Differences in the form of the salt-transformed estrogen receptor when bound by estrogen versus antiestrogen

Differences in the form of the salt-transformed estrogen receptor when bound by estrogen versus antiestrogen

Our laboratory has previously reported that antiestrogen binding to molybdate-stabilized non-transformed estrogen receptor results in a larger form of the receptor in 0.3 M KCl when compared with estrogen bound receptor. Estradiol promoted the formation of monomers in the presence of 0.3 M KC1 where...

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Veröffentlicht in:Journal of steroid biochemistry 1990-08, Vol.36 (6), p.509-516
Hauptverfasser: Ruh, Mary F., Turner, Jane W., Paulson, Christine M., Ruh, Thomas S.
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Antibodies - analysis
Centrifugation, Density Gradient
Chromatography, DEAE-Cellulose
Chromatography, Gel
Estradiol - pharmacology
Estrogen Antagonists - pharmacology
Female
Potassium Chloride - pharmacology
Protein Conformation
Rabbits
Receptors, Drug
Receptors, Estrogen - chemistry
Receptors, Estrogen - drug effects
Receptors, Estrogen - immunology
Uterus - chemistry
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Zusammenfassung:Our laboratory has previously reported that antiestrogen binding to molybdate-stabilized non-transformed estrogen receptor results in a larger form of the receptor in 0.3 M KCl when compared with estrogen bound receptor. Estradiol promoted the formation of monomers in the presence of 0.3 M KC1 whereas antiestrogen appeared to promote dimer formation. We have extended these studies examining the rabbit uterine salt-transformed estrogen receptor partially purified by DEAE-cellulose chromatography. We previously demonstrated that estrogen receptor prepared in this way bound to different sites on partially deproteinized chromatin subfractions or reconstituted chromosomal protein/DNA fractions when the receptor was complexed with estrogen vs antiestrogen. Analysis of these receptor preparations indicated that DEAE-cellulose step-elution resulted in a peak fraction which sedimented as a single 5.9S peak in 5–20% sucrose density gradients containing 0.3 M KCl for receptor bound by the antiestrogens H1285 and trans-hydroxytamoxifen. However, receptor bound by estradiol sedimented as 4.5S. These receptor complexes bound DNA-cellulose indicating that these partially purified receptors were transformed. DEAE rechromatography or agarose gel filtration of the partially purified antiestrogen-receptor complexes resulted in significant dissociation of the larger complex into monomers. Incubations of 5.9S antiestrogen-receptor complexes with antibodies against nontransformed steroid receptor-associated proteins (the 59 and 90 kDa proteins) did not result in the interaction of this larger antiestrogen-receptor complex with these antibodies (obtained from L.E. Faber and D.O. Toft, respectively). Our results support the concept that antiestrogen binding induces a different receptor conformation which could affect monomer-dimer equilibrium, thus rendering the antiestrogen-receptor complex incapable of inducing complete estrogenic responses in target tissues.
ISSN:0022-4731
DOI:10.1016/0022-4731(90)90166-P