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通过对hsp65 PCR产物进行高分辨率熔解分析快速鉴定龟分枝杆菌-脓肿分枝杆菌组内的菌种

Rapid species identification within the Mycobacterium chelonae-abscessus group by high-resolution melting analysis of hsp65 PCR products.

作者信息

Odell Ian D, Cloud Joann L, Seipp Michael, Wittwer Carl T

机构信息

Department of Pathology, University of Utah Medical School, Salt Lake City, 84132, USA.

出版信息

Am J Clin Pathol. 2005 Jan;123(1):96-101. doi: 10.1309/wdr082x9ffjbqqgb.

Abstract

Polymerase chain reaction (PCR) amplification of the heat shock protein 65 (hsp65) gene followed by high-resolution melting analysis with LCGreen I (Idaho Technology, Salt Lake City, UT) was used to differentiate the mycobacteria species Mycobacterium chelonae, Mycobacterium abscessus, and Mycobacterium immunogenum in less than 20 minutes. A 105-base-pair amplicon that clustered the different species by predicted melting temperature was found from available GenBank hsp65 sequences. We identified 24 clinical isolates within the M chelonae-abscessus group by proximal 16S ribosomal RNA and hsp65 gene sequencing. Rapid-cycle PCR followed by high-resolution melting analysis clustered these samples into the following groups: M abscessus, 12; M abscessus sequence variant, 2; M chelonae, 7; unexpected M chelonae sequence variant, 1; and M immunogenum, 2. The M chelonae variant had a single base change not found in reported GenBank sequences. Advantages of the method include speed, low risk of amplicon contamination (closed-tube), and no need for separation steps (sequencing, electrophoresis, high-performance liquid chromatography) or real-time monitoring.

摘要

采用聚合酶链反应(PCR)扩增热休克蛋白65(hsp65)基因,随后用LCGreen I(爱达荷技术公司,盐湖城,犹他州)进行高分辨率熔解分析,可在不到20分钟内区分龟分枝杆菌、脓肿分枝杆菌和免疫分枝杆菌这几种分枝杆菌。从GenBank中现有的hsp65序列中发现了一个105个碱基对的扩增子,该扩增子根据预测的熔解温度对不同物种进行聚类。我们通过近端16S核糖体RNA和hsp65基因测序鉴定了24株龟分枝杆菌-脓肿分枝杆菌组的临床分离株。快速循环PCR结合高分辨率熔解分析将这些样本分为以下几组:脓肿分枝杆菌,12株;脓肿分枝杆菌序列变异株,2株;龟分枝杆菌,7株;意外的龟分枝杆菌序列变异株,1株;免疫分枝杆菌,2株。龟分枝杆菌变异株有一个在已报道的GenBank序列中未发现的单碱基变化。该方法的优点包括速度快、扩增子污染风险低(闭管),且无需分离步骤(测序、电泳、高效液相色谱)或实时监测。

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