Attribut | Einzelheiten |
---|---|
Notiz | Nehmen Sie vor dem Test zwei oder drei verschiedene Proben zur Vorhersage |
Erkennungsinstrument | Spektrophotometer |
Katze nein | BC3400 |
Größe | 50T/48S |
Komponenten:
Lösung extrahieren: 55ml × 1, gespeichert bei 4 °C.
Reagens 1: 40ml × 1, gespeichert bei 4 °C and protected from light.
Reagens 2: Powder × 1, gespeichert bei -20 °C and protected from light. Just before use, hinzufügen 6 mL of distilled water to fully dissolve. Unused reagents are stored at -20 °C für 1 week after dispensing to avoid repeated freeze-thaw cycles.
Reagens 3: powder × 1, gespeichert bei -20 °C and protected from light. Just before use, hinzufügen 6 mL of distilled water to fully dissolve. Unused reagents are stored at -20 °C after dispensing. Prohibition of repeated freeze-thaw cycles.
Reagens 4: 91µL × 2, gespeichert bei 4 °C and protected from light. Just before use, hinzufügen 0.209 mL of distilled water to fully dissolve. Gespeichert bei 4 °C für 1 Woche.
Reagens 5: Powder × 2, gespeichert bei -20 °C and protected from light. Just before use, hinzufügen 0.3 mL of distilled water to fully dissolve. Unused reagents are stored at -20 °C für 1 week after dispensing.
Reagens 6: 60 µL × 1, gespeichert bei 4 °C and protected from light. Just before use, hinzufügen 0.6 mL of distilled water to fully dissolve. Gespeichert bei 4 °C für 1 Woche.
Produktbeschreibung:
Pyrophosphate: Fructose-6-phosphate-1-phosphotransferase (PFP, EC2.7.1.90) is a cytosolic enzyme that is widely present in plant tissues and catalyzes the phosphorylation of fructose-6-phosphate like phosphofructokinase. As a result, the single PEP catalytic reaction is a reversible reaction, and pyrophosphate is used instead of ATP, which plays an important role in carbon metabolism of photosynthesis.
PFP catalyzes the conversion of fructose 6-phosphate to fructose 1,6-diphosphate, which is converted to dihydroxyacetone phosphate by the action of aldolase and triose phosphate isomerase, and then catalyzed by α-phosphate glycerol dehydrogenase and NADH to from Glycerol 3-diphosphate and NAD. The change in absorbance at 340 nm reflects the level of PFP activity.
Required material
Low temperature centrifuge, spectrophotometer, water bath/constant temperature incubator, Mörtel/Homogenisator, 1 ml-Quarzküvette, Pipette übertragen, Eis und destilliertes Wasser, EP tube.
Verfahren:
ICH. Probe Extraction:
-
- Gewebeprobe:
According to the mass of the tissue (G): the volume of the extract solution (ml) is 1: 5 ~ 10. Suggested 0.1g of tissue with 1mL of extract solution. Fully grind on ice, centrifugated at 20000g and 4℃ for 15 Mindest. Supernatant is placed on ice for test.
- Bakterien oder Zellen:
According to the number of cells (104): the volume of the extract solution (ml) is 500 ~ 1000: 1. Recommend 5 million with 1mL of Extract Solution. Use ultrasonication to split bacteria or cells (power 300W, Arbeitszeit 3s, interval 7s, total time 3 Mindest). Centrifugated at, 20000g and 4℃ for 15 Mindest. Supernatant is placed on ice for test.
- Liquids: direct detection.
II. Bestimmung Verfahren:
- Das Spektrophotometer vorheizen 30 Mindest, Wellenlänge anpassen 340 nm, Null mit destilliertem Setzen
- Fügen Sie Reagenzien mit der folgenden Liste hinzu:
Reagenzname (μL) | Reagenzglas (T) | Leeres Rohr (T) |
Reagens 1 | 670 | 670 |
Reagens 2 | 100 | 100 |
Reagens 3 | 100 | 100 |
Reagens 4 | 10 | 10 |
Reagens 5 | 10 | 10 |
Reagens 6 | 10 | 10 |
Probe | 100 | – |
Destilliertes Wasser | – | 100 |
After thorough mixing, measure the initial value A1 at 340 nm and the absorbance A2 for 30 Minuten um 37 °C in a 1 ml-Quarzküvette, and record them as A1T, A1B, and A2T, A2B. Calculate ΔA = (A1T-A2T)- (A1B-A2B).
Notiz: Reagenzien 1, 2, 3, 4, 5, Und 6 can also be formulated into working fluids according to the proportions of the operation table, which is now prepared for use; The blank tubes need only be made 1–2 times. |
III. Calculation of PFP Aktivität:
1 Calculated by micro quartz cuvette
- Calculated by protein concentration:
Einheitendefinition: One unit of enzyme activity is defined as that 1 mg of tissue protein per minute consumes 1 nmol of NADH.
PFP activity (U/mg-Schutz) =ΔA÷(ε×d)×VRT×109÷(VS×Cpr) ÷T=53.59×ΔA÷Cpr
- Calculated by sample weight
Einheitendefinition: One unit of enzyme activity is defined as that 1g of tissue per minute consumes 1 nmol of NADH.
PFP activity (U/g fresh weight) =ΔA÷(ε×d)×VRT×109÷(W ×VS÷VE) ÷T=53.59×ΔA÷W
- Calculated by bacteria or cell amount:
Einheitendefinition: One unit of enzyme activity is defined as that 10 thousand bacteria or cells per minute consumes 1 nmol of NADH.
PFP activity (U/104 -Zelle) =ΔA÷(ε×d)×VRT×109÷(VS×N÷VE) ÷T=53.59×ΔA÷N(104)
- Calculated by serum and other liquids:
Einheitendefinition: One unit of enzyme activity is defined as that 1 mL of liquids per minute consumes 1 nmol of NADH.
PFP activity (U/ml) =ΔA÷(ε×d)×VRT×109÷VS÷T=53.59×ΔA
Vrt: total volume of reaction system, 0.001 L;
e: Molarer NADH-Extinktionskoeffizient, 6.22 × 103 L/mol/cm; D: cuvette light path, 1 cm;
Vs: added sample volume, 0.1 ml;
VE: volume of extract solution added, 1 ml; T: Reaktionszeit, 30 Mindest;
Cpr: Probenproteinkonzentration, mg/ml; W: Probenmasse, 0.1 G;
109:conversion factor, 1 mol = 109 nmol N: number of cell
- Calculated by 96-well UV plate:
Modify d = 1 cm in the above formula to d-0.6 cm (the light path of a 96-well plate) for calculation.
Notiz:
- The number of samples should not be too large to avoid delaying the enzymatic reaction time.
Experimentelle Beispiele:
- Nehmen 0.1 g of bean sprouts and add 1 mL of Extract solution for sample processing. After centrifugation to take the supernatant, Fahren Sie nach dem Bestimmungsverfahren fort. CalculateΔA = (A1T-A2T)-(A1B-A2B)= (1.041-0.963)-0=0.078. The enzyme activity is calculated according to the sample mass.
PFP activity (U/g fresh weight) =53.59×ΔA÷W=41.8 U/g fresh weight.
Verwandte Produkte:
BC0990/BC0995 Plant Chlorophyll Content Assay Kit
BC2210/BC2215 Glyceraldehyde-3-phosphate Dehydrogenase(GAPDH) Aktivitätstest-Kit
BC4330/BC4335 Plant Carotenoid Content Assay Kit
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