非白色念珠菌临床分离株的分子鉴定及抗真菌敏感性分析

K. Diba, K. Makhdoomi, Shima Aboutalebian
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摘要

背景:危及生命的全身性真菌病的发病率正在增加,特别是住院患者和免疫功能低下患者中念珠菌物种的暴发性感染。管理目前可用的有限数量的抗真菌药物需要识别含有耐药分离株的感染。目的:本研究的目的是鉴定从住院病例的痰液和支气管肺泡灌洗液标本中分离出的非白色念珠菌属抗唑真菌。方法:研究对象包括医院获得性感染(HAI)病例,通过直接显微镜检查进行初步诊断,以检测可能的真菌。采用PCR-限制性片段长度多态性(RFLP)和实时荧光定量PCR对分离的念珠菌进行鉴定和分子分型。采用临床与实验室标准协会(CLSI)肉汤微量稀释(BMD)最低抑菌浓度(MIC) (M27-A2)法对医院分离的念珠菌进行抗真菌药敏试验(AFST)。结果:2014年8月至2016年9月24个月内,共采集确诊HAI病例198份样本。标本实验研究结果显示,真菌或细菌感染阳性93例(47%),其中真菌感染54例(58%)。假设所有分离的生物都是HAI的病原体。结论:培养基CHROMagar™念珠菌是一种易于使用的感染鉴定方法,但不如PCR- rflp和real-time PCR方法准确可靠。结果还显示念珠菌对唑类药物(本研究为伊曲康唑)的敏感性降低。
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Molecular Identification and Antifungal Susceptibility Profiles of Non-albicans Candida Species Clinical Isolates
Background: There is an increasing incidence of life-threatening systemic mycoses, specifically fulminant infections by the Candida species in hospitalised patients and in those who are immunocompromised. Management of the limited number of antifungal drugs currently available requires the identification of infections containing drug-resistant isolates. Objectives: The aim of this study was to identify the non-albicans Candida species as azole-resistant fungi, isolated from sputum and bronchoalveolar lavage specimens of hospitalised cases. Methods: The subjects included hospital-acquired infection (HAI) cases, with a primary diagnosis using a direct microscopic examination, performed for the detection of probable fungi. The molecular tests of PCR-restriction fragment length polymorphism (RFLP) and real-time PCR were performed to confirm the identity and molecular typing of the Candida isolates. Antifungal susceptibility testing (AFST), by the Clinical and Laboratory Standards Institute (CLSI) broth microdilution (BMD) minimum inhibitory concentration (MIC) (M27-A2) method, was performed on the hospital-isolated Candida species. Results: During 24 months, from August 2014 to September 2016, a total of 198 samples were obtained from cases with proven HAI. The results of experimental studies on the specimens showed 93 (47%) positive cases for a fungal or bacterial infection, of which 54 (58%) had a fungal infection. It was hypothesised that all of the isolated organisms were causative agents of the HAI. Conclusions: The results showed that the medium CHROMagar™ Candida is an accessible and easy-to-use method for the identification of infection, but not as accurate and reliable as PCR-RFLP and real-time PCR methods. Results also showed decreasing susceptibility to azoles (itraconazole in this study) of the Candida species.
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