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采用 SmartGene IDNS [更正] 软件对 28S rDNA 大亚基的 D1/D2 区和内部转录间隔区进行核酸测序,以鉴定临床实验室中的丝状真菌。

Evaluation of nucleic acid sequencing of the D1/D2 region of the large subunit of the 28S rDNA and the internal transcribed spacer region using SmartGene IDNS [corrected] software for identification of filamentous fungi in a clinical laboratory.

机构信息

The Johns Hopkins Hospital Microbiology Laboratory, Department of Pathology, The Johns Hopkins University School of Medicine, 600 N Wolfe St, Baltimore, MD 21287, USA.

出版信息

J Mol Diagn. 2012 Jul;14(4):393-401. doi: 10.1016/j.jmoldx.2012.02.004. Epub 2012 May 11.

DOI:10.1016/j.jmoldx.2012.02.004
PMID:22579969
Abstract

Filamentous fungal infections have recently increased because of the increasing numbers of immunocompromised hosts. In this study, we evaluated DNA sequencing of the D1/D2 region of the large subunit of the 28S ribosomal RNA gene and the internal transcribed spacer (ITS) region using SmartGene (SG; SmartGene Inc., Raleigh, NC) for the identification of a broad range of commonly encountered filamentous fungi. The SG proofreaders were used to upload, align, and edit fragments, and the resultant sequences were interpreted using the quality-controlled SG database. The results were compared with reference identifications using conventional phenotypic methods or ITS DNA sequences obtained from GenBank if phenotypic identifications were inconclusive. A total of 146 clinical isolates were included in this study, representing 49 different genera. The overall agreements of the D1/D2 and the ITS sequencing methods to reference identification were 97.2% (95% CI, 93.1% to 98.9%) and 97.7% (95% CI, 92.8% to 99.4%), respectively. Of the 146 isolates, 18 (12.3%) did not amplify using the ITS universal primers after repeated attempts and, therefore, could not be sequenced using this target. Correct identification was achieved for 100% (95% CI, 97.4% to 100%) of the isolates when applying both the D1/D2 and ITS targets. In summary, DNA sequencing using SG software provides a rapid, accurate, and reliable tool for the identification of filamentous fungi in a clinical laboratory.

摘要

近年来,由于免疫功能低下宿主数量的增加,丝状真菌感染有所增加。在这项研究中,我们使用 SmartGene(SG;SmartGene Inc.,Raleigh,NC)评估了 28S 核糖体 RNA 基因大亚基的 D1/D2 区和内部转录间隔区(ITS)区的 DNA 测序,以鉴定广泛存在的常见丝状真菌。SG 校对员用于上传、对齐和编辑片段,并用经过质量控制的 SG 数据库解释生成的序列。将结果与使用传统表型方法或如果表型鉴定不确定则从 GenBank 获取的 ITS DNA 序列进行参考鉴定进行比较。这项研究共纳入了 146 株临床分离株,代表了 49 个不同的属。D1/D2 和 ITS 测序方法与参考鉴定的总体一致性分别为 97.2%(95%CI,93.1%至 98.9%)和 97.7%(95%CI,92.8%至 99.4%)。在 146 株分离株中,18 株(12.3%)在多次尝试后使用 ITS 通用引物未能扩增,因此无法使用该靶标进行测序。当应用 D1/D2 和 ITS 靶标时,100%(95%CI,97.4%至 100%)的分离株可以实现正确鉴定。总之,使用 SG 软件进行 DNA 测序为临床实验室鉴定丝状真菌提供了一种快速、准确和可靠的工具。

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