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Abstract
HLA-G is a non-classic class I MHC molecule specifically expressed by
human invasive cytotrophoblast cells, which has been suggested to play
a role in facilitating the immune tolerance of the conceptus. So far,
very little is known about the regulation of the human HLA-G gene. The
present study was, thus, designed to investigate the regulation of the
human HLA-G promoter. JEG3 choriocarcinoma cells, which express HLA-G
endogenously, were used as a model. A 890 bp fragment of the human
HLA-G promoter was amplified by nested PCR from genomic DNA, cloned
into pCR-Script and, after sequencing, subcloned into pGL3-Luc in front
of the luciferase reporter gene. This vector was then used in transient
transfection experiments in JEG3 cells. Parallel transfection
experiments were performed using an
subunit (
SU)-Luc reporter
plasmid as a control. Using this system, several potential modulating
substances were tested in different concentrations and for different
periods of time: phorbol ester (TPA), cAMP, IFN
, IL-1, and leukemia
inhibitory factor (LIF), with only LIF administration resulting in
induction of the HLA-G promoter. LIF treatment also resulted in
induction of HLA-G mRNA. JEG3 cells are shown to possess LIF receptors.
LIF is a pleiotropic cytokine produced at the maternal-fetal interface
which has been shown to play an essential role in implantation in mice.
LIF is produced in high amounts by the human endometrium and the
trophoblast itself, and LIF receptors are present on cytotrophoblast
cells. LIF could, thus, play a role in modulating HLA-G production and
immune tolerance at the maternal-fetal interface.
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