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mdx muscle pathology is independent of nNOS perturbationopen access

Authors
Crosbie, Rachelle HStraub, VolkerYun, Hye-YoungLee, Jane CRafael,Jill AChamberlain, Rafael Jeffrey SDawson, Valina LDawson, Ted MCampbell, Kevin P
Issue Date
May-1998
Publisher
OXFORD UNIV PRESS
Citation
HUMAN MOLECULAR GENETICS, v.7, no.5, pp 823 - 829
Pages
7
Journal Title
HUMAN MOLECULAR GENETICS
Volume
7
Number
5
Start Page
823
End Page
829
URI
https://scholarworks.bwise.kr/cau/handle/2019.sw.cau/66754
DOI
10.1093/hmg/7.5.823
ISSN
0964-6906
1460-2083
Abstract
In skeletal muscle, neuronal nitric oxide synthase (nNOS) is anchored to the sarcolemma via the dystrophin-glycoprotein complex. When dystrophin is absent, as in Duchenne muscular dystrophy patients and in mdx mice, nNOS is mislocalized to the interior of the muscle fiber where it continues to produce nitric oxide. This has led to the hypothesis that free radical toxicity from mislocalized nNOS may contribute to mdx muscle pathology. To test this hypothesis directly, we generated mice devoid of both nNOS and dystrophin. Overall, the nNOS-dystrophin null mice maintained the dystrophic characteristics of mdx mice. We evaluated the mice for several features of the dystrophic phenotype, including membrane damage and muscle morphology. Removal of nNOS did not alter the extent of sarcolemma damage, which is a hallmark of the dystrophic phenotype. Furthermore, muscle from nNOS-dystrophin null mice maintain the histological features of mdx pathology. Our results demonstrate that relocalization of nNOS to the cytosol does not contribute significantly to mdx pathogenesis.
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