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16S Ribosomal DNA-Based Analysis of Bacterial Diversity in Purified Water Used in Pharmaceutical Manufacturing Processes by PCR and Denaturing Gradient Gel Electrophoresis

机译:基于16S核糖体DNA的PCR和变性梯度凝胶电泳分析制药生产过程中使用的纯净水中细菌的多样性

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摘要

The bacterial community in partially purified water, which is prepared by ion exchange from tap water and is used in pharmaceutical manufacturing processes, was analyzed by denaturing gradient gel electrophoresis (DGGE). 16S ribosomal DNA fragments, including V6, -7, and -8 regions, were amplified with universal primers and analyzed by DGGE. The bacterial diversity in purified water determined by PCR-DGGE banding patterns was significantly lower than that of other aquatic environments. The bacterial populations with esterase activity sorted by flow cytometry and isolated on soybean casein digest (SCD) and R2A media were also analyzed by DGGE. The dominant bacterium in purified water possessed esterase activity but could not be detected on SCD or R2A media. DNA sequence analysis of the main bands on the DGGE gel revealed that culturable bacteria on these media were Bradyrhizobium sp., Xanthomonas sp., and Stenotrophomonas sp., while the dominant bacterium was not closely related to previously characterized bacteria. These data suggest the importance of culture-independent methods of quality control for pharmaceutical water.
机译:通过变性梯度凝胶电泳(DGGE)分析了部分纯净水中的细菌群落,该细菌是通过自来水的离子交换制备的,并用于制药生产过程。用通用引物扩增包括V6,-7和-8区在内的16S核糖体DNA片段,并通过DGGE分析。通过PCR-DGGE谱带模式确定的纯净水中的细菌多样性显着低于其他水生环境。通过流式细胞术对具有酯酶活性的细菌群体进行分类,并在大豆酪蛋白消化液(SCD)和R2A培养基上进行分离,并通过DGGE分析。纯净水中的优势细菌具有酯酶活性,但无法在SCD或R2A培养基上检测到。对DGGE凝胶上主要条带的DNA序列分析显示,这些培养基上的可培养细菌为缓生根瘤菌,Xanthomonas sp。和Stenotrophomonas sp。,而优势细菌与先前鉴定的细菌没有密切关系。这些数据表明对于制药用水而言,不依赖培养物的质量控制方法的重要性。

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