S. Hori et al., MULTIPLICITY OF ABNORMAL DYSTROPHIN IN BECKER MUSCULAR-DYSTROPHY - A BECKER MUSCULAR-DYSTROPHY GENE FREQUENTLY PRODUCED 2 SMALLER SIZES OF DYSTROPHIN, Journal of the neurological sciences, 121(2), 1994, pp. 183-189
Dystrophin is a muscle cytoskeletal protein with a molecular mass (MM)
of similar to 420 kDa and an isoelectric point (pI) of similar to 5.5
, which is abnormal in size and/or abundance in Becker muscular dystro
phy (BMD). We investigated the abnormality of dystrophin molecule in m
uscles biopsied from 23 BMD patients using the two-dimensional gel ele
ctrophoresis (TDGE). We found 7 protein spots which reacted specifical
ly with the monoclonal anti-dystrophin antibody (mAb) A1C raised again
st N-terminal domain of the normal dystrophin. These spots were focuse
d on the two-dimensional gel at the same position as the normal dystro
phin (#1), at the position with MM similar to 480 kDa/pI similar to 5.
35 (#2), the position with MM similar to 400-330 kDa/pI similar to 5.5
1-5.47(#3), the position with MM similar to 300 kDa/pI similar to 5.4(
#4), the position with MM similar to 235-250 kDa/pI similar to 5.53-5.
5 (#5), the position with MM similar to 165 kDa/pI similar to 6.0(#6),
and the position with MM similar to 160 kDa/pI similar to 5.75(#7). T
hese spots were classified into five patterns in individuals, that is,
#1 alone in 3 patients, #3 alone in 1, the combination of #3 and 5 in
17, the combination of #1, 3 and 5 in 1 and the combination of #1, 2,
4, 6 and 7 in 1. The combination of #3 and 5 was observed in 17 of 23
patients (75%). In addition, both of #3 and 5 reacted not only with t
he mAbs, AIC, Dys 3 and 5E2, which recognize the N-terminal domain of
the normal dystrophin, but also with the mAbs, 4C5 and Dys 2, which re
cognize the C-terminal domain. Thus, each of #3 and 5 preserved both N
- and C-terminal domains of the normal dystrophin in spite of signific
ant differences in MM and pI Our observations conclude that the #5 is
not a proteolytic fragment of the ''full-length'' dystrophin (#3), and
suggest that some exons encoding triple helical segments at the centr
al portion of dystrophin are spliced out to produce two abnormal dystr
ophins from a single mutated gene in the majority of BMD.