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曲霉属胶原蛋白样基因(acl):鉴定、序列多态性及基于PCR的病原体检测评估

Aspergillus collagen-like genes (acl): identification, sequence polymorphism, and assessment for PCR-based pathogen detection.

作者信息

Tuntevski Kiril, Durney Brandon C, Snyder Anna K, Lasala P Rocco, Nayak Ajay P, Green Brett J, Beezhold Donald H, Rio Rita V M, Holland Lisa A, Lukomski Slawomir

机构信息

Department of Microbiology, Immunology, and Cell Biology.

出版信息

Appl Environ Microbiol. 2013 Dec;79(24):7882-95. doi: 10.1128/AEM.02835-13. Epub 2013 Oct 11.

Abstract

The genus Aspergillus is a burden to public health due to its ubiquitous presence in the environment, its production of allergens, and wide demographic susceptibility among cystic fibrosis, asthmatic, and immunosuppressed patients. Current methods of detection of Aspergillus colonization and infection rely on lengthy morphological characterization or nonstandardized serological assays that are restricted to identifying a fungal etiology. Collagen-like genes have been shown to exhibit species-specific conservation across the noncollagenous regions as well as strain-specific polymorphism in the collagen-like regions. Here we assess the conserved region of the Aspergillus collagen-like (acl) genes and explore the application of PCR amplicon size-based discrimination among the five most common etiologic species of the Aspergillus genus, including Aspergillus fumigatus, A. flavus, A. nidulans, A. niger, and A. terreus. Genetic polymorphism and phylogenetic analysis of the aclF1 gene were additionally examined among the available strains. Furthermore, the applicability of the PCR-based assay to identification of these five species in cultures derived from sputum and bronchoalveolar fluid from 19 clinical samples was explored. Application of capillary electrophoresis on nanogels was additionally demonstrated to improve the discrimination between Aspergillus species. Overall, this study demonstrated that Aspergillus acl genes could be used as PCR targets to discriminate between clinically relevant Aspergillus species. Future studies aim to utilize the detection of Aspergillus acl genes in PCR and microfluidic applications to determine the sensitivity and specificity for the identification of Aspergillus colonization and invasive aspergillosis in immunocompromised subjects.

摘要

曲霉属对公共卫生构成负担,因为其在环境中普遍存在,会产生过敏原,并且在囊性纤维化患者、哮喘患者和免疫抑制患者中具有广泛的人群易感性。目前检测曲霉定植和感染的方法依赖于冗长的形态学特征分析或非标准化的血清学检测,这些检测仅限于确定真菌病因。已表明胶原蛋白样基因在非胶原蛋白区域表现出物种特异性保守性,在胶原蛋白样区域表现出菌株特异性多态性。在此,我们评估了曲霉属胶原蛋白样(acl)基因的保守区域,并探索了基于PCR扩增子大小的鉴别方法在曲霉属五个最常见致病菌种(包括烟曲霉、黄曲霉、构巢曲霉、黑曲霉和土曲霉)中的应用。此外,还对现有菌株中的aclF1基因进行了遗传多态性和系统发育分析。此外,还探讨了基于PCR的检测方法在19份临床样本的痰液和支气管肺泡灌洗液培养物中鉴定这五个菌种的适用性。还证明了在纳米凝胶上应用毛细管电泳可提高曲霉属菌种之间的鉴别能力。总体而言,本研究表明曲霉属acl基因可作为PCR靶点用于区分临床相关的曲霉属菌种。未来的研究旨在利用PCR和微流控应用中曲霉属acl基因的检测来确定免疫功能低下受试者中曲霉定植和侵袭性曲霉病鉴定的敏感性和特异性。

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