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Bacteriophage genotyping using BOXA repetitive-PCR

机译:使用Boxa Repetitive-PCR的噬菌体基因分型

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摘要

Repetitive-PCR (rep-PCR) using BOXA1R and BOXA2R as single primers was investigated for its potential to genotype bacteriophage. Previously, this technique has been primarily used for the discrimination of bacterial strains. Reproducible DNA fingerprint patterns for various phage types were generated using either of the two primers. The similarity index of replicates ranged from 89.4–100% for BOXA2R-PCR, and from 90 to 100% for BOXA1R-PCR. The method of DNA isolation (p?=?0.08) and the phage propagation conditions at two different temperatures (p?=?0.527) had no significant influence on generated patterns. Rep-PCR amplification products were generated from different templates including purified phage DNA, phage lysates and phage plaques. The use of this method enabled comparisons of phage genetic profiles to establish their similarity to related or unrelated phages and their bacterial hosts. The findings suggest that repetitive-PCR could be used as a rapid and inexpensive method to preliminary screen phage isolates prior to their selection for more comprehensive studies. The adoption of this rapid, simple and reproducible technique could facilitate preliminary characterisation of a large number of phage isolates and the investigation of genetic relationship between phage genotypes.
机译:研究了使用BoxA1R和BoxA2R作为单引物的重复-PCR(REP-PCR),以潜力对基因型噬菌体。以前,该技术主要用于鉴别细菌菌株。使用两个引物中的任一种产生用于各种噬菌体类型的可再现DNA指纹图案。 Boxa2R-PCR的重复相似度范围为89.4-100%,并且对于BoxA1R-PCR的90至1​​00%。 DNA分离的方法(p?= 0.08)和两个不同温度的噬菌体繁殖条件(p?= 0.527)对产生的模式没有显着影响。 REP-PCR扩增产物由不同模板产生,包括纯化的噬菌体DNA,噬菌体裂解物和噬菌体斑块。使用该方法使得能够比较噬菌体遗传谱来建立与相关或无关噬菌体和细菌宿主的相似性。结果表明,在选择更全面的研究之前,可以将重复-PCR作为初步筛网噬菌体分离物的快速和廉价的方法。采用这种快速,简单可再现的技术可以促进大量噬菌体分离株的初步表征和噬菌体基因型之间遗传关系的调查。

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