| Literature DB >> 20064630 |
Yutaka Nishigaki1, Hitomi Ueno, Jorida Coku, Yasutoshi Koga, Tatsuya Fujii, Ko Sahashi, Kazutoshi Nakano, Makoto Yoneda, Michiko Nonaka, Linya Tang, Chia-Wei Liou, Veronique Paquis-Flucklinger, Yasuo Harigaya, Tohru Ibi, Yu-ichi Goto, Hiroko Hosoya, Salvatore DiMauro, Michio Hirano, Masashi Tanaka.
Abstract
We established an extensive and rapid system using suspension array to detect 61 representative mitochondrial DNA (mtDNA) heteroplasmic or homoplasmic point mutations (29 for Series A and 32 for Series B) in 22 genes: 1 each in MT-RNR1, -TV, -ND1, -TQ, -TW, -TC, and -TH genes; 2 each in MT-TN, -TG, -ND4, -TL2, -TE, and -CYB genes; 3 each in MT-ATP6, -ND3, and -ND5 genes; 4 each in MT-CO1 and -TK genes; 5 each in MT-TI, -TS1, and -ND6 genes; and 10 in the MT-TL1 gene. We carefully selected 5'-biotinylated primers and pooled primers for use in two sets of multiplex-PCR amplifications. To detect both mutant and wild-type mtDNA, even when polymorphisms were present near the target mutation sites, we designed specific oligonucleotide probes. By using the mtDNA point mutation detection system of Series A (29 mutations) and Series B (32 mutations), we screened a total of 3103 mutant sites in 107 DNA samples for Series A and 13,101 mutant sites in 397 DNA samples for Series B. We succeeded in determining 99.4% (Series A) and 99.6% (Series B) of the targeted mutant sites by use of the system. The 22 samples with the m.3243A>G heteroplasmic mutation revealed positive signals with both mutant- and wild-type-specific probes in this detection system with a detection limit of approximately 2%. This genetic screening platform is useful to reach a definitive diagnosis for mitochondrial diseases. Copyright 2010 Mitochondria Research Society. Published by Elsevier B.V. All rights reserved.Entities:
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Year: 2010 PMID: 20064630 PMCID: PMC7568344 DOI: 10.1016/j.mito.2010.01.003
Source DB: PubMed Journal: Mitochondrion ISSN: 1567-7249 Impact factor: 4.160