Assay Procedure for Invertase
Principle
The appearance of reducing sugars is measured by the modified Fehling-Lehmann-Schoorl method.7)
Unit definition
One unit causes the formation of one milligram of reducing sugars equivalent to the glucose at 3 minutes under the conditions described below (This activity is equivalent to the international unit that hydrolyzes one micromole of saccharose per minute at the same temperature).
Method
Reagents
Procedure
- Pipette 1.0 mL of substrate solution (A) into a test tube and equilibrate at 20 ℃ for about 5 minutes.
- Add 1.0mL of the enzyme solution (pre-incubated at 20 ℃) and mix.
- After exactly 3 minutes at 20 ℃, add 2.0mL of alkaline solution (B) to stop the reaction. At the same time, prepare the blank by first mixing the substrate solution with 2.0mL of alkaline solution after a 3 min-incubation at 20 ℃, followed by the addition of the enzyme solution and carry out the same procedure as the test (Procedure 4-8).
- Transfer the stopped reaction mixture from the test tube to a 100mL volume of Erlenmeyer flask. Rinse the inside of the test tube with about 3mL of distilled water and transfer the rinsings to the flask. Repeat this procedure three times.
- Add 2.0mL of CuSO4 Solution (C) and place the flask directly on a electrothermic heater (1.2 KWH) in the presence of a glass bead (5mmφ) to prevent bumping.
- Keep for exactly 2 minutes in a boiling state and cool down to room temperature under running water.
- Add 2.0mL each of KI solution (D) and H2SO4 solution (E) in this order.
- Shake the flask and determine the amount of residual Cu++ by titration with Na2S2O3 solution (F) in the presence of a few drops of soluble starch (G) as an indicator.
- Record the titers (mL) of the test (t) and the blank (b), and calculate the titration difference (Δtiter, mL).
* Dissolve the enzyme preparation in ice-cold distilled water and dilute to 2.0-9.0 U/mL with the enzyme dilute (H), immediately before assay.
Calculation
Activity can be calculated by using the following formula:
Weight activity (U/mg)=(U/mL)×1/C
This procedure is for informational purposes. For a current copy of our quality control procedure, please contact our Technical Service Department.
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