Hexokinase competitive inhibitor

Figure 1. Plot of v/V ax versus the millimolar concentration of total substrate for a model enzyme displaying Michaelis-Menten kinetics with respect to its substrate MA (i.e., metal ion M complexed to otherwise inactive ligand A). The concentrations of free A and MA were calculated assuming a stability constant of 10,000 M k The Michaelis constant for MA and the inhibition constant for free A acting as a competitive inhibitor were both assumed to be 0.5 mM. The ratio v/Vmax was calculated from the Michaelis-Menten equation, taking into account the action of a competitive inhibitor (when present). The upper curve represents the case where the substrate is both A and MA. The middle curve deals with the case where MA is the substrate and where A is not inhibitory. The bottom curve describes the case where MA is the substrate and where A is inhibitory. In this example, [Mfotai = [Afotai at each concentration of A plotted on the abscissa. Note that the bottom two curves are reminiscent of allosteric enzymes, but this false cooperativity arises from changes in the fraction of total "substrate A" that has metal ion bound. For a real example of how brain hexokinase cooperatively was debunked, consult D. L. Purich H. J. Fromm (1972) Biochem. J. 130, 63.

The reaction of 5 -amino-5 -deoxyadenosine with trimetaphosphate affords the 5 -Af-triphosphate (23). When (23) is employed as substrate with glucose in the hexokinase-catalysed reaction, the 5 -AT-diphosphate (24) is obtained the latter is cleaved by snake venom phosphodiesterase to the 5 -phosphoramidate, and hydrolyses in acid to the amino-nucleoside. It does not appear to be polymerized by polynucleotide phosphorylase. In this context it is noteworthy that uridine 5 -5-thiopyrophosphate (25) is a competitive inhibitor for polynucleotide phosphorylase from E. coli, but not a substrate, and that the 5 -S-thiotriphosphates (26) and (27) show neither substrate nor inhibitory properties for RNA polymerase or DNA polymerase I, respectively. However, (23) can be polymerized using the latter enzyme, showing that the introduction of a 5 -heteroatom does not completely exclude these modified nucleotides as substrates for the polymerizing enzymes. 

Glucosamine is also phosphorylated in brain extracts, and it appears to be a competitive inhibitor of hexokinase in the phosphorylation of glucose or fructose by this tissue. The product of phosphorylation of D-glucosamine by yeast hexokinase has been isolated and identified as glucosamine-6-phosphate. This compound is converted to glucos-amine-l-phosphate in the presence of phosphoglucomatase. ... 

A series of glucose-adenosine diphosphate hybrids, in which carboxamide (88), acetylene (89) and allene (90) groups link the two moieties, has been prepared and evaluated as potential inhibitors of hexokinase. Both the carboxamide (88) and acetylene (89) derivatives were effective inhibitors of yeast hexcddnase (kj = 0.2 and 2.5 mM, respectively) and were competitive with glucose and non-competitive with ATP. 

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