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Glucose (Glu) Colorimetric Assay Kit (GOD-POD Method)– MSE Supplies LLC

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Glucose (Glu) Colorimetric Assay Kit (GOD-POD Method)

SKU: E-BC-K234-M-500

  • $ 34095
  • Save $ 6000


Glucose (Glu) Colorimetric Assay Kit (GOD-POD Method)

SKU # E-BC-K234-M
Detection Instrument Microplate reader (500-510 nm)
Detection method Colorimetric method


Product Details

Properties

Synonyms Glu
Sample Type Serum, plasma, whole blood
Sensitivity 0.04 mmol/L
Detection Range 0.04-30 mmol/L
Detection Method Colorimetric method
Assay type Quantitative
Assay time 30 min
Precision Average inter-assay CV: 2.300% | Average intra-assay CV: 1.900%
Other instruments required Vortex mixer, Micropipettor, Incubator
Other reagents required Normal saline (0.9% NaCl)
Storage 2-8℃
Valid period 12 months


Dilution of Sample

It is recommended to take 2~3 samples with expected large difference to do pre-experiment before formal experiment and dilute the sample according to the result of the pre-experiment and the detection range (0.04-30 mmol/L).

The recommended dilution factor for different samples is as follows (for reference only):

Sample type Dilution factor
Human serum 1
Mouse serum 1
Rat serum 1
Human plasma 1

 

Note: The diluent is normal saline (0.9% NaCl).

 

Detection Principle

Glucose oxidase can catalyze the oxidation of glucose to gluconic acid to produce hydrogen peroxide. In the presence of chromogenic oxygen receptors, peroxidase catalyzes hydrogen peroxide and oxidizes pigment sources to form colored substances. Measure the OD value at 505 nm and glucose content can be calculated indirectly.

 

Kit Components & Storage

Item Component Size 1(48 T) Size 2(96 T) Storage
Reagent 1 Phenol Solution 10 mL × 1 vial 20 mL × 1 vial 2-8°C, 12 months, shading light
Reagent 2 Enzyme Solution 10 mL × 1 vial 20 mL × 1 vial 2-8°C, 12 months, shading light
Reagent 3 50 mmol/L Glucose Standard 1.2 mL × 1 vial 1.2 mL × 1 vial 2-8℃, 12 months
Microplate 96 wells No requirement
Plate Sealer 2 pieces

 

Note: The reagents must be stored strictly according to the preservation conditions in the above table. The reagents in different kits cannot be mixed with each other. For a small volume of reagents, please centrifuge before use, so as not to obtain sufficient amount of reagents.

 

Technical Data:

Parameter:

Intra-assay Precision

Three human serum samples were assayed in replicates of 20 to determine precision within an assay. (CV = Coefficient of Variation)

Parameters Sample 1 Sample 2 Sample 3
Mean (mmol/L) 1.50 13.40 25.50
%CV 2.4 2.1 1.2


Inter-assay Precision

Three human serum samples were assayed 20 times in duplicate by three operators to determine precision between assays.

Parameters Sample 1 Sample 2 Sample 3
Mean (mmol/L) 1.50 13.40 25.50
%CV 2.5 1.7 2.7

 

Recovery

Take three samples of high concentration, middle concentration and low concentration to test the samples of each concentration for 6 times parallelly to get the average recovery rate of 100%.

Standard 1 Standard 2 Standard 3
Expected Conc. (mmol/L) 3.6 11.5 24.5
Observed Conc. (mmol/L) 3.6 11.4 24.5
Recovery rate (%) 101 99 100

 

Sensitivity

The analytical sensitivity of the assay is 0.04 mmol/L. This was determined by adding two standard deviations to the mean O.D. obtained when the zero standard was assayed 20 times, and calculating the corresponding concentration.

 

Standard Curve

As the OD value of the standard curve may vary according to the conditions of the actual assay performance (e.g. operator, pipetting technique or temperature effects), so the standard curve and data are provided as below for reference only:

Concentration (mmol/L) 0 2 5 10 15 20 25 30
Average OD 0.043 0.152 0.318 0.583 0.863 1.148 1.406 1.647
Absoluted OD 0 0.110 0.276 0.540 0.820 1.106 1.363 1.604