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首页> 外文期刊>Journal of applied microbiology >Isolation and biochemical characterisation of enterocins produced by enterococci from different sources
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Isolation and biochemical characterisation of enterocins produced by enterococci from different sources

机译:不同来源肠球菌产生的肠球菌的分离和生化特性

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Aims: Comparison of enterocins produced by six Enterococcus faecium strains and one Ent. faecalis strain isolated from different origin with regard to their microbiological and biochemical characteristics in view of their technological potential and practical use. Methods and Results: The seven enterococci were sensitive to the glycopeptide antibiotics vancomycin and teicoplanin and did not show haemolytic activity. The absence of the glycopeptide-resistant genotypes and the genes involved in the production of the lantibiotic cytolysin was confirmed by PCR. The enterocins were active towards Listeria innocua and other lactic acid bacteria. Their temperature stability was dependent on the pH and their activity wsa higher at acidic pH. A bactericidal and bacteriolytic effect was shown. PCR analyses revealed that the gene of enterocin A was present in the genome of Ent. faecium CCM 4231, Ent. faecium 306 I.2.20 and Ent. faecalis Y; both enterocin A and B genes were present in the genome of Ent. faecium LMG 11423~T, Ent. faecium RZS C5 and Ent. faecium RZS C13. Enterocin P was detced in the genome of Ent. faecium RZS C5 and Ent. faecium RZS C13. No signal was found for Ent. faecium SF 68. Enterocins from Ent. faecium RZS C5, Ent. faecium RZS C13 and Ent. faecium SF 68 were pruified to homogeneity. Conclusions: Ent. faecium RZS C5 and Ent. faecium RZS C13 produced an enterocin with a molecular mass of 5460 and 5477 Da, respectively, which was in the range of that of enterocin B. The amino acid sequence analysis of the enterocin from Ent. faecium RZS C13 revealed 24 N-terminal residues, which were identical to those of enterocin B. The enterocin from Ent. faecium SF 68 had a molecular mass of 4488 Da, which did not correspond to any enterocin known so far. Significance and Impact of the Study: The number of characterized enterocins is increasing. As this type of work is tedious and time-consuming, it may be interesting to include PCR as a first step to know if the Enterococcus strain in study produces either a known or a new enterocin. Also, it is important to check the absence of cytolysin and resistance to vancomycin for a further application of the Enterococcus strain in food or health applications.
机译:目的:比较6种粪肠球菌菌株和1种Ent产生的肠毒素。考虑到其技术潜力和实际应用,从不同来源分离的粪便菌株的微生物学和生化特性。方法和结果:7例肠球菌对糖肽抗生素万古霉素和替考拉宁敏感,没有溶血活性。通过PCR证实了不存在糖肽抗性基因型和羊毛硫抗生素细胞溶素的产生所涉及的基因。肠毒素对无毒李斯特菌和其他乳酸菌具有活性。它们的温度稳定性取决于pH,并且在酸性pH下它们的活性更高。显示了杀菌和溶菌作用。 PCR分析表明肠球蛋白A基因存在于Ent的基因组中。粪便CCM 4231,Ent。粪便306 I.2.20和Ent。粪便Y;肠基因A和B基因都存在于Ent的基因组中。粪便LMG 11423〜T,Ent。粪便RZS C5和Ent。粪便RZS C13。在Ent基因组中检测到肠球蛋白P。粪便RZS C5和Ent。粪便RZS C13。找不到Ent的信号。粪便SF 68。粪便RZS C5,Ent。粪便RZS C13和Ent。粪便SF 68被纯化为同质。结论:Ent。粪便RZS C5和Ent。粪肠球菌RZS C13分别产生了分子量为5460和5477 Da的肠球菌素,其分子量在肠球菌素B的范围内。Ent。肠球菌素的氨基酸序列分析。粪大肠菌RZS C13揭示了24个N末端残基,这些残基与肠球菌素B相同。粪便SF 68的分子量为4488 Da,与迄今已知的任何肠球蛋白都不对应。研究的意义和影响:特征性肠毒素的数量正在增加。由于这类工作繁琐且耗时,因此将PCR作为第一步来了解研究中的肠球菌菌株是产生已知肠球菌还是新肠球菌可能是有趣的。同样,对于肠球菌菌株在食品或健康应用中的进一步应用,检查细胞溶素的缺乏和对万古霉素的抗性也很重要。

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