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首页> 外文期刊>International Journal of Food Microbiology >The international standard ISO/TS 21872-1 to study the occurence of total and pathogenic Vibrio parahaemolyticus and Vibrio cholerae in seafood: ITS improvement by use of a chromogenic medium and PCR.
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The international standard ISO/TS 21872-1 to study the occurence of total and pathogenic Vibrio parahaemolyticus and Vibrio cholerae in seafood: ITS improvement by use of a chromogenic medium and PCR.

机译:研究海鲜中总和致病性副溶血弧菌和霍乱弧菌的发生的国际标准ISO / TS 21872-1:使用生色培养基和PCR改进ITS。

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During two surveys conducted in 2008 and 2009, the culture method described in the international standard ISO/TS 21872-1 was applied to the detection of Vibrio parahaemolyticus and Vibrio cholerae in 112 living bivalve mollusc samples, with a chromogenic medium used in addition to the TCBS agar, as second selective isolation medium and for enumeration of V. parahaemolyticus and V. cholerae by surface inoculation. A PCR method for detection of these 2 Vibrio species and the hemolysin genes tdh and trh, was applied in parallel. In 2009, the survey was extended to finfish fillets and crustaceans. PCR was also used for species confirmation of characteristic colonies. The identity of the PCR products, specifically targeting V. parahaemolyticus, was checked by sequencing. Occurrence of V. parahaemolyticus and V. cholerae isolates in living bivalve molluscs ranged from 30.4% to 32.6% and from 1.4% to 4.7% respectively. In frozen crustaceans (2009 survey) V. parahaemolyticus and V. cholerae isolates were respectively found in 45% and 10% of the samples. No V. parahaemolyticus or V. cholerae was detected in frozen fish fillets, neither by the ISO method nor by PCR. In 2009, enteropathogenic V. parahaemolyticus (trh+) was isolated from 4 out of 43 oyster samples while the trh gene was present in V. alginolyticus strains and in samples where V. parahaemolyticus was not detected (9 over 112 samples). The ISO method failed to isolate V. parahaemolyticus in 44% to 53% of the living bivalve molluscs where PCR detected the toxR gene specific of V. parahaemolyticus (Vp-toxR). Our results highlighted the need for a revision of the ISO/TS 21872-1 standard, at least, for analysis of living bivalve molluscs, and confirmed the increasing concern of enteropathogenic V. parahaemolyticus in French bivalve molluscs. Enrichment at 41.5 degrees C was questioned and some reliable solutions for the improvement of the ISO/TS 21872-1 method, such as the PCR method for screening of positive samples and confirmation of colonies, were pointed out
机译:在2008年和2009年进行的两次调查中,将国际标准ISO / TS 21872-1中所述的培养方法用于112种副溶血性弧菌和霍乱弧菌的检测。活的双壳贝类软体动物样品,除TCBS琼脂外,还使用了生色培养基作为第二种选择性分离培养基,用于V的计数。副溶血和 V。接种霍乱。并行应用了PCR方法检测这两个弧菌和溶血素基因 tdh 和 trh 。 2009年,调查范围扩大到有鳍鱼片和甲壳类动物。 PCR还用于特征性菌落的物种确认。 PCR产物的身份,特别针对V。副溶血性,通过测序检查。 V 的出现。 parahaemolyticus 和 V。活的双壳类软体动物中的霍乱分离株分别为30.4%至32.6%和1.4%至4.7%。在冷冻甲壳动物中(2009年调查) V 。 parahaemolyticus 和 V。分别在45%和10%的样本中发现了霍乱分离株。没有 V。副溶血或 V。既未通过ISO方法也未通过PCR在冷冻鱼片中检测到霍乱弧菌。在2009年,肠致病性V。从43个牡蛎样本中的4个中分离出parahaemolyticus ( trh + ),而 trh 基因存在于 V中。 alginolyticus 菌株和 V样品中。未检测到副溶血性(112个样本中有9个)。 ISO方法无法隔离 V。 PCR检测到 V特异的 toxR 基因的活双壳贝类软体动物中的副溶血性。副溶血性(Vp-toxR)。我们的结果强调,至少对于活双壳类软体动物的分析,有必要修订ISO / TS 21872-1标准,并证实对肠致病性 V 的关注日益增加。 parahaemolyticus 在法国双壳软体动物中。质疑在41.5摄氏度下的浓缩,并提出了一些改进ISO / TS 21872-1方法的可靠解决方案,例如用于筛选阳性样品的PCR方法和确认菌落的方法

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