Identification of an  Alu  element‐mediated deletion in the promoter region of   GNE   in siblings with  GNE  myopathy | Zendy

Garland Jennifer | Zendy; Stephen Joshi | Zendy; Class Bradley | Zendy; Gruber Angela | Zendy; Ciccone Carla | Zendy; Poliak Aaron | Zendy; Hayes Christina P. | Zendy; Singhal Vandana | Zendy; Slota Christina | Zendy; Perreault John | Zendy; Gavrilova Ralitza | Zendy; Shrader Joseph A. | Zendy; Chittiboina Prashant | Zendy; Joe Galen | Zendy; Heiss John | Zendy; Gahl William A. | Zendy; Huizing Marjan | Zendy; Carrillo Nuria | Zendy; Malicdan May Christine V. | Zendy

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Identification of an Alu element‐mediated deletion in the promoter region of GNE in siblings with GNE myopathy

Author(s) -

Garland Jennifer,

Stephen Joshi,

Class Bradley,

Gruber Angela,

Ciccone Carla,

Poliak Aaron,

Hayes Christina P.,

Singhal Vandana,

Slota Christina,

Perreault John,

Gavrilova Ralitza,

Shrader Joseph A.,

Chittiboina Prashant,

Joe Galen,

Heiss John,

Gahl William A.,

Huizing Marjan,

Carrillo Nuria,

Malicdan May Christine V.

Publication year - 2017

Publication title -

molecular genetics and genomic medicine

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.765

H-Index - 29

ISSN - 2324-9269

DOI - 10.1002/mgg3.300

Subject(s) - myopathy , exon , muscle biopsy , biology , genetics , gene , mutation , microbiology and biotechnology , pathology , medicine , biopsy

Abstract Background GNE myopathy is a rare genetic disease characterized by progressive muscle atrophy and weakness. It is caused by biallelic mutations in the GNE gene that encodes for the bifunctional enzyme, uridine diphosphate ( UDP )‐N‐acetylglucosamine (Glc NA c) 2‐epimerase/N‐acetylmannosamine (Man NA c) kinase. Typical characteristics of GNE myopathy include progressive myopathy, first involving anterior tibialis muscle and sparing the quadriceps, and rimmed vacuoles on muscle biopsy. Identifying biallelic mutations by sequencing of the GNE gene confirms the diagnosis of GNE myopathy. In a subset of patients, diagnostic confirmation is challenged by the identification of mutations in only one allele, suggesting mutations in deep intronic regions or regulatory regions. Methods We performed targeted sequencing and copy number variant ( CNV ) analysis of GNE in two siblings who clinically presented with GNE myopathy. Further molecular and biochemical studies were done to characterize the effect of a previously uncharacterized GNE mutation. Results We report two siblings of Indian descent with characteristic features of GNE myopathy, including progressive skeletal muscle weakness initially involving the anterior tibialis, and rimmed vacuoles on muscle biopsy, in which a heterozygous mutation, p.Val727Met, was identified in both affected siblings, but no other deleterious variants in either coding region or exon–intron boundaries of the gene. Subsequent insertion/deletion analysis identified a novel 11.3‐kb deletion (Chr9 [ GRC h37]: g.36257583_36268910del) encompassing the GNE promoter region, with breakpoints residing in Alu repeats. Gene expression analysis revealed reduced GNE mRNA and protein levels, confirming decreased expression of the deleted allele harboring the deletion. Conclusions We have identified GNE as one of the genes susceptible to Alu ‐mediated recombination. Our findings suggest that the deletion may encompass the promoter or another region necessary for GNE expression. In patients with typical manifestations of GNE myopathy and a single GNE variant identified, copy number variant ( CNV ) analysis may be useful in arriving at the diagnosis.

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