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Identification of Duchenne muscular dystrophy genomic probe P20 constant Taql fragment corresponding to the EcoRV and Mspl polymorphisms
Journal article   Peer reviewed

Identification of Duchenne muscular dystrophy genomic probe P20 constant Taql fragment corresponding to the EcoRV and Mspl polymorphisms

N. G Laing, A. P Walker, M. C Wapenaar, G VAN OMMEN, A. D Roses, B. A Kakulas, P. A Akkari, D. C Chandler, M. G Layton, M. E Mears, …
Prenatal diagnosis, Vol.11(1), pp.63-67
1991
PMID: 1709287

Abstract

Biological and medical sciences Diseases of striated muscles. Neuromuscular diseases Medical sciences Neurology
The majority of Duchenne and Becker muscular dystrophy cases are caused by deletions observable in Southern blots with cDNA probes for the gene. When the deletion includes polymorphic probes, they may be used to determine carrier status by deletion segregation analysis: non-inheritance of parental alleles, or heterozygosity. The polymorphic genomic probe P20 is deleted in a large percentage of probands. P20 hybridizes with two constant fragments of 6.7 and 0.8 kb in Taql digests. In a number of probands, only the larger P20 Taq1 fragment is deleted. This study demonstrates that this fragment corresponds with the polymorphic EcoRV and Mspl fragments of P20. Families in which the upper Taql fragment is deleted may be screened for carrier status using non-inheritance of parental alleles or heterozygosity of P20 in EcoRV or Mspl digests.

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Collaboration types
Domestic collaboration
International collaboration
Citation topics
1 Clinical & Life Sciences
1.255 Musculoskeletal Disorders
1.255.628 Duchenne Muscular Dystrophy
Web Of Science research areas
Genetics & Heredity
Obstetrics & Gynecology
ESI research areas
Clinical Medicine
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