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RNA Colony Blot Hybridization Method for Enumeration of Culturable Vibrio cholerae and Vibrio mimicus Bacteria▿

机译:RNA菌落印迹杂交法计算可培养的霍乱弧菌和模拟弧菌细菌

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摘要

A species-specific RNA colony blot hybridization protocol was developed for enumeration of culturable Vibrio cholerae and Vibrio mimicus bacteria in environmental water samples. Bacterial colonies on selective or nonselective plates were lysed by sodium dodecyl sulfate, and the lysates were immobilized on nylon membranes. A fluorescently labeled oligonucleotide probe targeting a phylogenetic signature sequence of 16S rRNA of V. cholerae and V. mimicus was hybridized to rRNA molecules immobilized on the nylon colony lift blots. The protocol produced strong positive signals for all colonies of the 15 diverse V. cholerae-V. mimicus strains tested, indicating 100% sensitivity of the probe for the targeted species. For visible colonies of 10 nontarget species, the specificity of the probe was calculated to be 90% because of a weak positive signal produced by Grimontia (Vibrio) hollisae, a marine bacterium. When both the sensitivity and specificity of the assay were evaluated using lake water samples amended with a bioluminescent V. cholerae strain, no false-negative or false-positive results were found, indicating 100% sensitivity and specificity for culturable bacterial populations in freshwater samples when G. hollisae was not present. When the protocol was applied to laboratory microcosms containing V. cholerae attached to live copepods, copepods were found to carry approximately 10,000 to 50,000 CFU of V. cholerae per copepod. The protocol was also used to analyze pond water samples collected in an area of cholera endemicity in Bangladesh over a 9-month period. Water samples collected from six ponds demonstrated a peak in abundance of total culturable V. cholerae bacteria 1 to 2 months prior to observed increases in pathogenic V. cholerae and in clinical cases recorded by the area health clinic. The method provides a highly specific and sensitive tool for monitoring the dynamics of V. cholerae in the environment. The RNA blot hybridization protocol can also be applied to detection of other gram-negative bacteria for taxon-specific enumeration.
机译:建立了一种物种特异性的RNA菌落杂交技术,用于枚举环境水样中可培养的霍乱弧菌和拟态弧菌。用十二烷基硫酸钠裂解选择性或非选择性平板上的细菌菌落,并将裂解物固定在尼龙膜上。将靶向霍乱弧菌和拟南芥弧菌的16S rRNA的系统发生特征序列的荧光标记寡核苷酸探针与固定在尼龙菌落提拉印迹上的rRNA分子杂交。该协议为15种不同的霍乱弧菌V的所有菌落产生了强阳性信号。测试了模拟菌株,表明探针对目标物种的100%敏感性。对于10个非目标物种的可见菌落,由于海洋细菌Grimontia(Vibrio)hollisae产生的弱阳性信号,因此探针的特异性计算为90%。当使用经生物发光霍乱弧菌菌株改良的湖水样品评估测定的灵敏度和特异性时,未发现假阴性或假阳性结果,表明当淡水样品中可培养细菌种群的敏感性和特异性为100%时G. hollisae不存在。当该方案应用于包含附着于活co足的霍乱弧菌的实验室缩影时,发现co足每个per足可携带约10,000至50,000 CFU霍乱弧菌。该协议还用于分析在孟加拉国霍乱流行地区9个月内收集的池塘水样。从六个池塘收集的水样表明,在观察到致病性霍乱弧菌增多之前,以及在该地区卫生诊所记录的临床病例中,发现了可培养的霍乱弧菌总数达1-2个月。该方法提供了高度特异性和灵敏的工具,用于监测环境中霍乱弧菌的动态。 RNA印迹杂交方案也可用于检测其他革兰氏阴性细菌以进行分类群特异性计数。

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