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首页> 外文期刊>Journal of Clinical Microbiology >Occurrence of Extended-Spectrum and AmpC Beta-Lactamases in Bloodstream Isolates of Klebsiella pneumoniae: Isolates Harbor Plasmid-Mediated FOX-5 and ACT-1 AmpC Beta-Lactamases
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Occurrence of Extended-Spectrum and AmpC Beta-Lactamases in Bloodstream Isolates of Klebsiella pneumoniae: Isolates Harbor Plasmid-Mediated FOX-5 and ACT-1 AmpC Beta-Lactamases

机译:肺炎克雷伯菌的血流分离物中出现广谱和AmpCβ-内酰胺酶:分离港口质粒介导的FOX-5和ACT-1 AmpCβ-内酰胺酶

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We tested 190 Klebsiella pneumoniae bloodstream isolates recovered from 189 patients in 30 U.S. hospitals in 23 states to determine the occurrence of extended-spectrum β-lactamase (ESBL) and AmpC β-lactamase producers. Based on growth inhibition by clavulanic acid by disk and MIC test methods, 18 (9.5%) of the isolates produced ESBLs. Although the disk diffusion method with standard breakpoints identified 28 cefoxitin-nonsusceptible isolates, only 5 (18%) of these were confirmed as AmpC producers. Of two AmpC confirmatory tests, the three-dimensional extract test was easier to perform than was the double-disk approximation test using a novel inhibitor, Syn2190. Three of the five AmpC producers carried the blaFOX-5 gene, while the other two isolates harbored the blaACT-1 gene. All AmpC genes were transferable. In vitro susceptibility testing with standard inocula showed that all five AmpC-producing strains were susceptible to cefepime, imipenem, and ertapenem but that with a high inoculum, more of these strains were susceptible to the carbapenems than to cefepime. All but 1 of 14 screen-positive AmpC nonproducers (and ESBL nonproducers) were susceptible to ceftriaxone and cefepime at the standard inoculum as were 6 of 6 isolates that were randomly selected and tested with a high inoculum. These results indicate that (i) a significant number of K. pneumoniae bloodstream isolates harbor ESBL or AmpC β-lactamases, (ii) confirmatory tests are necessary to identify true AmpC producers, and (iii) in vitro, carbapenems are active against AmpC-producing strains of K. pneumoniae.
机译:我们在23个州的30家美国医院中对189例肺炎克雷伯菌的血液分离株进行了测试,以确定是否存在超广谱β-内酰胺酶(ESBL)和AmpCβ-内酰胺酶生产者。基于磁盘和MIC测试方法对克拉维酸的生长抑制作用,有18(9.5%)的分离物产生了ESBLs。尽管采用标准断点的圆盘扩散方法鉴定出28种头孢西丁不敏感菌株,但只有5种(18%)被确认为AmpC生产者。在两个AmpC确认测试中,三维提取测试比使用新型抑制剂Syn2190的双盘近似测试更容易执行。五个AmpC生产者中的三个携带 bla FOX-5 基因,而其他两个分离株则携带 bla ACT-1 < / sub>基因。所有的AmpC基因都是可转移的。用标准接种物进行的体外药敏试验表明,所有五种产生AmpC的菌株均对头孢吡肟,亚胺培南和厄他培南敏感,但接种量高时,这些菌株对碳青霉烯的敏感性高于对头孢吡肟的敏感性。 14个筛查呈阳性的AmpC非生产者(和ESBL非生产者)中的除1个外,在标准接种物中均对头孢曲松和头孢吡肟易感,随机选择并用高接种量测试的6个分离株中有6个对此敏感。这些结果表明(i)大量的 K。肺炎分离株带有ESBL或AmpCβ-内酰胺酶,(ii)鉴定试验对于鉴定真正的AmpC产生者是必要的,并且(iii)碳青霉烯类对产生AmpC的 K菌株具有活性。肺炎

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