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首页> 外文期刊>Journal of Clinical Microbiology >Use of Fluorescent Probes To Determine MICs of Amphotericin B and Caspofungin against Candida spp. and Aspergillus spp.
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Use of Fluorescent Probes To Determine MICs of Amphotericin B and Caspofungin against Candida spp. and Aspergillus spp.

机译:使用荧光探针测定两性霉素B和卡泊芬净对念珠菌的MIC。和曲霉属。

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We investigated the utility of mechanism-based fluorescent probes for determination of MICs (FMICs) of amphotericin B and caspofungin against Candida spp. and Aspergillus spp. Amphotericin B was selected as a membrane-active antifungal agent, and caspofungin was selected as a cell wall-active agent. FMICs were also compared to the MIC determined by CLSI (formerly NCCLS) methods. Five isolates per species of Candida albicans, Candida glabrata, Candida parapsilosis, Aspergillus fumigatus, and Aspergillus terreus were studied with either amphotericin B or caspofungin. The fluorescent probes, carboxyfluorescein diacetate (CFDA) for cytoplasmic esterase activity and dihexyloxacarbocyanine iodide (DiOC6) for cell membrane potential, were each added to their respective plates. MICs and FMICs were determined in at least three separate experiments (in duplicate). Fluorescence was measured using a 96-well plate fluorometer. For amphotericin B and caspofungin, the FMIC end point was the lowest concentration of drug at which the percent growth inhibition from treated organisms versus control organisms displayed 80% inhibition for amphotericin B and 50% inhibition for caspofungin as measured by a fluorescent signal. The MIC for amphotericin B was defined as the lowest concentration of antifungal displaying no visible growth for both Aspergillus and Candida spp. The MIC for caspofungin was the lowest concentration of drug that displayed a minimum effective concentration for Aspergillus spp. For Candida spp., the MIC for caspofungin was defined as the concentration at which the antifungal agent significantly inhibits the organism. The FMICs of both antifungals, as measured by the DiOC6 membrane probe, showed good agreement (83% to 100%), within one well dilution, with the MICs against amphotericin B and caspofungin for all species. Also, the FMICs measured by the CFDA cytoplasmic esterase probe reflecting damage due to cell wall or cell membrane showed strong agreement (79 to 100%) with the MICs of both amphotericin B and caspofungin for all species. There was no significant difference in comparisons of MIC and FMIC values (P ≥ 0.05). The use of fluorescent probes provides a mechanism-based method of determination of MICs of amphotericin B and caspofungin against Candida spp. and Aspergillus spp. that correlates well with standard methods.
机译:我们调查了基于机理的荧光探针在确定两性霉素B和卡泊芬净对 Candida spp的MIC(FMIC)方面的实用性。和曲霉菌 spp。选择两性霉素B作为膜活性抗真菌剂,选择卡泊芬净作为细胞壁活性剂。 FMIC也与CLSI(以前称为NCCLS)方法确定的MIC进行了比较。每个白色念珠菌 glabrata Candida parapsilosis 烟曲霉和曲霉五个菌种用两性霉素B或卡泊芬净进行了研究。将分别用于细胞质酯酶活性的荧光探针,羧基乙酸荧光素二乙酸酯(CFDA)和用于细胞膜电位的二己基氧杂羰基花菁碘化物(DiOC 6 )分别添加到各自的平板中。 MIC和FMIC在至少三个独立的实验中确定(一式两份)。使用96孔板荧光计测量荧光。对于两性霉素B和卡泊芬净,FMIC终点是药物的最低浓度,在该浓度下,通过荧光信号测得,处理过的生物体相对于对照生物体的生长抑制百分数显示出对两性霉素B的抑制率为80%,对卡泊芬净的抑制率为50%。两性霉素B的MIC被定义为曲霉 Candida spp的最低抗真菌浓度,且无可见生长。卡泊芬净的MIC是最低浓度的药物,显示曲霉 spp的最小有效浓度。对于 Candida 菌种,卡泊芬净的MIC定义为抗真菌剂显着抑制生物体的浓度。用DiOC 6 膜探针测量的两种抗真菌剂的FMIC在所有孔中均与两性霉素B和卡泊芬净的MIC吻合良好(83%至100%)。而且,通过CFDA胞质酯酶探针测得的FMIC与所有物种的两性霉素B和卡泊芬净的MIC均显示出很强的一致性(79%至100%),反映了由于细胞壁或细胞膜造成的损害。 MIC和FMIC值的比较没有显着差异( P ≥0.05)。荧光探针的使用提供了一种基于机制的方法来确定两性霉素B和卡泊芬净对 Candida spp的MIC。和曲霉菌 spp。与标准方法紧密相关

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