Description

Pyruvate is a key intermediate in cellular metabolic pathways. Pyruvate can be converted to carbohydrates via gluconeogenesis, to fatty acids or energy through acetyl-CoA, to the amino acid alanine and to ethanol. Abnormal levels of pyruvate have been linked to liver diseases and metabolic disorders. Simple, direct and automation-ready procedures for measuring pyruvate concentrations find wide applications in research and drug discovery. BioAssay Systems pyruvate assay uses a single Working Reagent that combines pyruvate oxidase and hydrogen peroxide determination in one step. The color intensity of the reaction product at 570nm or fluorescence intensity at lem/ex = 585/530nm is directly proportional to pyruvate concentration in the sample.

Key features

Sensitive and accurate. Use as little as 10 mL samples. Linear detection range in 96-well plate: 2 to 500 mM (17 mg/dL to 4.4 mg/dL) pyruvate for colorimetric assays and 0.2 to 50 mM for fluorimetric assays.

Simple and convenient. The procedure involves addition of a single working reagent and incubation for 30 min at room temperature, compatible for HTS assays.

Improved reagent stability. The optimized formulation has greatly enhanced the reagent and signal stability.

Applications:

Direct Assays: pyruvate in biological samples.

Drug Discovery/Pharmacology: effects of drugs on pyruvate metabolism.

Kit Contents

  Enzyme Mix:     10 mL      

  Dye Reagent:  120 mL  

  Standard: 400 mL 25 mM Pyruvate

Storage conditions. The kit is shipped on dry ice. Store all reagents at -20°C. Shelf life of three months after receipt.

Precautions: reagents are for research use only. Normal precautions for laboratory reagents should be exercised while using the reagents. Please refer to Material Safety Data Sheet for detailed information.

Coloriemtric Procedure

Note: SH-group containing reagents (e.g. mercaptoethanol, DTT) may interfere with this assay and should be avoided in sample preparation.

1. Equilibrate all components to room temperature. Prepare a 500 mM Standard Premix by mixing 10 mL of the 25 mM Standard and 490 mL H₂O. Dilute Standard in distilled water as follows.

Transfer 10 mL standards and 10 mL samples into separate wells of a clear flat-bottom 96-well plate.

2. For each reaction well, mix 94 mL Enzyme Mix and 1 mL Dye Reagent in a clean tube. Transfer 90 mL Working Reagent into each assay well. Tap plate to mix. Freeze unused reagents for future use.

3. Incubate 30 min at room temperature. Read optical density at 570nm (550-585nm).

Note: if the Sample OD is higher than the Standard OD at 500 mM, dilute sample in water and repeat the assay. Multiply result by the dilution factor.

CALCULATION

Subtract blank OD (water, #8) from the standard OD values and plot the OD against standard concentrations. Determine the slope using linear regression fitting. The pyruvate concentration of Sample is calculated as

OD_SAMPLE and OD_H2O are optical density values of the sample and water.

Conversions: 1mM pyruvate equals 8.7 mg/dL or 87 ppm.

Fluorimetric Procedure

For fluorimetric assays, the linear detection range is 0.2 to 50 mM pyruvate. Dilute the Standards prepared in Colorimetric Procedure 1:10 in H₂O.  

Transfer 10 mL standards and 10 TUNEology 波长可调检测卡盒-->