Application of in vitro myo-differentiation of non-muscle cells to enhance gene expression and facilitate analysis of muscle proteins

被引:23
作者
Roest, PAM
vanderTuijn, AC
Ginjaar, HB
Hoeben, RC
HogerVorst, FBL
Bakker, E
denDunnen, JT
vanOmmen, GJB
机构
[1] LEIDEN UNIV,DEPT HUMAN GENET,MGC,2333 AL LEIDEN,NETHERLANDS
[2] LEIDEN UNIV,DEPT BIOCHEM MED,MGC,2333 AL LEIDEN,NETHERLANDS
[3] AZL,KLIN GENET CTR LEIDEN,LEIDEN,NETHERLANDS
关键词
Duchenne and Becker muscular dystrophy; MyoD; myogenesis; dystrophin; mutation detection;
D O I
10.1016/0960-8966(96)00006-5
中图分类号
R74 [神经病学与精神病学];
学科分类号
摘要
Introduction of the myogenic-determination gene MyoD forces non-muscle cell cultures into myogenesis, thereby inducing expression of muscle-specific proteins and facilitating their analysis. In several MyoD-transfected fibroblasts, immunohistochemical detection showed expression of desmin after three days, of titin after five days and of dystrophin after seven days. Cell fusion (myotube formation) could be observed after five days. After nine days a fraction of the cells showed a striated titin pattern, indicating an advanced state of muscle differentiation. Dystrophin (the protein absent in Ducbenne Muscular Dystrophy patients) can be detected in MyoD-transfected and differentiated fibroblasts from healthy individuals, and is absent in those of patients. MyoD-transfection increases transcription of the dystrophin gene, facilitating RNA-based mutation detection. Using RNA from MyoD-transfected, differentiated fibroblasts of a deceased patient with an unknown, non-deletion mutation, we were able to identify a CGA-->TGA nonsense mutation in the rod domain at basepair 6492 and to establish a rapid mutation specific test for future diagnosis of the mutation in his relatives. Copyright (C) 1996 Elsevier Science Ltd.
引用
收藏
页码:195 / 202
页数:8
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