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  • 發布時間:2019-04-22 23:41 原文鏈接: BradfordProteinConcentrationAssay

    Bradford Protein Concentration Assay
    version 01/07/2001

    Abbreviations:

    • mcg = micrograms

    • mcL = microliters

    • BSA = bovine serum albumin

    • O.D. = optical density

    • dI = deionized

    Background

    The Bradford protein assay (1) is one of several simple methods commonly used to determine the total protein concentration of a sample. The method is based on the proportional binding of the dye Coomassie to proteins. Within the linear range of the assay (~5-25 mcg/mL), the more protein present, the more Coomassie binds. Furthermore, the assay is colorimetric; as the protein concentration increases, the color of the test sample becomes darker. Coomassie absorbs at 595 nm. The protein concentration of a test sample is determined by comparison to that of a series of protein standards known to reproducibly exhibit a linear absorbance profile in this assay. Although different protein standards can be used, we have chosen the most widely used protein as our standard - Bovine Serum Albumin (BSA).

    Procedure

    • Prepare a 4-fold dilution of a 2 mg/mL BSA sample by adding 50 mcL of 2 mg/mL BSA to 150 mcL of dI water to make 200 mcL of 0.5 mg/mL BSA.

    • Generate test samples for the reference cell, blank, BSA standards and the protein sample to be tested according to Table 1 in disposable cuvettes.

    • Note that the "reference cell" and "blank" are identical. A reference cell test sample is only required when using a double-beam UV-visible spectrophotometer for absorbance measurements.

    • Note that a dilution of the protein sample may be required for the resulting absorbance to fall within the linear range of the assay.

    • Allow each sample to incubate at room temperature for 10-30 minutes. (Record the actual incubation time in your notebook.)

    • Measure the absorbance of each sample at 595 nm using a UV-visible spectrophotometer. Be sure to allow the instrument to warm up for at least 15 minutes prior to use.

    • Plot the absorbance of each BSA standard as a function of its theoretical concentration. The plot should be linear.

    • Determine the best fit of the data to a straight line in the form of the equation "y = mx + b" where y = absorbance at 595 nm and x = protein concentration.

    • Use this equation to calculate the concentration of the protein sample based on the measured absorbance. Note: If the absorbance of the test sample is outside of the absorbance range for the standards, then the assay must be repeated with a more appropriate dilution, if any. The linear range for the assay (and for most spectrophotometers is 0.2 - 0.8 O.D. units.

    Table 1. Preparation of test samples for the Bradford protein assay.

    Test Sample
    Sample Volume,
    mcL
    Vol. Water,
    mcL
    Vol. Bradford Reagent,
    mcL
    Reference Cell
    0
    800
    200
    Blank
    0
    800
    200
    BSA Standard - 5 mcg/mL
    10
    790
    200
    BSA Standard - 10 mcg/mL
    20
    780
    200
    BSA Standard - 15 mcg/mL
    30
    770
    200
    BSA Standard - 20 mcg/mL
    40
    760
    200
    BSA Standard - 25 mcg/mL
    50
    750
    200
    Protein Sample
    50
    750
    200


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