Glycogen Assay Kit
Nota: Prendi due o tre campioni diversi per la previsione prima del test.
Attrezzatura operativa: Spectrophotometer/ microplate reader
Numero di catalogo: BC0345
Misurare:100T/96S
Componenti:
Extract reagent: 100ml×1, storage at 4℃.
Regent I: Polvere×1, storage at 4℃.10 mg of glucose, aggiungere 1 mL of distilled water to dissolve it before use. Diluted with distilled water to 0.1 mg/mL glucose solution for standby, ready to use. 0.1 mg/mL glucose standard solution, storage at 4℃.
Regent Ⅱ: Polvere×1, storage at 4℃.
Soluzione funzionante: Pour 6 mL of distilled water into Reagent Ⅱ and slowly pour 24 mL of concentrated sulfuric acid. Dissolve and mix thoroughly before use. Unused reagents are valid at 4 °C for one week.
Descrizione del prodotto
Glycogen is a high molecular polysaccharide composed of glucose units. It is one of the main storage forms of sugar. It is mainly stored in the liver and muscle as backup energy, and is called liver glycogen and muscle glycogen, rispettivamente. Glycogen can regulate blood glucose concentration. Glycogen can be synthesized in the liver when blood glucose rises. When blood sugar decreases, liver glycogen is broken down into glucose to supplement blood sugar. Perciò, liver glycogen is important to maintain the relative balance of blood sugar. Muscle glycogen is a form of glycogen storage in muscles. When lots of blood sugar is consumed during strenuous exercise, muscle glycogen cannot be broken down directly into blood sugar. It must first be broken down to produce lactic acid, which is circulated to the liver with the blood, and transformed into liver glycogen through glycogen glucose.
Determination principle: anthrone method. Glycogen is extracted with strong alkaline extract, and the glycogen content is measured using an anthrone method under strongly acidic conditions.
Reagenti e attrezzature necessari ma non forniti.
Spectrophotometer/ microplate reader, centrifuga da tavolo, transfer pipette, micro glass cuvette/96-well plate, mortar, concentrated sulfuric acid (H2SO4) e acqua distillata.
Procedura:
IO. Sample extraction:
- Cells or bacteria: Raccogliere 5-10 million bacteria or cells into a centrifuge tube, discard the supernatant after centrifugation; add 0.75mL of extraction reagent to ultrasonically break bacteria or cells (energia 20% o 200 W, ultrasonic 3s, 10s interval, repeat 30 volte) ); Transfer to a 10mL tube, boil in a boiling water bath for 20min (close tightly to prevent water loss), shake the tube every 5 min to fully mix; take out the tube and cool, take up to 5mL with distilled water and mix. Centrifuge at 8000g and 25℃ for 10min, take the supernatant for testing.
- Tessuto: Weigh 0.1~0.2g sample and put it in a 10 mL tube, aggiungere 0.75 mL of Extraction solution, boil in boiling water bath for 20 min (close tightly to prevent water loss), shake the test tube every 5 min to fully mix. After all the tissue dissolved, take out the tube and cool down, then make up to 5 mL with distilled water. Centrifuge at 8000g and 25℃ for 10 min, take the supernatant for testing.
II. Determinazione procedura:
- Preheat the Spectrophotometer/ microplate reader for 30 min, regolare la lunghezza d'onda su 620 nm, azzerare con il distillato
- Sampling table (add the following regents in EPtube)
| Regent(μL) | Tubo vuoto (A1) | Standard Tube (A2) | Provetta (A3) |
| Campione | 60 | ||
| Regent I | 60 | ||
| distilled water | 60 | ||
| Regent Ⅱ | 240 | 240 | 240 |
Mix well, place in a boiling water bath for 10 minuti (close tightly to prevent water loss), cool, and take 200 μL into micro glass cuvette/96-well plate to read the absorbance of the blank tube, standard tube, and measurement tube at 620 nm, and record them as A1, A2, and A3. The blank tube and standard tube need only be tested once.
III. Calcolo:
- Peso del campione
Sorbitol (mg/g fresh weight) =(Cs×V1)×(A3-A1)÷(A2-A1)÷(W×V1÷V2)÷1.11
= 0.450×(A3-A1)÷(A2-A1)÷W
- Concentrazione proteica
Sorbitol (mg/mg prot) = (Cs×V1)×(A3-A1) ÷(A2-A1) ÷(V1×Cpr) ÷1.11
=0.09×(A3-A1) ÷(A2-A1) ÷Cpr
- The number of bacteria or cells:
Sorbitol(mg/104 cell)= (Cs×V1)×(A3-A1)÷(A2-A1)÷(number of bacteria or cells×V1÷V2) ÷1.11
= 0.450×(A3-A1)÷(A2-A1)÷number of bacteria or cells
1.11: It is a constant that glucose content converted to glycogen content, That is, the color of 111 μg of glucose with anthrone reagent is equivalent to that of 100 μg of glycogen with anthrone reagent.
Cs: the concentration of standard, 0.1 mg/mL V1: sample volume, 0.06 ml;
V2: Total sample volume, 5 ml;
Cpr: concentrazione delle proteine del campione, mg/ml; W: Peso del campione, G
Number of bacteria or cells: 104 as the unit, ten thousand
Nota:
If A is greater than 1.4, dilute the sample with distilled water and multiply it by the corresponding dilution factor in the calculation formula.
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Technical Specification:
The detection limit: 0.002 mg/ml
The linear range: 0.003125-0.25 mg/ml
Recensioni
Non ci sono ancora recensioni.