Cell Technology’s Cholesterol assay kit provides a simple, one-step fluorimetric or colorimetric method for the determination of total cholesterol in serum and plasma samples. The assay is based on an enzyme-coupled reaction that detects both free cholesterol and cholesterol esters. Cholesterol esters are hydrolyzed by cholesterol esterase into cholesterol, which is then oxidized by cholesterol oxidase to yield hydrogen peroxide and cholest-4-en-3-one (ketone). The hydrogen peroxide then reacts with the cholesterol probe (detection reagent) in a 1:1 stoichiometry to produce the stable fluorescent product

Cholesterol ester↓ Cholesterol esteraseCholesterol↓ Cholesterol OxidaseH2O2 + Cholest-4-en-3-one↓Cholesterol probe

Fluorescent Product

λmax 570nm. λ ex/em 535/585nm.

Colorimetric assay can be read on a spectrophotometer at 570nm.

Fluorescence is measured at excitation 530nm and emission 585nm.

Figure 1. Cholesterol standard curve was generated using fluorimetric detection: excitation 535nm and emission 585nm. R2 value=0.9977. Incubation time= 1 hr at Room temperature. Standard curve range 0.15625 µM to 10µM.

Figure 2. Cholesterol standard curve generated using colorimetric detection: absorbance read-out at 570nm. R2 =0.9993. Incubation time=30 minutes. Standard curve range 1.25µM to 80µM.

Figure 3. demonstrates the quantitation of total cholesterol in mg/dL in animal sera