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GDH (Glucose Dehydrogenase) HCD5007C Featured Image
  • GDH (Glucose Dehydrogenase) HCD5007C

GDH (Glucose Dehydrogenase)


Cat No:HCD5007C

Package:5ku/100ku/1000ku/10000ku

This enzyme is useful for clinical analysis of D-glucose determination in blood glucose meter.

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Product Description

Product data

This enzyme is useful for clinical analysis of D-glucose determination in blood glucose meter.

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    • Specification

    Appearance

    Yellow amorphous powder, lyophilized

    Purity( SDS-PAGE)

    ≥90.0%

    Enzyme powder specific

    ≥400.0 U/mg

    activity

    ≤0.02%

    Glucose dehydrogenase

    ≤0.02%

    α-glucosidase

    ≤0.02%

     

    Properties

    EC number

    1.1.5.9 (Recombinant from microorganism)

    Molecular weight

    66 kDa (SDS-PAGE)

    Isoelectric point

    5.04

    Michaelis  constant

    7.45 ×10 -2 M (D-glucose) 

    Inhibitor

    Ag + , Cu 2+ , SDS

    Optimum pH

    7.0                                                                                   Fig. 1

    Optimum temperature

    50-55 °C                                                                          Fig. 2

    pH stability

    pH 5.0 – 9.0 (25 °C, 16 h)                                               Fig. 3

    Thermal stability

    Stable at 50 °C and blow (pH7.0, 30 min)                      Fig. 4

    Storage stability

    At least one year at -25~-15 ℃                                    Fig.5  

     

    Figures

    This enzyme is useful for clinical analysis of  D-glucose determination in blood glucose meter.

     

     

    Assay principle

     

    Unit definition   

    One unit (U) is defined as the amount of enzyme which generates 1 μmol of DCIP per minute at 37 °C under the conditions described below.

     

    Reagents preparation

    Reagent I: 0.1 M potassium phosphate buffer, pH 7.0.

    Reagent II: 2 M D-glucose solution.

    Reagent III: 1.8 mM DCIP solution (be prepared when using).

    Reagent IV: 30 mM PMS solution.

    Enzyme dilution buffer: 0.1 M potassium phosphate buffer pH 6.0, contains 0.1% BSA.

    Sample: The enzyme was diluted to 0.1-0.9 U/mL with enzyme dilution buffer.

     

    Procedure

    1. Add 2.05 mL reagent I, 0.6 mL reagent II and 0.15 mL reagent III to the 3 mL cuvette at 37 ℃

    2. for about 5 minutes;

    3. Add 0.1 mL reagent IV to the 3mL cuvette and mix;

    4. Add 0.1 mL enzyme solution to the 3 mL cuvette and mix; 

    5. Record the ΔAs at 600 nm in 1 minute in a spectrophotometer thermostated at 37 °C;

    6. Replace the enzyme solution with enzyme dilution buffer, and record the change of blank absorbance (∆Ab) in the same steps;

    ∆A = ∆As - ∆Ab

     

    Calculation  

     

    Vt: Total volume (3 mL);

    Vs: Enzyme volume (0.1 mL);

    1.0: Light path length (cm);

    df: Dilution factor;

    C: Enzyme concentration (mg/mL);

    20.4: Millimolar extinction coefficient of quinoneimine dye under 600 nm (cm2/μmol).

     

    References

    Satake, R. et al., J. Biosci. Bioeng., 120, 498–503 (2015).

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