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J. Biol. Chem., Vol. 263, Issue 14, 6695-6702, May, 1988
DB Mendel and E Orti
We have observed that the approximately 90-kDa non-steroid-binding
component of nonactivated glucocorticoid receptors purified from WEHI-7
mouse thymoma cells (which has been identified as the approximately 90- kDa
heat shock protein) consistently migrates as a doublet during
polyacrylamide gel electrophoresis under denaturing and reducing
conditions. It has recently been reported that murine Meth A cells contain
a tumor-specific transplantation antigen (TSTA) which is related or
identical to the approximately 90-kDa heat shock protein (Ullrich, S.J.,
Robinson, E.A., Law, L.W., Willingham, M., and Appella, E. (1986) Proc.
Natl. Acad. Sci. U.S.A. 83, 3121-3125). The observation that TSTA and the
approximately 90-kDa heat shock protein isolated from these cells exists as
two isoforms of similar molecular mass and charge has suggested to us that
the doublet we observed is also due to the existence of two isoforms.
However, unlike TSTA, which appears to contain the two isoforms in similar
relative abundance, nonactivated glucocorticoid-receptor complexes seem to
contain predominantly the lower molecular mass isoform. We have therefore
conducted this study to determine whether TSTA and the approximately 90-kDa
component of glucocorticoid receptors are indeed related, to establish
whether the receptor preferentially binds one isoform of the approximately
90-kDa heat shock protein, and to investigate the stoichiometry of the
nonactivated receptor complex. By comparing Meth A TSTA and the
approximately 90-kDa component of the receptor in their reactions with the
AC88 monoclonal antibody (specific for the approximately 90-kDa heat shock
protein) and a polyclonal antibody directed against Meth A TSTA, we found
that these two proteins are indistinguishable and probably identical. We
then used the BuGR1 (directed against the steroid-binding subunit of
glucocorticoid receptors) and AC88 monoclonal antibodies to purify,
respectively, receptor-associated and free approximately 90-kDa heat shock
protein from WEHI-7 cells grown for 48 h with [35S]methionine to
metabolically label proteins to steady state. Following analysis of the
proteins by polyacrylamide gel electrophoresis under denaturing and
reducing conditions, the relative amounts of the two isoforms in each
sample were determined from the 35S counts and the known methionine content
of each isoform. We found that approximately three-quarters of both the
receptor-associated and the free approximately 90-kDa heat shock protein is
present as the lower molecular weight isoform, indicating no preferential
binding of either isoform in the receptor. The long-term metabolic labeling
approach has also enabled us to direc
Isoform composition and stoichiometry of the approximately 90-kDa heat shock protein associated with glucocorticoid receptors
Department of Physiology, Dartmouth Medical School, Hanover, New Hampshire 03756.
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