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Macrolide Resistance in Campylobacter jejuni and Campylobacter coli: Molecular Mechanism and Stability of the Resistance Phenotype

机译:空肠弯曲菌和大肠弯曲菌中的大环内酯类耐药性:耐药表型的分子机理和稳定性

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摘要

A collection of 23 macrolide-resistant Campylobacter isolates from different geographic areas was investigated to determine the mechanism and stability of macrolide resistance. The isolates were identified as Campylobacter jejuni or Campylobacter coli based on the results of the hippurate biochemical test in addition to five PCR-based genotypic methods. Three point mutations at two positions within the peptidyl transferase region in domain V of the 23S rRNA gene were identified. About 78% of the resistant isolates exhibited an A→G transition at Escherichia coli equivalent base 2059 of the 23S rRNA gene. The isolates possessing this mutation showed a wide range of erythromycin and clarithromycin MICs. Thus, this mutation may incur a greater probability of treatment failure in populations infected by resistant Campylobacter isolates. Another macrolide-associated mutation (A→C transversion), at E. coli equivalent base 2058, was detected in about 13% of the isolates. An A→G transition at a position cognate with E. coli 23S rRNA base 2058, which is homologous to the A2142G mutation commonly described in Helicobacter pylori, was also identified in one of the C. jejuni isolates examined. In the majority of C. jejuni isolates, the mutations in the 23S rRNA gene were homozygous except in two cases where the mutation was found in two of the three copies of the target gene. Natural transformation demonstrated the transfer of the macrolide resistance phenotype from a resistant Campylobacter isolate to a susceptible Campylobacter isolate. Growth rates of the resulting transformants containing A-2058→C or A-2059→G mutations were similar to that of the parental isolate. The erythromycin resistance of six of seven representative isolates was found to be stable after successive subculturing in the absence of erythromycin selection pressure regardless of the resistance level, the position of the mutation, or the number of the mutated copies of the target gene. One C. jejuni isolate showing an A-2058→G mutation, however, reverted to erythromycin and clarithromycin susceptibility after 55 subcultures on erythromycin-free medium. Investigation of ribosomal proteins L4 and L22 by sequence analysis in five representative isolates of C. jejuni and C. coli demonstrated no significant macrolide resistance-associated alterations in either the L4 or the L22 protein that might explain either macrolide resistance or enhancement of the resistance level.
机译:调查了来自不同地理区域的23种对大环内酯类耐药的弯曲杆菌菌株的分离物,以确定大环内酯类耐药的机理和稳定性。除5种基于PCR的基因型方法外,还根据马尿酸盐生化测试的结果将分离物鉴定为空肠弯曲菌或大肠弯曲菌。在23S rRNA基因的结构域V的肽基转移酶区域内两个位置的三个点突变被确定。约78%的抗性分离株在23S rRNA基因的大肠杆菌等效碱基2059处显示了A→G过渡。具有此突变的分离株显示出广泛的红霉素和克拉霉素MIC。因此,这种突变可能在耐药的弯曲杆菌分离株感染的人群中引起更大的治疗失败可能性。在大约13%的分离物中检测到了另一种与大环内酯类相关的突变(A→C转化),在大肠杆菌当量碱基2058处。在所研究的空肠弯曲杆菌分离株之一中,也鉴定出与大肠杆菌23S rRNA碱基2058同源的位置的A→G过渡,其与幽门螺杆菌中通常描述的A2142G突变同源。在大多数空肠弯曲菌分离株中,23S rRNA基因中的突变是纯合的,除了在两种情况下,在目标基因的三个拷贝中的两个拷贝中发现了突变。自然转化表明大环内酯类耐药表型从耐药弯曲杆菌分离株转移到易感弯曲杆菌分离株。得到的含有A-2058→C或A-2059→G突变的转化体的生长速率与亲本分离株的生长速率相似。发现在没有红霉素选择压力的情况下连续传代培养后,七个代表性分离物中的六个对红霉素的抵抗是稳定的,而与靶基因的抗性水平,突变位置或突变拷贝数无关。在无红霉素培养基上进行55次传代培养后,显示A-2058→G突变的一种空肠弯曲杆菌分离株恢复为对红霉素和克拉霉素的敏感性。通过对空肠弯曲杆菌和大肠杆菌的五个代表性分离株进行序列分析对核糖体蛋白L4和L22进行的研究表明,L4或L22蛋白中没有与大环内酯类药物相关的显着耐药性变化,这可能解释了大环内酯类药物的耐药性或耐药水平的提高。

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