Abstract
S-Adenosylmethionine (AdoMet) synthetase catalyzes the formation of AdoMet from ATP and L-methionine with subsequent hydrolysis of the bound tripolyphosphate intermediate. Maximal activity requires the presence of two divalent and one monovalent cation per active site. Recently, the x-ray structure of the Escherichia coli AdoMet synthetase was solved, and the positions of the two Mg2+ binding sites were identified. Based on additional spherical electron density, the K+ binding site was postulated to be a nearby site where the uranyl heavy atom derivative also bound in the crystal. The side chain of glutamate 42 is within ligation distance of the metals. Mutagenesis of glutamate 42 to glutamine (E42QMetK) abolished monovalent cation activation and produced an enzyme that has kinetic properties virtually identical to those of K(+)-free wild type AdoMet synthetase in both the overall AdoMet synthetase reaction and in the hydrolysis of tripolyphosphate. Thus, there is a approximately 100-fold decrease in the Vmax for AdoMet synthesis and large increases in the Km values for both substrates. In contrast there is only a 2-fold decrease in Vmax for tripolyphosphate hydrolysis. The uranyl ion, UO2(2+), is a competitive inhibitor with respect to K+ (Ki = 350 nM) and is the first ion to bind at this site and inhibit the enzyme. The UO2(2+) inhibition is reversible and tight-binding, and results from UO2(2+) and not UO2(2+)-ATP. Analogous to K+ activation, UO2(2+) predominantly inhibits AdoMet formation rather than tripolyphosphate hydrolysis. The kinetic results indicate that UO2(2+) inhibition is likely to result from interference with productive ATP binding. UO2(2+) remains a tight-binding inhibitor of the E42Q mutant, which suggests that K+ and UO2(2+) have different ligation preferences when bound in the monovalent cation binding pocket. The results support the model that glutamate 42 provides ligands to the K+ and has a major role in monovalent cation binding.
Highlights
AdoMet synthesis and large increases in the K". values for both substrates
The crystal structure of E. coli metK-encoded AdoMet synthetase isozyme has been solved at 3-A resolution by Takusagawa and co-workers.f The location of the two divalent metal ion binding sites have been identified from differences in electron density maps ofenzyme crystals grown in the presence of either Mg2+ or Co2+
The construction of the E42QMetK mutant was motivated by the observation that the U022+ binding site in the x-ray structure of AdoMet synthetase was likely to be the K+ binding site
Summary
18277-18284, 1995 Printed in U.S.A. Investigation of Monovalent Cation Activation of S-Adenosylmethionine Synthetase Using Mutagenesis and Uranyl Inhibition*. Markham§ From the Institute for Cancer Research, Fox Chase Cancer Center, Philadelphia, Pennsylvania 19111. S-Adenosylmethionine (AdoMet) synthetase catalyzes the formation of AdoMet from ATP and L-methionine with subsequent hydrolysis of the bound tripolyphosphate intermediate. § To whom correspondence should be addressed: Institute for Cancer Research, Fox Chase Cancer Center, 7701 Burholme Ave., Philadelphia, PA 19111. The crystal structure of E. coli metK-encoded AdoMet synthetase isozyme has been solved at 3-A resolution by Takusagawa and co-workers.f The location of the two divalent metal ion binding sites have been identified from differences in electron density maps ofenzyme crystals grown in the presence of either Mg2+ or Co2+.
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