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Transfer of Plasmid DNA to Clinical Coagulase-Negative Staphylococcal Pathogens by Using a Unique Bacteriophage

机译:通过使用独特的噬菌体将质粒DNA转移至临床凝血酶阴性葡萄球菌病原体

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Genetic manipulation of emerging bacterial pathogens, such as coagulase-negative staphylococci (CoNS), is a major hurdle in clinical and basic microbiological research. Strong genetic barriers, such as restriction modification systems or clustered regularly interspaced short palindromic repeats (CRISPR), usually interfere with available techniques for DNA transformation and therefore complicate manipulation of CoNS or render it impossible. Thus, current knowledge of pathogenicity and virulence determinants of CoNS is very limited. Here, a rapid, efficient, and highly reliable technique is presented to transfer plasmid DNA essential for genetic engineering to important CoNS pathogens from a unique Staphylococcus aureus strain via a specific S. aureus bacteriophage, Φ187. Even strains refractory to electroporation can be transduced by this technique once donor and recipient strains share similar Φ187 receptor properties. As a proof of principle, this technique was used to delete the alternative transcription factor sigma B (SigB) via allelic replacement in nasal and clinical Staphylococcus epidermidis isolates at high efficiencies. The described approach will allow the genetic manipulation of a wide range of CoNS pathogens and might inspire research activities to manipulate other important pathogens in a similar fashion.
机译:对新兴细菌病原体(例如凝固酶阴性葡萄球菌(CoNS))的遗传操作是临床和基础微生物研究的主要障碍。强大的遗传屏障,例如限制性修饰系统或成簇的规则间隔的短回文重复序列(CRISPR),通常会干扰DNA转化的可用技术,因此使CoNS的操作复杂化或使其变得不可能。因此,目前关于CoNS致病性和毒力决定因素的知识非常有限。在这里,提出了一种快速,有效和高度可靠的技术,通过特定的金黄色葡萄球菌噬菌体Φ187,将基因工程必不可少的质粒DNA转移到独特的金黄色葡萄球菌菌株中的重要CoNS病原体上。一旦供体和受体菌株具有相似的Φ187受体特性,甚至可以通过电穿孔技术转化为难治性菌株。作为原理的证明,该技术被用于通过等位基因置换在鼻和临床表皮葡萄球菌分离物中高效地删除替代转录因子sigma B(SigB)。所描述的方法将允许对多种CoNS病原体进行遗传操作,并可能激发研究活动以类似方式操纵其他重要的病原体。

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