Direct detection and genotyping of Toxoplasma gondii in meat samples using magnetic capture and PCR

被引:179
作者
Opsteegh, Marieke [1 ,2 ]
Langelaar, Merel [1 ]
Sprong, Hein [1 ]
den Hartog, Laurien [1 ]
De Craeye, Stephane [3 ]
Bokken, Gertie [2 ]
Ajzenberg, Daniel [4 ,5 ]
Kijlstra, Aize [6 ]
van der Giessen, Joke [1 ]
机构
[1] Natl Inst Publ Hlth & Environm, NL-3720 BA Bilthoven, Netherlands
[2] Univ Utrecht, Inst Risk Assessment Sci, Utrecht, Netherlands
[3] Direct Communicable & Infect Dis, Sci Inst Publ Hlth, Brussels, Belgium
[4] Ctr Hosp Univ Dupuytren, CNR, Toxoplasmose Toxoplasma Biol Resource Ctr BRC, Limoges, France
[5] Univ Limoges, Fac Med, Lab Parasitol Mycol, Limoges, France
[6] Univ Wageningen & Res Ctr, Anim Sci Grp, Lelystad, Netherlands
关键词
Toxoplasma gondii; Detection; Meat; Magnetic capture; Quantitative PCR; Genotyping; Source attribution; Bioassay; POLYMERASE-CHAIN-REACTION; CONGENITAL TOXOPLASMOSIS; TISSUES; SHEEP; DNA; HISTOPATHOLOGY; INFECTION; BIOASSAY; ANTIGEN;
D O I
10.1016/j.ijfoodmicro.2010.02.027
中图分类号
TS2 [食品工业];
学科分类号
0832 ;
摘要
Different transmission routes, including the ingestion of undercooked meat, can result in Toxoplasma gondii infection in humans. The development of effective prevention strategies is hampered by a lack of quantitative information on the contamination level of different types of meat. Therefore, we developed a method for detection and quantification of T. gondii. The method involved preparation of crude DNA extract from hundred gram samples of meat, magnetic capture of T. gondii DNA and, quantitative real-time PCR targeting the T. gondii 529-bp repeat element. The detection limit of this assay was approximately 230 tachyzoites per 100 g of meat sample. There was a linear relation between the number of parasites added to the samples and Cp-values. Results obtained with the PCR method were comparable to bioassay results for experimentally infected pigs, and to serological findings for sheep. In addition, the T. gondii in 50% of the positive sheep samples could be genotyped by sequencing of the GRA6 gene, after isolation of the gene by magnetic capture. Two subtypes of GRAB type II were identified in the 16 samples from sheep. For seven samples, the identification of T. gondii as type II was confirmed by microsatellite typing. The PCR method can be used as an alternative to bioassay for detection and genotyping of T. gondii, and to quantify the organism in meat samples of various sources. (C) 2010 Elsevier B.V. All rights reserved.
引用
收藏
页码:193 / 201
页数:9
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