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Glycogen Fluorometric Assay Kit

  • Cat.No.:E-BC-F040

  • Detection instrument: Fluorescence microplate reader (Ex/Em=535 nm/587 nm)

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  • 96T
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Detection principle

Glycogen produces glucose under the action of starch glycosidase, and glucose is catalyzed by glucose oxidase to produce hydrogen peroxide. In the presence of the peroxidase, hydrogen peroxide be oxidized to produce the fluorescence substrate. The fluorescence intensity at the excitation wavelength of 535 nm and emission wavelength of 587 nm is proportional to the glycogen content.

Performance characteristics

Sample type Animal liver and muscle tissue
Sensitivity 0.06 μg/mL
Detection range 0.06-4.0 μg/mL
Detection method Fluorescence method
Assay type Quantitative
Assay time 50min
Precision Average inter-assay CV: 6.600%Average intra-assay CV: 3.400%
Other instruments required Micropipettor, Incubator, Centrifuge
Storage -20℃
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 (0.06-4.0 μg/mL).

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

Sample type

Dilution factor

10% Rat liver tissue homogenate

3000-5000

10% Mouse muscle tissue homogenate

10-20

Note: The diluent is reagent 1. Liver samples can be diluted step by step.

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