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AMCoR:Asahikawa Medical University Collection and Research (旭川医科大学学術成果リポジトリ)は、本学で生産された電子的な知的生産物(学術雑誌論文の原稿・教材・学術資料など)を保存し、原則的に無償で発信するためのインターネット上の保管庫です。

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閲覧数:3282
ID 14766815
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タイトル DNA differential diagnosis of taeniasis and cysticercosis by multiplex PCR
著者
伊藤, 亮 (Ito, Akira)
Yamasaki, H
Allan, JC
Sato, MO
Sako, Y
Nakaya, K
Dongchuan, Q
Nakao, M
Mamuti, W
Craig, PS
上位タイトル
Journal of Clinical Microbiology Vol.42, No.2  (2004. 2) ,p.548- 553
識別番号
ISSN
0095-1137
DOI 10.1128/JCM.42.2.548-553.2004
URI http://www.ncbi.nlm.nih.gov/pubmed/14766815
抄録 Multiplex PCR was established for differential diagnosis of taeniasis and cysticercosis, including their causative agents. For identification of the parasites, multiplex PCR with cytochrome c oxidase subunit 1 gene yielded evident differential products unique for Taenia saginata and Taenia asiatica and for American/African and Asian genotypes of Taenia solium with molecular sizes of 827, 269, 720, and 984 bp, respectively. In the PCR-based detection of tapeworm carriers using fecal samples, the diagnostic markers were detected from 7 of 14 and 4 of 9 T. solium carriers from Guatemala and Indonesia, respectively. Test sensitivity may have been reduced by the length of time (up to 12 years) that samples were stored and/or small sample volumes (ca. 30 to 50 mg). However, the diagnostic markers were detected by nested PCR in five worm carriers from Guatemalan cases that were found to be negative by multiplex PCR. It was noteworthy that a 720 bp-diagnostic marker was detected from a T. solium carrier who was egg-free, implying that it is possible to detect worm carriers and treat before mature gravid proglottids are discharged. In contrast to T. solium carriers, 827-bp markers were detected by multiplex PCR in all T. saginata carriers. The application of the multiplex PCR would be useful not only for surveillance of taeniasis and cysticercosis control but also for the molecular epidemiological survey of these cestode infections.
注記 Copyright © American Society for Microbiology, Journal of Clinical Microbiology, volume 42, 548-553, 2004

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