Abstract
Casein kinase II, purified from reticulocytes, was covalently labeled with the ATP affinity analog, 5'-p-fluorosulfonylbenzoyl adenosine. The reaction was monitored by the decrease in enzyme activity and showed saturation kinetics with respect to the sulfonyl compound. This suggested a rapid equilibrium was established between the enzyme and affinity reagent prior to a slower, rate-determining step in the overall inactivation process. The enzyme was protected from the covalent modification by ATP and a series of ATP analogs. Their effectiveness in preventing inactivation by the affinity labeling reagent paralleled their ability to function as inhibitors of the phosphotransferase reaction. When radioactive p-fluorosulfonyl [14C]benzoyl adenosine was used to inactivate the enzyme, the alpha subunit was labeled and incorporation of radioactivity into the alpha subunit was blocked when ADP was included in the reaction mixture. Thus the ATP binding site of casein kinase II was shown to be contained within the domain of the alpha subunit of the alpha 2 beta 2 complex.
Highlights
The ATPaffiiity label, 5’-p-fluorosulfonylbenzoyaldenosine, covalently labeled with the ATP affinity analog, S‘-p- has been shownto inactivate several protein kinases including fluorosulfonylbenzoyal denosine
Reaction of Casein Kinase 11 with 5'-p-FSOzBzAdo-The addition of 5'-p-FSOzBzAdo to casein kinase I1 resulted in a loss of enzymaticactivity as showninFig. 1
Casein Kinase Z I by 5'-p-FSOzRzAdo-The effectiveness of ATP analogs to function as inhibitors of the casein kinase phosphotransferase reaction was investigated by examining each nucleotide at a final concentration of 1.0 mM in the standard assay and comparing it with the ability of ATP to compete with itself
Summary
MM Tris-HC1, 10mM potassium phosphate buffer, pH 7.3, and 0.2 M KCl. The reagent, 5”p-FSOZBzAdo in Me2S0 was added so that a final concentration of 10% MezSO was obtained in the incubation mixture. Bands corresponding to the a and P subunits of casein kinase I1 as well as areas containing no protein (for background determination) were excised and placed in 0.9 ml of 3 M P-mercaptoethanol. 1 4 reaction containing 25 mM Tris-HC1, 10 m~ potassium phosphate, pH 7.3, 10 m~ MgCI2,and 0.2 M KC1 at 30 "C.A, time course of casein kinase I1 inactivation; enzyme which received only M e 8 0 to 10%final concentration (0)e;nzymewhich received 1.6mM 5'-p-FSOeBzAdoin Me2SO (0)B;, determination of k o fr~om the dataof A ;E and EOrepresent the activity at time (t) and zero time, respectively The enzyme (2500 enzyme units) was incubated in a 0 . 1 4 reaction containing 25 mM Tris-HC1, 10 m~ potassium phosphate, pH 7.3, 10 m~ MgCI2,and 0.2 M KC1 at 30 "C.A, time course of casein kinase I1 inactivation; enzyme which received only M e 8 0 to 10%final concentration (0)e;nzymewhich received 1.6mM 5'-p-FSOeBzAdoin Me2SO (0)B;, determination of k o fr~om the dataof A ;E and EOrepresent the activity at time (t) and zero time, respectively
Sign-in/Register to view highlights & summary Sign-in/Register to access full text options 
Free) 
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call
