Nitratna reduktaza (NR) Komplet za ispitivanje (Griess-borimetrijska metoda)

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Opis

Pregled proizvoda

NR (EC 1.7.1.3) is a widely found enzyme in plants. It plays a crucial role in converting nitrate nitrogen to ammonia nitrogen and is also an inducible enzyme, affecting crop yield and quality. NR catalyzes the reduction of nitrate to nitrite: NO3- + NADH+H+ → NO2- + NAD+ + H2O. Under acidic conditions, the produced NO2- can participate in a diazotization reaction to form a magenta-colored compound. This compound has an absorption peak at 540 NM, and the change in absorbance at 540 nm can be used to represent enzyme activity.

Kit Components

  • Inducer Stock Solution: 50 mL x 1 bottle
  • Extraction Solution: 30 mL x 1 bottle
  • Reagent One: 12 mL x 1 bottle
  • Reagent Two: Powder x 2 bočice
  • Reagent Three: 15 mL x 1 bottle
  • Reagent Four: 15 mL x 1 bottle
  • Standard: 1 mL x 1 vial

Solution Preparation

  1. Inducer Solution: Dilute the inducer stock solution 10-fold with distilled water before use. uzeti 10 mL of inducer stock solution and add 90 mL of distilled water. Temeljito promiješajte. Prepare fresh before each use.
  2. Reagent Two: Dodati 1 mL of distilled water. Aliquot and store at -20°C. It can be stored for 2 weeks at -20°C. Prije upotrebe, dilute Reagent Two 50-fold with distilled water. uzeti 10 μL of Reagent Two and add 490 μL of distilled water. Mix well.
  3. Standard: Prepare a 0.1 μmol/mL sodium nitrite standard solution by diluting the 10 μmol/mL sodium nitrite standard solution 100-fold with distilled water before use.

Bilješke

  1. If the absorbance is greater than 0.8, dilute the sample with extraction solution. Pay attention to adjusting the dilution factor accordingly in the calculation formula.
  2. Strictly follow the order of adding reagents listed in the sample assay table for the experiment.

Experimental Procedures

Ja. Sample Treatment

  1. Tissue Pre-treatment:

    • Add an appropriate amount of inducer solution to a beaker. Wash fresh samples, dry them with filter paper, and place them in the inducer solution (enough to submerge). Incubate in the dark for 2 sati. Remove samples, dry them with filter paper, and freeze at -20°C for 30 minuta. Thaw samples and dry them with filter paper again. (Perform induction treatment as needed. Općenito, induction treatment is not required. If the pre-experiment results show no activity, induction treatment is necessary.)
    • Weigh approximately 0.1 g of sample and add 1 mL of extraction solution according to the ratio of tissue weight (g) to extraction solution volume (ml) od 1:5 do 10. Grind in an ice bath, centrifuga na 8000 g, 4°C for 10 minuta, and collect the supernatant. Keep the supernatant on ice for testing.
  2. Cell or Bacteria Pre-treatment:

    • Collect cell or bacteria samples in a centrifuge tube and discard the supernatant. Dodati 1 mL of extraction solution per 5 Milijun stanica ili bakterije. Sonicate the bacteria or cells (vlast 200 W, sonication 3 sekundi, interval 10 sekundi, ponoviti 30 vrijeme). Centrifuga na 8000 g, 4°C for 10 minuta, collect the supernatant and keep it on ice for testing.

Ii. Assay Steps

  1. Preheat the visible spectrophotometer for at least 30 minuta, Podesite valnu duljinu na 540 NM, and zero with distilled water.
  2. Sample Assay:
Ime reagensa Test Tube Control Tube Standard Tube Blank Tube
Uzorak 100 μL
0.1 μmol/mL Standard Solution 100 μL
Distilled Water 375 μL 475 μL
Reagent One 375 μL 375 μL
Reagent Two 125 μL 125 μL 125 μL 125 μL
Reagent Three 250 μL 250 μL 250

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