| Literature DB >> 23790109 |
Hiroki Takagi1,2, Aiko Uemura1, Hiroki Yaegashi1, Muluneh Tamiru1, Akira Abe1, Chikako Mitsuoka1, Hiroe Utsushi1, Satoshi Natsume1,2, Hiroyuki Kanzaki1, Hideo Matsumura3, Hiromasa Saitoh1, Kentaro Yoshida1,4, Liliana M Cano4, Sophien Kamoun4, Ryohei Terauchi1.
Abstract
Next-generation sequencing allows the identification of mutations responsible for mutant phenotypes by whole-genome resequencing and alignment to a reference genome. However, when the resequenced cultivar/line displays significant structural variation from the reference genome, mutations in the genome regions missing from the reference (gaps) cannot be identified by simple alignment. Here we report on a method called 'MutMap-Gap', which involves delineating a candidate region harboring a mutation of interest using the recently reported MutMap method, followed by de novo assembly, alignment, and identification of the mutation within genome gaps. We applied MutMap-Gap to isolate the blast resistant gene Pii from the rice cv Hitomebore using mutant lines that have lost Pii function. MutMap-Gap should prove useful for cloning genes that exhibit significant structural variations such as disease resistance genes of the nucleotide-binding site-leucine rich repeat (NBS-LRR) class.Entities:
Keywords: MutMap; R-gene; de novo assembly; next-generation sequencing; rice; whole-genome sequencing
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Year: 2013 PMID: 23790109 DOI: 10.1111/nph.12369
Source DB: PubMed Journal: New Phytol ISSN: 0028-646X Impact factor: 10.151