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Volume 272, Number 48,
Issue of November 28, 1997
pp. 30387-30399
©1997 by The American Society for Biochemistry and Molecular Biology, Inc.
Characterization of Multiple Enhancer Regions Upstream of the
Apolipoprotein(a) Gene
(Received for publication, June 3, 1997, and in revised form, August 2, 1997)
David P.
Wade
,
Loretto H.
Puckey
,
Brian L.
Knight
,
Francesco
Acquati
§
,
Alessandra
Mihalich
§
and
Roberto
Taramelli
¶
From the Medical Research Council Lipoprotein Team, Clinical
Sciences Centre, Hammersmith Hospital, London W12 0NN, United
Kingdom, § Istituto Scientifico San Raffaele, 20132 Milan,
Italy, and the ¶ Dipartimento di Biologia Animale, Universita
degli Studi di Catania, 95124 Catania, Italy
Plasma concentrations of the atherogenic
lipoprotein(a) (Lp(a)) are predominantly determined by inherited
sequences within or closely linked to the apolipoprotein(a) gene locus.
Much of the interindividual variability in Lp(a) levels is likely to
originate at the level of apo(a) gene transcription. However, the
liver-specific apo(a) basal promoter is extremely weak and does not
exhibit common functional variations that affect plasma Lp(a)
concentrations. In a search for additional apo(a) gene control
elements, we have identified two fragments with enhancer activity
within the 40-kilobase pair apo(a)-plasminogen intergenic region that
coincide with DNase I-hypersensitive sites (DHII and DHIII) observed in
liver chromatin of mice expressing a human apo(a) transgene. Neither
enhancer exhibits tissue specificity. DHIII activity was mapped to a
600-base pair fragment containing nine DNase I-protected elements
(footprints) that stimulates luciferase expression from the apo(a)
promoter 10-15-fold in HepG2 cells. Binding of the ubiquitous
transcription factor Sp1 plays a major role in the function of this
enhancer, but no single site was indispensable for activity. DHIII
comprises part of the regulatory region of an inactive long
interspersed nucleotide element 1 retrotransposon, raising the
possibility that retrotransposon insertion can influence the regulation
of adjacent genes. DHII enhancer activity was localized to a 180-base pair fragment that stimulates transcription from the apo(a) promoter 4-8-fold in HepG2 cells. Mutations within an Sp1 site or either of two
elements composed of direct repeats of the nuclear hormone receptor
half-site AGGTCA in this sequence completely abolished enhancer
function. Both nuclear hormone receptor elements were shown to bind
peroxisome proliferator-activated receptors and other members of
the nuclear receptor family, suggesting that this enhancer may mediate
drug and hormone responsiveness.

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Copyright © 1997 by the American Society for Biochemistry and Molecular Biology.
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