individuals at two dilution rates (D = 0.03 h(-1) and D = 0.30 h(-1)) to select for slow- and fast-growing amylolytic communities. The fermentations were studied by analysis of short-chain fatty acids, amylase and alpha-glucosidase activities, and viable counts of the predominant culturable populations and the use of 16S rRNA-targeted oligonucleotide probes. Considerable butyrate was produced at D = 0. 30 h(-1), which corresponded with reduced branched-chain fatty acid formation. At both dilution rates, high levels of extracellular amylase activity were produced, while alpha-glucosidase was predominantly cell associated. Bacteroides and bifidobacteria predominated at the low dilution rate, whereas saccharolytic clostridia became more important at D = 0.30 h(-1). Microscopic examination showed that within 48 h of inoculation, one particular bacterial morphotype predominated in RS enrichments at D = 0.30 h(-1). This organism attached apically to RS granules and formed rosette-like structures which, with glycocalyx formation, agglomerated to form biofilm networks in the planktonic phase. Attempts to isolate this bacterium in pure culture were repeatedly unsuccessful, although a single colony was eventually obtained. On the basis of its 16S rDNA sequence, this RS-degrading, butyrate-producing organism was identified as being a previously unidentified group I Clostridium sp. A 16S rRNA-targeted probe was designed using this sequence and used to assess the abundance of the population in the enrichments. At 240 h, its contributions to total rRNA in the chemostats were 5 and 23% at D = 0.03 and 0.30 h(-1), respectively. This study indicates that bacterial populations with significant metabolic potential can be overlooked using culture-based methodologies. This may provide a paradigm for explaining the discrepancy between the low numbers of butyrate-producing bacteria that are isolated from fecal samples and the actual production of butyrate.
使用恒化器进行抗性淀粉(RS)富集培养,接种来自两个人的人类粪便,设置两种稀释率(D = 0.03 h⁻¹和D = 0.30 h⁻¹),以筛选生长缓慢和快速的淀粉分解菌群。通过分析短链脂肪酸、淀粉酶和α-葡萄糖苷酶活性、主要可培养菌群的活菌计数以及使用靶向16S rRNA的寡核苷酸探针来研究发酵过程。在D = 0.30 h⁻¹时产生了大量丁酸盐,这与支链脂肪酸形成减少相对应。在两种稀释率下,均产生了高水平的细胞外淀粉酶活性,而α-葡萄糖苷酶主要与细胞相关。在低稀释率下,拟杆菌和双歧杆菌占主导地位,而在D = 0.30 h⁻¹时,解糖梭菌变得更为重要。显微镜检查显示,接种后48小时内,在D = 0.30 h⁻¹的RS富集培养物中,一种特定的细菌形态型占主导地位。这种生物体顶端附着在RS颗粒上,形成玫瑰花结样结构,随着糖萼形成,在浮游相中聚集形成生物膜网络。尽管最终获得了一个单菌落,但多次尝试在纯培养中分离这种细菌均未成功。根据其16S rDNA序列,这种降解RS、产生丁酸盐的生物体被鉴定为一种先前未鉴定的I群梭菌属。使用该序列设计了一种靶向16S rRNA的探针,并用于评估富集培养物中该菌群的丰度。在240小时时,在D = 0.03和0.30 h⁻¹时,其对恒化器中总rRNA的贡献分别为5%和23%。这项研究表明,使用基于培养的方法可能会忽略具有显著代谢潜力的细菌群体。这可能为解释从粪便样本中分离出的产生丁酸盐细菌数量较少与实际丁酸盐产量之间的差异提供了一个范例。
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