Ordered sequential mechanism of substrate recognition and binding by KB cell DNA polymerase .alpha.
- 1 August 1981
- journal article
- research article
- Published by American Chemical Society (ACS) in Biochemistry
- Vol. 20 (16), 4560-4569
- https://doi.org/10.1021/bi00519a008
Abstract
A steady-state kinetic approach was used in conjunction with direct velocity gradient sedimentation binding studies to examine the detailed steps involved in the recognition of DNA primer-template and dNTP [deoxy-nucleoside triphosphates] by nearhomogeneous human DNA polymerase .alpha.. The interaction of the polymerase with its substrates obeys a rigidly ordered sequential terreactant mechanism, with template as the 1st substrate, followed by primer as the 2nd substrate and dNTP as the 3rd. Although the binding of primer is prerequisite to the kinetically significant binding of dNTP, specification of which of the 4 dNTP can then add to the enzyme is absolutely determined by the base sequence of the template (the 1st substrate). The critical element in the proof of the ordered mechanism is the demonstration of the phenomenon of induced substrate inhibition; the presence of a dideoxy-terminated primer (dead-end inhibitor) induces substrate inhibition by dNTP which is absolutely restricted to the dNTP complementary to the template to which the blocked primer is annealed. This inhibition is kinetically competitive with 3''-hydroxyl-terminated (unblocked) primer and approaches 100% at saturating levels of the complementary dNTP. Direct binding studies document the specific and exclusive ability of complementary dNTP to drive the polymerase into a stable dead-end complex with the proposed structure, enzyme-template-dideoxy primer-dNTP, corroborating the kinetic observations. Attempts to elucidate the order of product release from the enzyme by product inhibition studies have shown the polymerization reaction to be essentially irreversible and have been unsuccessful. Based on the known processivity of KB [human male oral epidermoid carcinoma] cell DNA polymerase .alpha., a preliminary model involving initial release of pyrophosphate is reasonable; the relationship between product release and the process of polymerase translocation remains obscure. All kinetic and sedimentation binding studies were performed on a variety of homopolymeric and natural heteropolymeric DNA substrates, and the consistency of the results establishes absolutely the qualitative identity of the general mechanism by which human DNA polymerase .alpha. recognizes and replicates polydeoxynucleotide primer-templates, regardless of their precise physicochemical nature.This publication has 7 references indexed in Scilit:
- Enzymological characterization of KB cell DNA polymerase-alpha. Regulation of template binding by nucleic acid base composition.Journal of Biological Chemistry, 1981
- The energy relay: a proofreading scheme based on dynamic cooperativity and lacking all characteristic symptoms of kinetic proofreading in DNA replication and protein synthesis.Proceedings of the National Academy of Sciences, 1980
- Interactions between DNA-bound repressors govern regulation by the λ phage repressorProceedings of the National Academy of Sciences, 1979
- Enzymological characterization of DNA polymerase alpha. Basic catalytic properties processivity, and gap utilization of the homogeneous enzyme from human KB cells.Journal of Biological Chemistry, 1979
- Steady-state kinetics of mouse DNA polymerase .beta.Biochemistry, 1979
- Enzymatic determinants of DNA polymerase accuracy. Theory of coliphage T4 polymerase mechanismsJournal of Molecular Biology, 1978
- DNA polymerase-alpha. Purification and structural characterization of the near homogeneous enzyme from human KB cells.Journal of Biological Chemistry, 1977