Abstract

Proximal spinal muscular atrophy (SMA) is an autosomal recessive neuro-degenerative disease that is the primary genetic cause of infant mortality in the United States. Absence of the survival of motor neuron-1 gene (SMN1) gene product as a result of deletion or mutation leads to the disease. The SMN1 protein is necessary for motor neuron survival. The human genome harbors a nearly identical gene, SMN2, that is functionally redundant with SMN1 and could potentially rescue the disease phenotype. The SMN2 gene, however, is expressed at greatly reduced levels due to ineffective processing of the SMN2 RNA product. Specifically, the SMN2 varies from the SMN1 gene at a single nucleotide positioned in exon 7. This altered nucleotide leads to decreased recognition of exon 7 by the splicing machinery and results, ultimately, in skipping of the exon and the generation of a non-functional protein product. Correction of the SMN2 splicing phenotype is therefore a powerful therapeutic option to reinstate SMN activity in the correct time and place in SMA patients. However, no animal models exist to accurately test this therapeutic option. The primary goal of this proposal is to generate a SMA mouse model that contains the human SMN2 exon 7 point mutation in the mouse Smn gene. We hypothesize that this mouse model will more precisely recapitulate the human SMA condition relative to splicing of the SMN2 gene. Furthermore this model is necessary to address potential therapies aimed at correcting SMN2 splicing, and to evaluate the timing and dosage of SMN replacement therapies. We will use the new and improved SMA model to address the proper timing for the administration of such therapies. The main focus of this proposal is to generate mouse models for Spinal Muscular Atrophy (SMA), a devastating neuro-degenerative disease that is a primary genetic cause of infant mortality in the United States. In order to model the disease, we plan to generate a mouse model that has an alteration in the survival of motor neuron (SMN) gene that is known to lead to the SMA disease in humans. This mouse will be utilized to answer many questions pertaining the therapeutic possibilities of SMN gene replacement therapies with the long-term goal of testing candidate therapies to correct the neuro- degenerative defect in patients. ? ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Exploratory/Developmental Grants (R21)
Project #
1R21NS054690-01A2
Application #
7313482
Study Section
National Institute of Neurological Disorders and Stroke Initial Review Group (NSD)
Program Officer
Gwinn, Katrina
Project Start
2007-05-15
Project End
2009-04-30
Budget Start
2007-05-15
Budget End
2008-04-30
Support Year
1
Fiscal Year
2007
Total Cost
$157,500
Indirect Cost

  Institution

Name
Nationwide Children's Hospital
Department
Type
DUNS #
147212963
City
Columbus
State
OH
Country
United States
Zip Code
43205

  Publications

Bebee, Thomas W; Dominguez, Catherine E; Samadzadeh-Tarighat, Somayeh et al. (2012) Hypoxia is a modifier of SMN2 splicing and disease severity in a severe SMA mouse model. Hum Mol Genet 21:4301-13
Bebee, Thomas W; Gladman, Jordan T; Chandler, Dawn S (2011) Generation of a tamoxifen inducible SMN mouse for temporal SMN replacement. Genesis 49:927-34
Bebee, Thomas W; Gladman, Jordan T; Chandler, Dawn S (2010) Splicing of the Survival Motor Neuron genes and implications for treatment of SMA Front Biosci (Landmark Ed) 15:1191-1204
Gladman, Jordan T; Bebee, Thomas W; Edwards, Chris et al. (2010) A humanized Smn gene containing the SMN2 nucleotide alteration in exon 7 mimics SMN2 splicing and the SMA disease phenotype. Hum Mol Genet 19:4239-52
Gladman, Jordan T; Chandler, Dawn S (2009) Intron 7 conserved sequence elements regulate the splicing of the SMN genes. Hum Genet 126:833-41