Endogenous digitalis-like factors: In vitro comparison of biological and immunological activities of peptide and steroid candidates
Endogenous substances that modulate the activity of (Na + + K +)-ATPase through interaction at the cardiac glycoside site have been postulated. Reports of digitalis-like biological and immunological activity exhibited by certain ACTH/MSH peptides and 14-OH steroids make these compounds potential can...
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Veröffentlicht in: | European journal of pharmacology 1984-11, Vol.106 (3), p.567-575 |
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Sprache: | eng |
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Zusammenfassung: | Endogenous substances that modulate the activity of (Na
+ + K
+)-ATPase through interaction at the cardiac glycoside site have been postulated. Reports of digitalis-like biological and immunological activity exhibited by certain ACTH/MSH peptides and 14-OH steroids make these compounds potential candidates as endogenous digitalis-like factors. We tested several ACTH/MSH peptides and 14α-OH steroids in four in vitro assays and detected no significant cardiac glycoside-like activity. On the other hand, chlormadinone acetate, a progesterone derivative shown to bind with high affinity to the digitalis receptor, was nearly equipotent to digoxigenin in a [
3H]ouabain radioreceptor assay. In a [
3H]digoxin radioimmunoassay, however, digoxigenin and digoxin were equipotent but chlormadinone acetate was inactive. A clear dissociation between radioreceptor assay and radioimmunoassay activity was also observed using 15 β-OH-progesterone. Our findings indicate that (a) ACTH/MSH peptides and 14α-OH steroids are not viable candidates as endogenous digitalis-like factors, (b) digoxin antibodies are not necessarily directed at molecular determinants critical for biological activity, and (c) among the compounds reported to exhibit digitalis-like activity and postulated to share structural features with an endogenous steroidal digitalis-like factor, only chlormadinone acetate and its congeners appear to constitute tenable models. |
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ISSN: | 0014-2999 1879-0712 |
DOI: | 10.1016/0014-2999(84)90060-8 |