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Volume 272, Number 48,
Issue of November 28, 1997
pp. 30583-30588
©1997 by The American Society for Biochemistry and Molecular Biology, Inc.
Identification of a Placental Enhancer for the Human Leptin
Gene
(Received for publication, April 25, 1997, and in revised form, July 30, 1997)
Sheng
Bi
,
Oksana
Gavrilova
,
Da-Wei
Gong
,
Mark M.
Mason
and
Marc
Reitman
From the Diabetes Branch, NIDDK, National Institutes of Health,
Bethesda, Maryland 20892-1770
Leptin is a hormone that regulates metabolic
efficiency, energy expenditure, and food intake. Leptin is produced
chiefly in adipose cells, but in humans, mRNA encoding leptin is
also present in the placenta. Here we elucidate the basis for placental
leptin production. The same promoter is used for adipose and placental transcription. An upstream enhancer functions in the JEG-3 and JAR
choriocarcinoma cell lines but not in adipocytes or HeLa cells. The
minimal positive acting region is 60 base pairs in length. This region
is within a MER11 repetitive element, suggesting that human placental
expression of leptin is the result of insertion of this element.
Binding analyses demonstrated three protein binding sites, designated
placental leptin enhancer elements (PLE)1, PLE2, and PLE3. PLE2 binds
Sp1. Enhancer activity was reduced by mutation of the PLE1 or PLE3
sites but was unaffected by alteration of PLE2. Proteins binding to
PLE3 were present in JEG-3 and human placental nuclear extracts but not
in extracts from non-placental sources. Upon triplication, the PLE3
element was a strong enhancer in choriocarcinoma cells but not in HeLa
cells. The protein binding to the PLE3 motif appears to be a novel,
placenta-specific transcription factor.

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