NSF International, 789 Dixboro Road, Ann Arbor, MI 48105, USA.
J Ind Microbiol Biotechnol. 2010 Sep;37(9):909-18. doi: 10.1007/s10295-010-0738-1. Epub 2010 May 22.
Brevundimonas diminuta is a small Gram-negative bacterium used for validation of membranes and filters used in the pharmaceutical and drinking water treatment industries. Current assays are time consuming, nonselective, and may be subject to interference by competing indigenous microorganisms. The focus of this study is to develop rapid and specific enumeration methodologies for B. diminuta. Quantitative real-time polymerase chain reaction (qPCR) and fluorescence in situ hybridization (FISH) assays were developed based on the gyrB (1,166 bp) and rpoD (829 bp) gene sequences of B. diminuta ATCC 19146. Species-specific primers and probes were designed, and a 100-200 bp segment of each gene was targeted in the qPCR studies. For both the qPCR and FISH assays, an internal 25 bp sequence was selected for use as a TaqMan probe (labeled with 6-FAM and a Black Hole Quencher). Probe specificity studies, conducted against Gram-negative and Gram-positive reference strains as well as environmental strains, revealed high specificity of the primer/probe pairs to B. diminuta. Sensitivities of the qPCR reactions using purified genomic DNA from B. diminuta were determined to be 0.89 pg for rpoD and 8.9 pg for gyrB. The feasibility of using whole-cell B. diminuta suspensions directly with the rpoD qPCR protocol was also evaluated. The greatest sensitivity observed for B. diminuta was 1 x 10(3) colony forming units (CFU) per mL when tryptic soy broth was used as the growth medium. When compared with direct microscopic enumeration using a 5' 6-FAM FISH probe, traditional plating methods showed significant underestimation of B. diminuta concentration (P = 0.01) when this organism was cultivated in saline lactose broth. The results of this investigation demonstrate that qPCR and FISH are effective methods for rapid (<4 h) enumeration of B. diminuta and may be viable alternatives to plating when validating drinking water filtration systems.
小食酸菌是一种革兰氏阴性的小细菌,用于验证制药和饮用水处理行业中使用的膜和过滤器。目前的检测方法耗时、非选择性,并且可能受到竞争的土著微生物的干扰。本研究的重点是开发快速和特定的小食酸菌计数方法。基于小食酸菌 ATCC 19146 的 gyrB(1166bp)和 rpoD(829bp)基因序列,开发了定量实时聚合酶链反应(qPCR)和荧光原位杂交(FISH)检测方法。设计了种特异性引物和探针,并在 qPCR 研究中针对每个基因的 100-200bp 片段进行了靶向。对于 qPCR 和 FISH 检测方法,选择内部 25bp 序列作为 TaqMan 探针(用 6-FAM 和黑腔猝灭剂标记)。针对革兰氏阴性和革兰氏阳性参考菌株以及环境菌株进行的探针特异性研究表明,引物/探针对小食酸菌具有高度特异性。使用从小食酸菌中纯化的基因组 DNA 进行 qPCR 反应的灵敏度分别确定为 rpoD 为 0.89pg 和 gyrB 为 8.9pg。还评估了使用 rpoD qPCR 方案直接使用小食酸菌全细胞悬液的可行性。当使用胰蛋白胨大豆肉汤作为生长培养基时,观察到小食酸菌的最大灵敏度为 1 x 10(3)菌落形成单位(CFU)/mL。与使用 5' 6-FAM FISH 探针直接进行显微镜计数相比,当该生物体在盐乳糖肉汤中培养时,传统的平板计数方法对小食酸菌浓度的低估非常明显(P=0.01)。本研究结果表明,qPCR 和 FISH 是快速(<4h)计数小食酸菌的有效方法,在验证饮用水过滤系统时,可能是平板计数的可行替代方法。
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