Glycerol Kinase Assay

Method

The reaction velocity is measured in a coupled system with pyruvate kinase and lactate dehydrogenase. One unit results in the oxidation of one micromole of NADH per minute at 25°C and pH 8.9 under the specified conditions.

Reagents

Reagent solution: the required amount of solution should be prepared containing:

ATP 8.5 mM

NADH 1.22 mM

PEP 2.0 mM

Lactate Dehydrogenase
(Worthington code: LADCL) 15.3 u/ml

Pyruvate kinase
(Worthington code: PKL) 7.0 u/ml

MgSO₄⋅7H₂O 28.0 mM

Reduced Glutathione 26.0 mM

pH adjusted to 7.4

0.4 M Glycine, pH 8.9 containing 45 mM potassium carbonate
0.1 M Triethanolamine⋅HCl buffer, pH 7.4
0.1 M Glycerol

Enzyme

Dissolve at a concentration of one mg/ml in 0.1 M TEA buffer, pH 7.4. Immediately prior to use, dilute further in TEA buffer to obtain a rate of 0.02 - 0.04 ΔA/min.

Procedure

Adjust spectrophotometer to 340 nm and 25°C.

Pipette into cuvettes as follows:

Carbonate-glycine buffer 2.1 ml

Reagent solution 0.7 ml

0.1 M Glycerol 0.1 ml

Incubate in spectrophotometer for 3 - 4 minutes to achieve temperature equilibration and establish blank rate, if any.

Add 0.1 ml of appropriately diluted enzyme and record ΔA₃₄₀ for 6 - 8 minutes. Determine ΔA₃₄₀/min from the linear portion of the curve. A short lag period may be observed.

Calculation

\frac{\text{Units}}{\text{mg}}\text{ = } \frac{\frac{\Delta \text{A}_{340}}{\text{min}}}{\text{6.22 x }\frac{\text{mg enzyme}}{\text{ml reaction mixture}}}

ATP	8.5 mM
NADH	1.22 mM
PEP	2.0 mM
Lactate Dehydrogenase (Worthington code: LADCL)	15.3 u/ml
Pyruvate kinase (Worthington code: PKL)	7.0 u/ml
MgSO₄⋅7H₂O	28.0 mM
Reduced Glutathione	26.0 mM
pH adjusted to	7.4

Carbonate-glycine buffer	2.1 ml
Reagent solution	0.7 ml
0.1 M Glycerol	0.1 ml

Please enter catalog number and quantity

Glycerol Kinase - Assay

Glycerol Kinase Assay