Single-nucleotide polymorphisms in the C-reactive protein (CRP) gene promoter that affect transcription factor binding, alter transcriptional activity, and associate with differences in baseline serum CRP level

Single-nucleotide polymorphisms in the C-reactive protein (CRP) gene promoter that affect transcription factor binding, alter transcriptional activity, and associate with differences in baseline serum CRP level

To investigate whether functional polymorphisms exist in the C-reactive protein (CRP) gene, i.e., ones that contribute directly to differences in baseline CRP among individuals, we sequenced a 1,156-nucleotide-long stretch of the CRP gene promoter in 287 ostensibly healthy people. We identified two...

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Bibliographic Details
Published in:Journal of molecular medicine (Berlin, Germany) Germany), 2005-06, Vol.83 (6), p.440-447
Main Authors: SZALAI, A. J, WU, J, XIE, F, FAN, Z, EDBERG, J. C, KIMBERLY, R. P, LANGE, E. M, MCCRORY, M. A, LANGEFELD, C. D, WILLIAMS, A, ZAKHARKIN, S. O, GEORGE, V, ALLISON, D. B, COOPER, G. S
Format: Article
Language:eng
Subjects:
Adult
African Americans - genetics
Alleles
Biological and medical sciences
C-Reactive Protein - chemistry
C-Reactive Protein - genetics
C-Reactive Protein - metabolism
Electrophoretic Mobility Shift Assay
European Continental Ancestry Group - genetics
Female
Gene Expression Regulation - genetics
Gene Frequency
General aspects
Haplotypes - genetics
Humans
Male
Medical sciences
Middle Aged
Polymorphism, Single Nucleotide
Promoter Regions, Genetic
Prospective Studies
Serum - chemistry
Transcription Factors - metabolism
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Summary:To investigate whether functional polymorphisms exist in the C-reactive protein (CRP) gene, i.e., ones that contribute directly to differences in baseline CRP among individuals, we sequenced a 1,156-nucleotide-long stretch of the CRP gene promoter in 287 ostensibly healthy people. We identified two single-nucleotide polymorphisms (SNPs), a bi-allelic one at nucleotide -409 (G-->A), and a tri-allelic one at -390 (C-->T-->A), both resident within the hexameric core of transcription factor binding E-box elements. Electrophoretic mobility shift assays confirmed that the SNP within the sequence (-412)CACGTG(-407) (E-box 1) modulates transcription factor binding, and that the one within (-394)CACTTG(-389) (E-box 2) supports transcription factor binding only when the -390 T allele is present. The commonest of four E-box 1/E-box 2 haplotypes (-409G/-390T) identified in the population supported highest promoter activity in luciferase reporter assays, and the rarest one (-409A/-390T) supported the least. Importantly, serum CRP in people with these haplotypes reproduced this rank order, i.e., people with the -409G/-390T haplotype had the highest baseline serum CRP (mean +/- SEM 10.9 +/- 2.25 microg/ml) and people with the -409A/-390T haplotype had the lowest (5.01 +/- 1.56 microg/ml). Furthermore, haplotype-associated differences in baseline CRP were not due to differences in age, sex, or race, and were still apparent in people with no history of smoking. At least two other SNPs in the CRP promoter lie within E-box elements (-198 C-->T, E-box 4, and -861 T-->C, E-box 3), indicating that not only is the quality of E-box sites in CRP a major determinant of baseline CRP level, but also that the number of E-boxes may be important. These data confirm that the CRP promoter does encode functional polymorphisms, which should be considered when baseline CRP is being used as an indicator of clinical outcome. Ultimately, development of genetic tests to screen for CRP expression variants could allow categorization of healthy people into groups at high versus low future risk of inflammatory disease.
ISSN:0946-2716
1432-1440