首页> 外文期刊>Veterinary Microbiology >Improvement and validation of RAPD in combination with PFGE analysis of Salmonella enterica ssp. enterica serovar Senftenberg strains isolated from feed mills.
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Improvement and validation of RAPD in combination with PFGE analysis of Salmonella enterica ssp. enterica serovar Senftenberg strains isolated from feed mills.

机译:RAPD的改进和验证结合沙门氏菌ssp的PFGE分析。从饲料厂分离出的肠型血清型Senftenberg菌株。

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In 1995 and 1996 a Swedish feed mill had problems due to a persistent contamination of Salmonella enterica spp. enterica serovar Senftenberg that was difficult to eliminate. Forty-eight strains isolated from the feed mill, together with unrelated strains included to evaluate the discriminatory power and reproducibility, were analysed by pulsed-field gel electrophoresis (PFGE). The source of contamination in the feed mill was identified and preventative measures were taken, that led to a resolution of the problem. A previously developed randomly amplified polymorphic DNA (RAPD) protocol was used, to evaluate a rapid and low-cost alternative to PFGE typing. The use of the alternative thermostable DNA polymerase Tth was shown to increase the reproducibility of the RAPD analysis. The reproducibility, in terms of Pearson's and Dice's similarity coefficients for duplicate runs, increased from 72.0+or-16.9% and 72.3+or-12.9% for Taq to 91.6+or-7.5% and 90.9+or-5.3% for the fingerprints obtained for the RAPD method employing Tth DNA polymerase. Simpson's index of diversity was calculated and found to be 0.580 for RAPD and 0.896 for PFGE. All of the seven RAPD types could be subdivided into one or more PFGE types, whereas none of the 22 PFGE types was divided into more than one RAPD type. RAPD provides a simple, rapid and powerful screening method that can be used to initially select isolates for further analysis by PFGE..
机译:在1995年和1996年,瑞典的一家饲料厂由于肠杆菌沙门氏菌的持续污染而出现问题。很难消除的肠型血清型Senftenberg。通过脉冲场凝胶电泳(PFGE)分析了从饲料厂分离出的48株菌株,以及用于评估判别力和重现性的无关菌株。确定了饲料厂中的污染源并采取了预防措施,从而解决了该问题。使用先前开发的随机扩增多态性DNA(RAPD)方案,以评估PFGE分型的快速且低成本的替代方法。显示使用替代的热稳定DNA聚合酶Tth可提高RAPD分析的可重复性。就重复运行而言,就皮尔逊氏和骰子的相似性系数而言,重现性从Taq的72.0+或-16.9%和72.3+或-12.9%增加到获得的指纹的91.6+或-7.5%和90.9+或-5.3% Tth DNA聚合酶用于RAPD方法。计算得出辛普森多样性指数,对于RAPD为0.580,对于PFGE为0.896。七个RAPD类型中的所有类型都可以细分为一种或多种PFGE类型,而22种PFGE类型中没有一个被划分为不止一种RAPD类型。 RAPD提供了一种简单,快速且功能强大的筛选方法,可用于最初选择分离株进行PFGE进一步分析。

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