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首页> 外文期刊>Journal of Clinical Microbiology >Preparation of mycobacterial DNA from blood culture fluids by simple alkali wash and heat lysis method for PCR detection.
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Preparation of mycobacterial DNA from blood culture fluids by simple alkali wash and heat lysis method for PCR detection.

机译:通过简单的碱洗和热裂解法从血液培养液中制备分枝杆菌DNA进行PCR检测。

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摘要

A sodium iodide-isopropanol (NI) method was compared with an alkali wash and heat lysis (AH) procedure for the preparation and extraction of DNA from BACTEC 13A blood culture fluid samples from AIDS patients for use in a PCR for the detection and identification of mycobacteria. The sensitivity and efficiency of the DNA extraction methods were assessed by a multiplex PCR which detected the members of the genus Mycobacterium and differentiated between M. intracellulare, M. tuberculosis, and M. avium isolates with a limit of detection of between 0.28 pg (67 cells) and 120 pg (28,571 cells) of standard mycobacterial DNA. The PCR amplified mycobacterial DNA prepared by the AH procedure from 40 acid-fast bacillus-positive blood cultures with growth index values of > 20 U but not from 48 blood cultures with growth index values of < 21 U. The AH method was about 10 times more sensitive than the NI method for extracting DNA from 13 acid-fast bacillus-positive BACTEC fluid samples for PCR analysis. The study shows that the AH procedure in combination with the multiplex PCR is a simple, specific, and sensitive method which can be used in the routine diagnostic laboratory to detect and identify different members of the genus Mycobacterium in blood culture fluid samples from AIDS patients.
机译:将碘化钠-异丙醇(NI)方法与碱洗和热裂解(AH)方法进行了比较,以从AIDS患者的BACTEC 13A血液培养液样品中制备和提取DNA,用于PCR检测和鉴定分枝杆菌。通过多重PCR评估DNA提取方法的灵敏度和效率,该PCR检测了分枝杆菌属的成员,并区分了胞内分枝杆菌,结核分枝杆菌和鸟分枝杆菌,检出限在0.28 pg之间(67细胞)和120 pg(28,571个细胞)的标准分枝杆菌DNA。 PCR通过AH程序从40株生长指数值> 20 U的抗酸杆菌阳性血液培养物中扩增分枝杆菌DNA,而不是从48株生长指数值<21 U的血液培养物中扩增分枝杆菌DNA。AH方法约为10倍从NI提取13种耐酸杆菌阳性BACTEC液体样品中的DNA进行PCR分析的灵敏度比NI方法高。研究表明,AH程序与多重PCR结合是一种简单,特异性和灵敏的方法,可在常规诊断实验室中用于检测和鉴定来自AIDS患者的血液培养液样本中分枝杆菌属的不同成员。

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