Binding of Rb86 by a microsomal fraction of bovine cerebral cortex cells]

The maximal binding of 86Rb was noted when ions of Mg, ATP and Na were present simultaneously. The availability of olytoriside (1-10(-4)M), CaCl2 (1-10(-3)M) and phospholipase A (1-10(-5)M) in the medium and the removal of Na and substitution of ATP for ADP decreased to a different extent the binding of 86Rb.     

Effect of small doses of gamma radiation on the activity of marker enzymes in the plasma membranes of chick embryo liver

A study was made of marker enzyme activity in plasma membranes of chick liver during embryogenesis in normal conditions and after exposure to ionizing radiation. It was shown that irradiation with small doses of eggs prior to incubation and of chick embryos during different periods of the prenatal ontogenesis caused essential changes in activity of membrane-bound enzymes of liver plasmolemma. Stimulation with small radiation doses was most effective with preincubation irradiation of eggs and most manifest at later stages of the prenatal ontogenesis. Thus, the marker enzymes were shown to play a significant role in the realization of the stimulatory effect of low-level radiation.     

Effect of transformed steroids on Na,K-dependent ATPase

The transformed steroids containing delta 5-3 beta-hydroxy- or 3 beta, 5 alpha-dihydroxy-6-keto groups in the A/B rings and an additional cycle E (17,20-dihydroxy-delta-lactone, 16,23-pyranone or delta 20(22)-16 alpha, 17 alpha-dihydroxy-23-carbethoxy-side chain) (1 . 10(-5) M) inhibit Na+,K+-ATPase from pig kidney medulla or from ox brain. The steroid structure has a noticeable effect on ATPase inhibition varying from 3 to 26%. The data obtained suggest that the uneven distribution of polar substituents in the steroid molecule is essential for ATPase inhibition by steroid aglycons.     

Ion-transporting properties and ATPase activity of (Na+ + K+)-ATPase large subunit incorporated into bilayer lipid membranes

A purified (Na+ + K+)-ATPase large subunit obtained from microsomes by water-alcohol extraction was incorporated into a bilayer lipid membrane. The protein formed in the membrane conductance channels which were sensitive to ouabain and selective for monovalent cations. ATP activated these channels in the presence of sodium and potassium ions. When sodium ions were eliminated ATP did not change the conductance of the modified membrane whereas p-nitrophenyl phosphate increased it. The (Na+ + K+)-ATPase large subunit incorporated into bilayer lipid membrane possessed an ATPase activity. The presence of a potential on the membrane was a necessary condition for the enzyme incorporated into a bilayer lipid membrane to show high ATPase activity. Increasing the potential above 100 mV resulted in the closing of conductance channels.     

Interaction of Na,K-ATPase with modifying ATP analogs and chloromethylphosphonic acid

The interaction of synthetic ATP analogs, containing active groups in the triphosphate moiety and in the 8-position of the nucleotide molecule, with highly purified Na, K-ATPase from the medullar layer of porcine kidney was studied. It was found that 11 out of 17 ATP analogs studied irreversibly inhibit the ATPase activity of the enzyme. The pH optimum of the enzyme inactivation by adenosine-5'-(beta-chloroethylphosphate) and adenosine-5'-(p-fluorosulfonylphenylphosphate) beside the pronounced protective effect of ATP suggests possible covalent blocking of histidine and dicarboxylic amino acid residues in the enzyme active center. The irreversible inhibition of the enzyme by "oxo-ATP" containing aldehyde groups in the modified ribose residue in the presence of sodium borohydride suggests a possible presence of the lysine residue epsilon-amino group in the ATP binding site of the enzyme. Na, K-ATPase was found to possess an inorganic phosphate binding site, which is specifically blocked by chloromethylphosphonic acid. the accessibility of this site for modification depends on ATP, NA+ and K+.     

Molecular polarity dependence of the transformed steroid effect on Na,K-ATPase

The transformed steroids containing an additional cycle E (delta-lactone or 16.23-pyranone) or 23-carbethoxy side chain (1.10(-5) M) inhibit Na,K-ATPase from pig kidney medulla. The steroid structure has a noticeable effect on ATPase inhibiton varying from 9 to 35%. The data obtained suggest that the position, stereochemistry and the uneven distribution of polar substituents in the steroid molecule are essential for ATPase inhibition by steroid aglycons.     

The effect of the distribution of polar groups in a steroid molecule on its inhibition of Na+,K+-ATPase

Transformed steroids having oxidized side chains in the D ring site and varying by polarity of the substituent at the ring A C(3)-position--acetates, glucosides or with free hydroxyls--in the concentration range 1 X 10(-4) - 1 X 10(-7) M were found to inhibit Na+, K+-ATPase. The extent of inhibition decreases with the rise in the polarity of the A region of the steroid molecule. With the compound devoid of polar groups in the D region an increase in the inhibitory activity is observed on passing from 3-acetate to 3-glucoside. The data obtained confirm the relationship between the extent of Na+, K+-ATPase inhibition and biphilicity of the molecule.     

Stabilization of Na+, K+-adenosine triphosphatase by dimethyl sulfoxide under inactivation by urea]

Hydrophobic agents, e.g. methanol, ethanol, isopropanol, acetone and dioxane were shown to induce irreversible inactivation of Na+, K+-adenosine triphosphatase beginning with their concentrations of 20 to 35%, whereas dimethyl sulphoxide exerted similar effect only at concentration of 50% and higher. Urea also irreversibly inactivated Na+, K+-adenosine triphosphatase, beginning with a concentration of about 20%. It was found that, dimethyl sulphoxide contrary to the other hydrophobic agents studied, protected Na+, K+-adenosine triphosphatase against the inactivating (denaturing) action of urea. The highest stabilizing effect of dimethyl sulphoxide was displayed at concentrations from 20 to 30%.