Establishment of a semi-automated pathogen DNA isolation from whole blood and comparison with commercially available kits

被引:24
|
作者
Wiesinger-Mayr, Herbert [1 ]
Jordana-Lluch, Elena [2 ]
Martro, Elisa [2 ,3 ]
Schoenthaler, Silvia [1 ]
Noehammer, Christa [1 ]
机构
[1] AIT Austrian Inst Technol GmbH, A-1190 Vienna, Austria
[2] Autonomous Univ Barcelona, Germans Trias & Pujol Univ Hosp, Microbiol Serv, Badalona, Spain
[3] Biomed Res Ctr Network Epidemiol & Publ Hlth CIBE, Barcelona, Spain
关键词
DNA isolation; Bloodstream infection; Molecular diagnostics; Sepsis; Automation; BACTERIAL PATHOGENS; MICROBIAL DNA; PCR; MICROARRAY; IDENTIFICATION; BACTEREMIA; EXTRACTION; DIAGNOSIS; SAMPLES;
D O I
10.1016/j.mimet.2011.03.003
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Molecular methods for bacterial pathogen identification are gaining increased importance in routine clinical diagnostic laboratories. Achieving reliable results using DNA based technologies is strongly dependent on pre-analytical processes including isolation of target cells and their DNA of high quality and purity. In this study a fast and semi-automated method was established for bacterial DNA isolation from whole blood samples and compared to different commercially available kits: Looxster, MolYsis kit, SeptiFast DNA isolation method and standard EasyMAG protocol. The newly established, semi-automated method utilises the EasyMAG device combined with pre-processing steps comprising human cell lysis, centrifugation and bacterial pellet resuspension. Quality of DNA was assessed by a universal PCR targeting the 16S rRNA gene and subsequent microarray hybridisation. The DNA extractions were amplified using two different PCR-mastermixes, to allow comparison of a commercial mastermix with a guaranteed bacterial DNA free PCR mastermix. The modified semi-automated EasyMAG protocol and the Looxster kit gave the most sensitive results. After hybridisation a detection limit of 10(1) to 10(2) bacterial cells per mL whole blood was achieved depending on the isolation method and microbial species lysed. Human DNA present in the isolated DNA suspension did not interfere with PCR and did not lead to non-specific hybridisation events. (C) 2011 Elsevier B.V. All rights reserved.
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页码:206 / 213
页数:8
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