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Comparison of Molecular Microscopic and Culture Methods for Diagnosis of Cutaneous Leishmaniasis

机译:皮肤利什曼病诊断的分子显微镜和培养方法的比较

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摘要

Cutaneous leishmaniasis (CL) is endemic in the northwest of Isfahan province, Iran. Increase in the incidence of the disease in Kashan has made it necessary to find out the best method for diagnosis and molecular characterization of species. In the present study, 130 patients suspected to cutaneous leishmaniosis referred to health care centers of Kashan were examined. Serosity of lesion was collected for smear preparation and cultured in Novy‐Nicolle‐McNeal medium. DNA was extracted from serosity, and species was determined by polymerase chain reaction (PCR) and nested PCR using kinetoplast DNA (kDNA) specific primers. The diagnostic criteria of CL were based on the observation of amastigotes in the smear, promastigotes in culture, presence of expected bands in PCR, or nested PCR. Of 130 specimens, 87 (66.9%), 72 (56.2%), 98 (75.4 %), 96 (73.8%), and 99 (76.2%) were positive for microscopic culture, PCR, nested PCR, and combined PCR and microscopy (proposed method), respectively. Sensitivity, specificity, positive and negative predictive values of PCR were 99%, 100%, 100%, 96.9%, respectively, for microscopy 87.9%, 100%, 100%, 72.1%, for culture 72.7%, 100%, 100%, 53.4 %, and for nested PCR 97%, 100%, 100%, 91.2%, respectively. Based on the results of the study, kDNA‐PCR was the most sensitive method for diagnosis of CL.
机译:皮肤利什曼病(CL)是伊朗伊斯法罕省西北部的地方病。在喀山,该病的发病率不断增加,因此有必要找到诊断和鉴定物种的最佳方法。在本研究中,检查了130名疑似皮肤利什曼病的患者,转诊至喀山卫生保健中心。收集病灶的浆液性,用于涂片准备,并在Novy-Nicolle-McNeal培养基中培养。从浆液性中提取DNA,并通过动酶DNA(kDNA)特异性引物通过聚合酶链反应(PCR)和巢式PCR来确定物种。 CL的诊断标准是基于对涂片中的变形虫,培养中的前鞭毛虫,PCR中预期带的存在或巢式PCR的观察。在130个标本中,显微培养,PCR,巢式PCR以及组合PCR和显微镜检查阳性的有87个(66.9%),72个(56.2%),98个(75.4%),96个(73.8%)和99个(76.2%)阳性(建议的方法)。对于显微镜,PCR的灵敏度,特异性,阳性和阴性预测值分别为99%,100%,100%,96.9%,对于显微镜检查分别为87.9%,100%,100%,72.1%,对于培养物则为72.7%,100%,100% ,53.4%和嵌套PCR分别为97%,100%,100%和91.2%。根据研究结果,kDNA-PCR是诊断CL最敏感的方法。

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