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AMPK Methods and Protocols

(Rick Simeone) #1

  1. Enter the average absorbance value from each experimental
    duplicate into the rearranged equation (as they-value), and
    then proceed to solve equation to produce the known protein
    concentration.

  2. Normalize disintegrations per minute (DPM) to milligram of
    protein for each sample (seeNote 14).


3.3 acLDL Uptake 1. After BMDM have differentiated, seed cells at a density of
2.5 105 cells per 24-well.



  1. The following day, remove medium and wash cells with
    1 PBS.

  2. Add 0.5 mL of BMDM medium containing 10 μg/mL
    Dil-acLDL, and incubate in a humidified 5% CO 2 incubator
    at 37C for 1–2 h.

  3. Remove the medium and wash twice with 1PBS.

  4. Add 250μL of isopropyl alcohol to each well, seal plates with
    parafilm, and cover with aluminum foil.

  5. Incubate plate at room temperature for 10 min and then at
    4 C overnight with gentle rocking.

  6. Collect isopropyl alcohol from each well in a 1.5 mL microfuge
    tube (seeNote 15).

  7. Load 70μL on a fluorescence compatible 96-well plate.

  8. Add a serial dilution of Dil-acLDL as standards to calibrate
    fluorescence, as well as non-Dil-acLDL loaded samples and
    isopropyl alcohol controls.

  9. Read the plate using a fluorometric plate reader with an excita-
    tion of 545 nm and emission wavelength of 580 nm (or com-
    parable fluorescent plate reader) (seeNote 16).


3.4 Cholesterol
Efflux



  1. After BMDM have differentiated, seed cells at 2.5 105 cells/
    well in 24-well plates.

  2. Incubate lipid-loading DMEM with 1μCi/mL^3 H-cholesterol
    at 37C overnight to conjugate.

  3. The following day, remove the media from the cells and wash
    with 1PBS.

  4. Add 0.5 mL of the lipid-loading medium supplemented with
    1 μCi/mL^3 H-cholesterol to each well (seeNote 17).

  5. Incubate cells in a humidified 5% CO 2 incubator at 37C for
    30 h to induce acLDL uptake and accumulation.

  6. Remove the medium and wash the cells twice with 1PBS to
    remove all exogenous lipid and radioactivity.

  7. To allow time for the cholesterol pools to equilibrate, add
    0.5 mL of equilibration medium.


Assessing Macrophage Cholesterol Homeostasis 487
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