首页> 外文OA文献 >Comparison between the Standardized Clinical and Laboratory Standards Institute M38-A2 Method and a 2,3-Bis(2-Methoxy-4-Nitro-5-[(Sulphenylamino)Carbonyl]-2H-Tetrazolium Hydroxide- Based Method for Testing Antifungal Susceptibility of Dermatophytes ▿
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Comparison between the Standardized Clinical and Laboratory Standards Institute M38-A2 Method and a 2,3-Bis(2-Methoxy-4-Nitro-5-[(Sulphenylamino)Carbonyl]-2H-Tetrazolium Hydroxide- Based Method for Testing Antifungal Susceptibility of Dermatophytes ▿

机译:标准化临床和实验室标准协会M38-A2方法与基于2,3-双(2-甲氧基-4-硝基-5-[(Sulphenylamino)Carbonyl] -2H-Tetrazolium Hydroxide的抗真菌药敏性测试方法的比较)皮肤癣菌▿

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摘要

In this study, we determined the utility of a 2,3-bis(2-methoxy-4-nitro-5-[(sulfenylamino)carbonyl]-2H-tetrazolium hydroxide (XTT)-based assay for determining antifungal susceptibilities of dermatophytes to terbinafine, ciclopirox, and voriconazole in comparison to the Clinical and Laboratory Standards Institute (CLSI) M38-A2 method. Forty-eight dermatophyte isolates, including Trichophyton rubrum (n = 15), Trichophyton mentagrophytes (n = 7), Trichophyton tonsurans (n = 11), and Epidermophyton floccosum (n = 13), and two quality control strains, were tested. In the XTT-based method, MICs were determined spectrophotometrically at 490 nm after addition of XTT and menadione. For the CLSI method, the MICs were determined visually. With T. rubrum, the XTT assay revealed MIC ranges of 0.004 to >64 μg/ml, 0.125 to 0.25 μg/ml, and 0.008 to 0.025 μg/ml for terbinafine, ciclopirox, and voriconazole, respectively. Similar MIC ranges were obtained against T. rubrum by using the CLSI method. Additionally, when tested with T. mentagrophytes, T. tonsurans, and E. floccosum isolates, the XTT and CLSI methods resulted in comparable MIC ranges. Both methods revealed similar lowest drug concentrations that inhibited 90% of the isolates for the majority of tested drug-dermatophyte combinations. The levels of agreement within 1 dilution between both methods were as follows: 100% with terbinafine, 97.8% with ciclopirox, and 89.1% with voriconazole. However, the agreement within 2 dilutions between these two methods was 100% for all tested drugs. Our results revealed that the XTT assay can be a useful tool for antifungal susceptibility testing of dermatophytes.
机译:在这项研究中,我们确定了一种基于2,3-双(2-甲氧基-4-硝基-5-[(亚磺酰基氨基)羰基] -2H-氢氧化四唑(XTT)的测定方法,用于测定皮肤癣菌对真菌的抗药性特比萘芬,环吡酮和伏立康唑与临床和实验室标准协会(CLSI)M38-A2方法的比较。48种皮肤真菌分离物,包括红毛癣菌(n = 15),毛癣菌毛癣菌(n = 7),扁桃体毛癣菌(n = 11),表皮藻(n = 13)和两个质量控制菌株进行了测试。在基于XTT的方法中,加入XTT和甲萘醌后在490 nm处以分光光度法测定了MIC。对于CLSI方法,则为MIC用T. rubrum进行XTT检测,发现特比萘芬,环吡酮和伏立康唑的MIC范围分别为0.004至> 64μg/ ml,0.125至0.25μg/ ml和0.008至0.025μg/ ml。通过使用CLSI方法获得了针对红毛锥菌的范围。从离子上讲,当用薄荷茶,扁桃体和絮状大肠杆菌分离物进行测试时,XTT和CLSI方法得出的MIC范围相当。两种方法均显示出相似的最低药物浓度,对于大多数测试的药物-皮肤真菌组合,其抑制了90%的分离物。两种方法在1种稀释度内的一致水平如下:特比萘芬100%,环吡酮97.8%,伏立康唑89.1%。但是,对于所有测试药物,这两种方法在2种稀释度之内的一致性为100%。我们的结果表明,XTT分析可作为皮肤真菌抗真菌药敏试验的有用工具。

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