Abstract

The investigator has evaluated a 5 generation family (MN1) with a previously undefined autosomal dominant muscle disease. Although this family has the clinical features associated with myotonic dystrophy (myotonia, neck and facial weakness, frontal balding, cataracts and cardiac arrhythmias), affected individuals do not have the CTG expansion associated with DM, nor is the disease locus linked to the DM region of chromosome 19. The investigator also excluded linkage to the other genetic loci that cause myotonia, i.e., the muscle sodium channel gene (SCN4A) and the chloride channel gene (CLC-1). The identification of a second locus for myotonic dystrophy will facilitate the identification of additional families with the MN1 form of myotonic dystrophy and will be a first step toward identifying the MN1 gene. Because the MN1 disorder causes the same broad range of clinical features as classic myotonic dystrophy, the eventual isolation and characterization of the gene(s) affected will provide insights into the pathology of both DM and the disease afflicting the MN1 family.
Our specific aims are: A) To further characterize patients clinically by performing: 1) blood tests to look for muscle fiber disruption, glucose intolerance, and primary gonadal failure in males; 2) EMG studies to better characterize their myotonia; 3) EKG studies to look for conduction block and arrhythmias; 4) muscle biopsies to characterize their myopathy. B) To identify and study additional branches of the MN1 family that are affected by the disease and to look for additional unrelated families with the MN1 form of myotonic dystrophy. C) To localize the MN1 gene to a specific chromosome by linkage analysis. Preliminary results indicate a high likelihood of detecting linkage by performing a genome screen using a marker spacing of 10 cM (360 markers). D) To construct a high resolution (1-2 cM) genetic map for the chromosomal region containing the MN1 gene. In order to genetically narrow the critical region containing the MN1 gene to a 1-2 cM interval it is anticipated that we will need to identify additional branches of the family and or other families with the MN1 form of """"""""myotonic dystrophy"""""""". Once the MN1 locus has been well mapped, candidate genes within the region can be examined for their possible involvement in the disease process. If the number of affected individuals is sufficient to allow us to narrow the candidate region to 1-2 cM, then physical mapping and cloning strategies will be used to isolate the defective gene.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Neurological Disorders and Stroke (NINDS)
Type
Research Project (R01)
Project #
5R01NS035870-03
Application #
2892176
Study Section
Mammalian Genetics Study Section (MGN)
Program Officer
Spinella, Giovanna M
Project Start
1997-06-01
Project End
2000-05-31
Budget Start
1999-06-01
Budget End
2000-05-31
Support Year
3
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
University of Minnesota Twin Cities
Department
Neurology
Type
Schools of Medicine
DUNS #
168559177
City
Minneapolis
State
MN
Country
United States
Zip Code
55455

  Publications

Cleary, John Douglas; Ranum, Laura Pw (2017) New developments in RAN translation: insights from multiple diseases. Curr Opin Genet Dev 44:125-134
Savkur, R S; Philips, A V; Cooper, T A et al. (2004) Insulin receptor splicing alteration in myotonic dystrophy type 2. Am J Hum Genet 74:1309-13
Day, J W; Roelofs, R; Leroy, B et al. (1999) Clinical and genetic characteristics of a five-generation family with a novel form of myotonic dystrophy (DM2). Neuromuscul Disord 9:19-27
Koob, M D; Benzow, K A; Bird, T D et al. (1998) Rapid cloning of expanded trinucleotide repeat sequences from genomic DNA. Nat Genet 18:72-5
Ranum, L P; Rasmussen, P F; Benzow, K A et al. (1998) Genetic mapping of a second myotonic dystrophy locus. Nat Genet 19:196-8