| Literature DB >> 25772937 |
Lucas Fares-Taie1, Sylvie Gerber1, Akihiko Tawara2, Arturo Ramirez-Miranda3, Jean-Yves Douet4, Hannah Verdin5, Antoine Guilloux1, Juan C Zenteno6, Hiroyuki Kondo2, Hugo Moisset1, Bruno Passet7, Ken Yamamoto8, Masaru Iwai9, Toshihiro Tanaka10, Yusuke Nakamura11, Wataru Kimura12, Christine Bole-Feysot13, Marthe Vilotte7, Sylvie Odent14, Jean-Luc Vilotte7, Arnold Munnich1, Alain Regnier4, Nicolas Chassaing15, Elfride De Baere5, Isabelle Raymond-Letron4, Josseline Kaplan1, Patrick Calvas15, Olivier Roche16, Jean-Michel Rozet17.
Abstract
Congenital microcoria (MCOR) is a rare autosomal-dominant disorder characterized by inability of the iris to dilate owing to absence of dilator pupillae muscle. So far, a dozen MCOR-affected families have been reported worldwide. By using whole-genome oligonucleotide array CGH, we have identified deletions at 13q32.1 segregating with MCOR in six families originating from France, Japan, and Mexico. Breakpoint sequence analyses showed nonrecurrent deletions in 5/6 families. The deletions varied from 35 kbp to 80 kbp in size, but invariably encompassed or interrupted only two genes: TGDS encoding the TDP-glucose 4,6-dehydratase and GPR180 encoding the G protein-coupled receptor 180, also known as intimal thickness-related receptor (ITR). Unlike TGDS which has no known function in muscle cells, GPR180 is involved in the regulation of smooth muscle cell growth. The identification of a null GPR180 mutation segregating over two generations with iridocorneal angle dysgenesis, which can be regarded as a MCOR endophenotype, is consistent with the view that deletions of this gene, with or without the loss of elements regulating the expression of neighboring genes, are the cause of MCOR.Entities:
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Year: 2015 PMID: 25772937 PMCID: PMC4385178 DOI: 10.1016/j.ajhg.2015.01.014
Source DB: PubMed Journal: Am J Hum Genet ISSN: 0002-9297 Impact factor: 11.025