首页> 外文OA文献 >Echinocandin Susceptibility Testing of Candida spp. Using EUCAST EDef 7.1 and CLSI M27-A3 Standard Procedures: Analysis of the Influence of Bovine Serum Albumin Supplementation, Storage Time, and Drug Lots▿
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Echinocandin Susceptibility Testing of Candida spp. Using EUCAST EDef 7.1 and CLSI M27-A3 Standard Procedures: Analysis of the Influence of Bovine Serum Albumin Supplementation, Storage Time, and Drug Lots▿

机译:念珠菌的Echinocandin药敏试验。使用EUCAST EDef 7.1和CLSI M27-A3标准程序:分析牛血清白蛋白补充,保存时间和药品批次的影响▿

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摘要

The MICs of echinocandins against Candida isolates with fks mutations are higher than those for wild-type (WT) isolates. However, the MIC ranges for susceptible and mutant populations overlap or are poorly separated. It was recently reported that a greater separation could be achieved in the presence of serum. To more fully explore this possibility, we compared the performances of the reference microdilution methods by using standard and bovine serum albumin (BSA)-supplemented growth medium. Anidulafungin, caspofungin, and micafungin MICs were determined according to EUCAST and CLSI methods and with 50% BSA in the medium for 93 clinical isolates, including Candida albicans (20/10 [number of isolates/number of mutants]), C. glabrata (19/10), C. dubliniensis (2/1), C. krusei (16/3), C. parapsilosis (19), and C. tropicalis (19/4) isolates. Stability of the plates was tested after storage at −80°C for 2 and 6 months, and the performance of two different lots of caspofungin was investigated. The addition of BSA to the medium resulted in higher MICs (1 to 9 2-fold dilution steps) for all isolates and compounds. The increases were greatest for anidulafungin and micafungin and, among WT isolates, for C. parapsilosis. The number of very major errors (VMEs) was reduced (24% [20/84 isolates] versus ≤7% [6/84 isolates]) using BSA-supplemented EUCAST medium but not using BSA-supplemented CLSI medium (6% versus 9%). MIC results were unchanged after 6 months of storage of test plates. The two lots of caspofungin yielded identical results. Addition of BSA to the EUCAST medium increases the ability to differentiate between WT isolates and isolates harboring resistance mutations.
机译:棘球and素对带有fks突变的念珠菌分离株的MIC高于野生型(WT)分离株的MIC。但是,易感人群和突变人群的MIC范围重叠或分离差。最近报道,在血清存在下可以实现更大的分离。为了更充分地探索这种可能性,我们通过使用标准和牛血清白蛋白(BSA)补充的生长培养基比较了参考微量稀释方法的性能。根据EUCAST和CLSI方法测定了Anidulafungin,caspofungin和micafungin MIC,并在培养基中对93种临床分离株(包括白色念珠菌(20/10 [分离株的数量/突变体数量]),光滑念珠菌(C. glabrata)(50%BSA)进行了测定。 19/10),杜比尼梭菌(2/1),克鲁斯梭菌(16/3),副梭菌(19)和热带梭菌(19/4)分离株。在-80°C下保存2个月和6个月后,测试板的稳定性,并研究了两种不同批次的卡泊芬净的性能。向所有分离物和化合物的培养基中添加BSA会导致更高的MIC(1至9倍2倍稀释步骤)。对于阿尼芬净和米卡芬净,以及在野生型分离株中,对于副枝梭菌的增加最大。使用补充了BSA的EUCAST培养基,但不使用补充了BSA的CLSI培养基,减少了非常重大错误(VME)的数量(24%[20/84分离株]比≤7%[6/84分离株])(6%对9) %)。储存测试板6个月后,MIC结果没有变化。两组卡泊芬净产生的结果相同。在EUCAST培养基中添加BSA可提高区分WT分离株和具有耐药性突变的分离株的能力。

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