Me. Black et De. Hruby, SITE-DIRECTED MUTAGENESIS OF A CONSERVED DOMAIN IN VACCINIA VIRUS THYMIDINE KINASE - EVIDENCE FOR A POTENTIAL ROLE IN MAGNESIUM BINDING, The Journal of biological chemistry, 267(10), 1992, pp. 6801-6806
Alignment of prokaryotic and vertebrate type II thymidine kinases (TK)
(EC 2.7.1.21), such as that encoded by vaccinia virus (VVTK), reveals
three conserved regions: designated domains I, III, and VII. Domains
I and III of VVTK contain residues which closely resemble segments A (
ATP) and B (Mg2+), respectively, of a Mg.ATP binding descriptor propos
ed previously (Walker, J.E., Saraster, M., Runswick, M-J., and Gay, N.
J. (1982) EMBO J. 1, 945-951). In support of this hypothesis, domain
I of the VVTK enzyme has previously been identified as the ATP binding
site (Black and Hruby, 1990b). With regard to Mg2+ binding, several f
eatures of the VVTK domain III suggest that it may be responsible for
this activity: 1) sequence similarity to a magnesium binding motif pro
posed previously (Walker, J. E., Saraster, M., Runswick, M-J., and Gay
, N. J. (1982) EMBO J. 1, 945-951);2) alignment of the predicted secon
dary structure of type II TK enzymes with other magnesium-binding enzy
mes such as adenylate kinase, EF-TU, and p21 reveals a conserved aspar
tic acid residue preceded by several hydrophobic residues within domai
n III; and 3) the conserved VVTK domain III aspartic acid residue (D82
) aligns with D93 residue of adenylate kinase which is has been shown
by NMR to participate in Mg2+ binding (Yan, H., and Tsai, M.-D., Bioch
emistry, in press). To directly examine the potential contribution of
the conserved domain III D82 residue of VVTK in magnesium binding, sit
e-directed mutagenesis was performed on positions D82 and G84 to gener
ate four mutants, N82, L82, I82, and V84. Each mutant was analyzed for
enzyme activity, divalent cation requirements, tetramer formation, an
d ATP binding ability. The results obtained were consistent with D82 p
laying a direct role in Mg2+ binding and suggest that while the aspart
ic acid does not appear to participate directly with ATP binding it ma
y instead act to facilitate ATP hydrolysis by binding Mg2+ which aids
to correctly position ATP for nucleophilic attack.