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Journal of Lipid Research, Vol 36, 931-938, Copyright © 1995 by Lipid Research, Inc.
M Miller, K Zeller, PC Kwiterovich, JJ Albers and G Feulner
Previous mutations associated with lecithin:cholesterol acyltransferase
(LCAT) deficiency have been identified using genomic DNA. To facilitate
mutation analysis, we used cDNA from cultured fibroblasts which were shown
to express LCAT mRNA. Using reverse-transcriptase PCR, LCAT cDNA was
obtained from a 13-year-old boy with complete LCAT deficiency,
characterized by low HDL-C (3 mg/dl), nondetectable initial cholesterol
esterification rate, LCAT activity, and minimal LCAT mass (0.16 vs. 5- 7.5
micrograms/ml). Sequencing of LCAT cDNA clones identified two mutations. A
novel frameshift mutations caused by deletion of cytosine at the third
nucleotide position of amino acid 168 (exon 5) predicts a disrupted protein
catalytic site by converting Ser181-->Ala and creates a Pvu-II
restriction site prior to premature truncation at amino acid 238. A
C-->T transition results in a substitution of methionine for threonine
at amino acid position 321 and creates an Nla-III restriction site on the
maternal allele. Expression studies of mutant LCAT cDNA confirmed the
virtual absence of LCAT activity in transfected COS-1 cells. The molecular
defect in a young male with complete LCAT deficiency has been identified
using fibroblast cDNA.
ARTICLES
Lecithin: cholesterol acyltransferase deficiency: identification of two defective alleles in fibroblast cDNA
Department of Medicine, Veterans Administration Medical Center, Baltimore, MD 21201, USA.
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