Journal of Biological Chemistry 1983-08-25

Subunit associations of (Na+ + K+)-dependent adenosine triphosphatase. Chemical cross-linking studies.

S M Periyasamy, W H Huang, A Askari

Index: J. Biol. Chem. 258(16) , 9878-85, (1983)

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Abstract

Cross-linking reactions of the alpha- and beta-subunits of the purified membrane-bound enzyme with several reagents were studied. In the presence of 1,5-difluoro-2,4-dinitrobenzene, formation of a cross-linked alpha, beta-dimer was affected specifically by K+ + ATP or enzyme phosphorylation. The same conditions affected the formation of cross-linked alpha, alpha-dimer in the presence of 4,4'-difluoro-3,3'-dinitrodiphenyl sulfone or o-phenanthroline-Cu2+. Since noncovalent alpha, beta-association has been established, the data suggest K+ + ATP-induced or phosphorylation-induced changes in alpha, beta-domain and alpha, alpha-domain of an oligomer of alpha, beta-dimer. When the formation of cross-linked alpha, beta-dimer or alpha, alpha-dimer was induced by phosphorylation, only half of the subunits were cross-linked, suggesting the existence of a cooperative tetramer of alpha, beta-dimer. When microsomes or red cell membranes were exposed to 32Pi under phosphorylation-induced cross-linking conditions, the only products were alpha, beta-dimer and alpha, alpha-dimer, indicating the existence of an oligomer of alpha, beta-dimer in crude membranes. Subunits of the enzyme solubilized with octaethylene glycol dodecyl ether, by methods that have been suggested to yield unassociated alpha, beta-dimers, underwent spontaneous cross-linking that was not affected by enzyme dilution. Since the largest product was alpha 2 beta 2, the solubilized enzyme is at least a dimer of alpha, beta-dimer. The findings establish that the membrane-bound enzyme is an oligomer of alpha, beta-dimer. Whether or not a single alpha, beta-dimer is capable of catalytic and transport functions has not been determined.

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