REEP1 mutation spectrum and genotype/phenotype correlation in hereditary spastic paraplegia type 31.

6533b82ffe1ef96bd1294907

RESEARCH PRODUCT

REEP1 mutation spectrum and genotype/phenotype correlation in hereditary spastic paraplegia type 31.

Peter De Jonghe Margaret A. Pericak-vance Paula C. Byrne Jan Kassubek Bernard Dan Thomas Klopstock Wendy A. G. Van Zelst-stams Christian Beetz Suzanna G.m. Frints Sven Klimpe Tine Deconinck Berry Kremer Khanh-nhat Tran-viet H. Stolze Michael Hutchinson Jonathan Baets Thomas Deufel Hui Zhu Constance T.r.m. Schrander-stumpel Narasimhan Nagan Bart P.c. Van De Warrenburg Berten Ceulemans Hubert J.m. Smeets Stephan Züchner Rebecca Schüle Ludger Schöls Anders O H Nygren S. Otto Katrien Smets Corey D. Braastad

subject

Adult Male Mutation rate Adolescent Genotype Hereditary spastic paraplegia DNA Mutational Analysis Biology medicine.disease_cause Article Cognitive neurosciences [UMCN 3.2]Gene duplication Genotype medicine Perception and Action [DCN 1]Humans Copy-number variation Age of Onset Mutation frequency Child Aged Aged 80 and over Genetics Mutation Hereditary cancer and cancer-related syndromes [ONCOL 1]Spastic Paraplegia Hereditary Infant Membrane Transport Proteins Middle Aged medicine.disease Pedigree Phenotype Child Preschool Mutation Female Neurology (clinical)Haploinsufficiency Functional Neurogenomics [DCN 2]

description

Contains fulltext : 71291.pdf (Publisher’s version ) (Closed access) Mutations in the receptor expression enhancing protein 1 (REEP1) have recently been reported to cause autosomal dominant hereditary spastic paraplegia (HSP) type SPG31. In a large collaborative effort, we screened a sample of 535 unrelated HSP patients for REEP1 mutations and copy number variations. We identified 13 novel and 2 known REEP1 mutations in 16 familial and sporadic patients by direct sequencing analysis. Twelve out of 16 mutations were small insertions, deletions or splice site mutations. These changes would result in shifts of the open-reading-frame followed by premature termination of translation and haploinsufficiency. Interestingly, we identified two disease associated variations in the 3'-UTR of REEP1 that fell into highly conserved micro RNA binding sites. Copy number variation analysis in a subset of 133 HSP index patients revealed a large duplication of REEP1 that involved exons 2-7 in an Irish family. Clinically most SPG31 patients present with a pure spastic paraplegia; rare complicating features were restricted to symptoms or signs of peripheral nerve involvement. Interestingly, the distribution of age at onset suggested a bimodal pattern with the appearance of initial symptoms of disease either before the age of 20 years or after the age of 30 years. The overall mutation rate in our clinically heterogeneous sample was 3.0%; however, in the sub-sample of pure HSP REEP1 mutations accounted for 8.2% of all patients. These results firmly establish REEP1 as a relatively frequent autosomal dominant HSP gene for which genetic testing is warranted. We also establish haploinsufficiency as the main molecular genetic mechanism in SPG31, which should initiate and guide functional studies on REEP1 with a focus on loss-of-function mechanisms. Our results should be valid as a reference for mutation frequency, spectrum of REEP1 mutations, and clinical phenotypes associated with SPG31.

year	journal	country	edition	language
2008-01-01

10.1093/brain/awn026 http://hdl.handle.net/2066/71291