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(Received for publication, April 30, 1995; and in revised form, June 21, 1995) Glucocorticoid induction of the tyrosine aminotransferase gene
deviates from that of many glucocorticoid-responsive genes by having a
lower EC
Volume 270,
Number 37,
Issue of September 15, pp. 21893-21901, 1995
©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
and displaying more agonist activity with a given
antiglucocorticoid. A cis-acting element, located 3646 base
pairs upstream of the start of tyrosine aminotransferase gene
transcription, has been found to be sufficient to reproduce these
variations with heterologous genes and promoters (Oshima, H., and
Simons, S. S., Jr.(1992) Mol. Endocrinol. 6, 416-428).
This element has been called a glucocorticoid modulatory element, or
GME. Others have called this sequence a cyclic AMP-responsive element
(CRE) due to the binding of the cyclic AMP response element binding
protein (CREB). We now report the partial purification and
characterization of two new proteins (GMEB1 and -2) of 88 and 67 kDa
that bind to the GME/CRE as a heteromeric complex. This purification
was followed by the formation of a previously characterized,
biologically relevant band in gel shift assays. By several biochemical
criteria, the GMEBs differed from many of the previously described
CREB/CREM/ATF family members. Partial peptide sequencing revealed that
the sequences of these two proteins have not yet been described. Size
exclusion chromatography and molecular weight measurements of the
gel-shifted band demonstrated that the GMEBs bound to the GME as a
macromolecular complex of about 550 kDa that could be dissociated by
deoxycholate. Similar experiments showed that CREB bound to the GME as
heteromeric complexes of about 310 and 360 kDa. As determined from gel
shift assays, GMEB1 and -2 are not restricted to rat liver cells but
appear to be ubiquitous. Thus, these novel GMEBs may participate in a
similar modulation of other glucocorticoid-inducible genes in a variety
of cells.
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