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(Received for publication, April 4, 1996, and in revised form, July 8, 1996)
From the Section on Connective Tissue Disorders, Heritable
Disorders Branch, NICHD, National Institutes of Health,
Bethesda, Maryland 20892-1830
We have identified a novel multiexon
genomic deletion in one COL1A1 collagen allele that results in three
alternative forms of mutant mRNA. This mutation occurs in a
9-year-old girl and her father, both affected with severe type III
osteogenesis imperfecta (OI). We previously reported detection of a
mismatch in their PCR amplification and RNase protection experiments were used to
investigate the mRNA structure and occurrence of alternative
splicing. One form of the mutant cDNA has a deletion with end
points that are identical to the genomic deletion. This results in a
combination deletion/insertion, with a deletion of amino acids 603-639
followed by an insertion of 156 nt from the 3
Volume 271, Number 45,
Issue of November 8, 1996
pp. 28617-28623
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
1(I) amino acids 558-861 region by RNA/RNA hybrid
analysis (Grange, D. K., Gottesman, G. S., Lewis, M. B., and Marini, J.
C. (1990) Nucleic Acids Res. 18, 4227-4236). Single Strand
Conformational Polymorphism further localized the mRNA mutation to
the amino acids 579-679 coding region. At the gene level, polymerase
chain reaction (PCR) amplification of patient leukocyte DNA from the
exon 33-38 region yielded the normal 1004-base pair (bp) fragment and
an additional 442-bp fragment. Sequencing of the shorter genomic PCR
product confirmed the presence of a 562-bp deletion, extending from the
last 3 nucleotides (nt) of exon 34 to 156 nt from the 3
-end of intron
36. The genomic deletion was also detected in the clinically normal
grandmother, who was confirmed to be a mosaic carrier.
-end of intron 36. In
addition, we found two alternatively spliced forms. One form uses a
cryptic donor site in exon 34 and the exon 37 acceptor. The second form
uses the normal exon 32 splice donor and exon 37 acceptor. Use of the
cryptic donor results in a coding sequence that is out-of-frame. Both
the retained intron form and the use of the exon 32 donor site result
in coding sequences that are in-frame. This is the first report of a
collagen defect in OI with alternative splicing generating both
in-frame and out-of-frame forms of mRNA. Although the in-frame
forms constitute more than 60% of the mRNA from the mutant allele,
no mutant protein chain was identified. Collagen produced by cultured
OI osteoblasts showed a significant increase in the relative amount of
type III collagen but no mutant 1(I) chain.
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  X. Roca, R. Sachidanandam, and A. R. Krainer Intrinsic differences between authentic and cryptic 5' splice sites Nucleic Acids Res., November 1, 2003; 31(21): 6321 - 6333. [Abstract] [Full Text] [PDF]
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