Robbins Steven, Jacob Jisha, Lu Xinxin, Moran Mary Ann, Mou Xiaozhen
Biological Sciences, Kent State University, USA.
J Vis Exp. 2011 Sep 10(55):2855. doi: 10.3791/2855.
Microbes are major agents mediating the degradation of numerous dissolved organic carbon (DOC) substrates in aquatic environments. However, identification of bacterial taxa that transform specific pools of DOC in nature poses a technical challenge. Here we describe an approach that couples bromodeoxyuridine (BrdU) incorporation, fluorescence activated cell sorting (FACS), and 16S rRNA gene-based molecular analysis that allows culture-independent identification of bacterioplankton capable of degrading a specific DOC compound in aquatic environments. Triplicate bacterioplankton microcosms are set up to receive both BrdU and a model DOC compound (DOC amendments), or only BrdU (no-addition control). BrdU substitutes the positions of thymidine in newly synthesized bacterial DNA and BrdU-labeled DNA can be readily immunodetected. Through a 24-hr incubation, bacterioplankton that are able to use the added DOC compound are expected to be selectively activated, and therefore have higher levels of BrdU incorporation (HI cells) than non-responsive cells in the DOC amendments and cells in no-addition controls (low BrdU incorporation cells, LI cells). After fluorescence immunodetection, HI cells are distinguished and physically separated from the LI cells by fluorescence activated cell sorting (FACS). Sorted DOC-responsive cells (HI cells) are extracted for DNA and taxonomically identified through subsequent 16S rRNA gene-based analyses including PCR, clone library construction and sequencing.
微生物是介导水生环境中多种溶解有机碳(DOC)底物降解的主要媒介。然而,鉴定自然界中转化特定DOC库的细菌类群面临技术挑战。在此,我们描述了一种结合溴脱氧尿苷(BrdU)掺入、荧光激活细胞分选(FACS)和基于16S rRNA基因的分子分析方法,该方法能够在不依赖培养的情况下鉴定水生环境中能够降解特定DOC化合物的浮游细菌。设置一式三份的浮游细菌微观世界,分别加入BrdU和一种模型DOC化合物(DOC添加物),或仅加入BrdU(无添加对照)。BrdU替代新合成细菌DNA中胸腺嘧啶的位置,并且BrdU标记的DNA能够很容易地通过免疫检测到。经过24小时的培养,预期能够利用添加的DOC化合物的浮游细菌会被选择性激活,因此与DOC添加物中的无反应细胞以及无添加对照中的细胞(低BrdU掺入细胞,LI细胞)相比,具有更高水平的BrdU掺入(HI细胞)。经过荧光免疫检测后,通过荧光激活细胞分选(FACS)将HI细胞与LI细胞区分并物理分离。对分选得到的对DOC有反应的细胞(HI细胞)提取DNA,并通过后续基于16S rRNA基因的分析(包括PCR、克隆文库构建和测序)进行分类鉴定。