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Phosphoethanolamine Modification of Lipid A in Colistin-Resistant Variants of Acinetobacter baumannii Mediated by the pmrAB Two-Component Regulatory System▿

机译:pmrAB两组分调节系统介导的鲍曼不动杆菌抗共Listin变体中脂质A的磷酸乙醇胺修饰▿

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摘要

Colistin resistance is rare in Acinetobacter baumannii, and little is known about its mechanism. We investigated the role of PmrCAB in this trait, using (i) resistant and susceptible clinical strains, (ii) laboratory-selected mutants of the type strain ATCC 19606 and of the clinical isolate ABRIM, and (iii) a susceptible/resistant pair of isogenic clinical isolates, Ab15/133 and Ab15/132, isolated from the same patient. pmrAB sequences in all the colistin-susceptible isolates were identical to reference sequences, whereas resistant clinical isolates harbored one or two amino acid replacements variously located in PmrB. Single substitutions in PmrB were also found in resistant mutants of strains ATCC 19606 and ABRIM and in the resistant clinical isolate Ab15/132. No mutations in PmrA or PmrC were found. Reverse transcriptase (RT)-PCR identified increased expression of pmrA (4- to 13-fold), pmrB (2- to 7-fold), and pmrC (1- to 3-fold) in resistant versus susceptible organisms. Matrix-assisted laser desorption ionization-time of flight (MALDI-TOF) mass spectrometry showed the addition of phosphoethanolamine to the hepta-acylated form of lipid A in the resistant variants and in strain ATCC 19606 grown under low-Mg2+ induction conditions. pmrB gene knockout mutants of the colistin-resistant ATCC 19606 derivative showed >100-fold increased susceptibility to colistin and 5-fold decreased expression of pmrC; they also lacked the addition of phosphoethanolamine to lipid A. We conclude that the development of a moderate level of colistin resistance in A. baumannii requires distinct genetic events, including (i) at least one point mutation in pmrB, (ii) upregulation of pmrAB, and (iii) expression of pmrC, which lead to addition of phosphoethanolamine to lipid A.
机译:鲍氏不动杆菌对共价素的抗性很少见,对其机制了解甚少。我们使用(i)抗药性和易感性临床菌株,(ii)ATCC 19606型菌株和临床分离株ABRIM的实验室选择突变体和(iii)易感/抗性对对研究了PmrCAB在此性状中的作用。从同一患者中分离出的同基因临床分离株Ab15 / 133和Ab15 / 132。所有对大肠杆菌敏感的分离株中的pmrAB序列与参考序列相同,而抗药性临床分离株在PmrB中具有一个或两个氨基酸替换。在菌株ATCC 19606和ABRIM的耐药突变体以及耐药临床分离株Ab15 / 132中也发现了PmrB的单取代。未发现PmrA或PmrC突变。逆转录酶(RT)-PCR鉴定了抗药性与易感生物中pmrA(4至13倍),pmrB(2至7倍)和pmrC(1至3倍)的表达增加。基质辅助激光解吸电离飞行时间(MALDI-TOF)质谱表明,在抗性变异体和在低Mg2 +诱导条件下生长的ATCC 19606菌株中,脂乙醇的七酰化形式添加了磷酸乙醇胺。耐大肠菌素的ATCC 19606衍生物的pmrB基因敲除突变体显示对大肠菌素的敏感性增加了100倍,而pmrC的表达降低了5倍。他们还缺乏在脂质A中添加磷酸乙醇胺的结论。我们得出结论,鲍曼不动杆菌中等水平的大肠菌素抗性的发展需要独特的遗传事件,包括(i)pmrB至少有一个点突变,(ii)pmrAB上调,以及(iii)pmrC的表达,这导致将磷乙醇胺添加到脂质A中。

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