The correlation between ouabain binding and potassium pump inhibition in human and sheep erythrocytes
1. [3H]Ouabain binding to human and sheep red blood cells was shown to be specific for receptors associated with Na/K transport. Virtually all tritium binding was abolished by dilution with unlabelled drug. Saturation levels of binding were independent of glycoside concentration and were identical t...
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Veröffentlicht in: | The Journal of physiology 1978-10, Vol.283 (1), p.155-175 |
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Sprache: | eng |
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Zusammenfassung: | 1. [3H]Ouabain binding to human and sheep red blood cells was shown to be specific for receptors associated with Na/K transport.
Virtually all tritium binding was abolished by dilution with unlabelled drug. Saturation levels of binding were independent
of glycoside concentration and were identical to those associated with 100% inhibition of K pumping. 2. [3H]Ouabain binding
and 42K influx were measured simultaneously in order to correlate the degree of K pump inhibition with the amount of glycoside
bound. Results by this method agreed exactly with those obtained by pre-exposing cells to drug, followed by washing and then
measuring K influx. 3. Plots of [3H]oubain binding vs. K pump inhibition were rectilinear for human and low K (LK) sheep red
cells, indicating one glycoside receptor per K pump site and functional homogeneity of pump sites. High K (HK) sheep red cells
exhibited curved plots of binding versus inhibition, which were best explained in terms of one receptor per pump, but a heterogeneous
population of pump sites. 4. External K reduced the rate of glycoside binding, but did not alter the relationship between
binding and inhibition. 5. The number of K pump sites was estimated as 450--500 per human cell and 30--50 per LK sheep cell.
HK sheep cells had 90--130 sites per cell, of which eighty to ninety were functionally dominant. The number of K pump sites
on LK sheep cells was not changed by anti-L, although the maximum velocity of pump turnover was increased. |
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ISSN: | 0022-3751 1469-7793 |
DOI: | 10.1113/jphysiol.1978.sp012494 |