Circulation, Vol 86, 147-153, Copyright © 1992 by American Heart Association
RD Bies, D Friedman, R Roberts, MB Perryman and CT Caskey
BACKGROUND. Mutations in the dystrophin gene produce clinical
manifestations of disease in heart, brain, and skeletal muscle in patients
with Duchenne and Beckers muscular dystrophy (DMD/BMD). Conduction
disturbances and heart block contribute to cardiac decompensation in these
patients, which suggests an important role for dystrophia in the cardiac
conduction system. We therefore examined the messenger RNA (mRNA)
expression and protein localization of dystrophin in normal human cardiac
Purkinje fibers. METHODS AND RESULTS. Polymerase chain reaction
amplification of isolated Purkinje fiber complementary DNA identified
several alternatively spliced mRNA transcripts encoding for
carboxy-terminal isoforms of the dystrophin protein. The predominant mRNA
transcript detected was a splice form previously detected in the brain.
Antipeptide antibodies specific for a carboxy-terminal dystrophin sequence
were used for Western blot analysis and immunocytochemical localization.
These antisera detect approximately 400,000-d immunoreactive band or bands
on Western blot in normal heart and Purkinje fibers but not in DMD heart.
Immunocytochemical staining showed that dystrophin was localized to the
membrane surface of the Purkinje fiber. CONCLUSIONS. These results suggest
that dystrophin may be an important molecule for membrane function in the
Purkinje conduction system of the heart and support the hypothesis that
defective dystrophin expression contributes to the cardiac conduction
disturbances seen in DMD/BMD.
ARTICLES
Expression and localization of dystrophin in human cardiac Purkinje fibers
Cardiology Division, Baylor College of Medicine, Houston, Tex.
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