Figure 4.
Figure 4. A decrease in lipid packing precedes PS exposure in B cells. (A) Lymphocytes from C57BL/10 mice were labeled with anti-CD19APC antibody and preincubated with either 0.05 μM MC540 or AVFITC. Histograms show (mean fluorescence units) the rate of (Ai) MC540 binding or (Aii) PS exposure (binding of AV) by CD19+ B cells following stimulation with 3 μM (red lines), 2 μM (blue lines), or 1 μM (green lines) calcimycin. (Bi) Lymphocytes from C57BL/10 and NOD mice were labeled with anti-CD19APC and anti-CD19PERCP antibodies, respectively, mixed, and preincubated with 0.05 μM MC540. Panels show density plots of the rate of decrease in lipid packing (increased uptake of MC540) by B cells from C57BL/10 (left panel) and from NOD mice (center panel) in the same tube following stimulation with 2 μM calcimycin (arrows). The right panel shows an alternative plot of the same data plotted as the percentage of cells binding high levels of MC540 as a function of time. Red lines, NOD B cells; blue lines, C57BL/10 B cells. (Bii) Histograms of MC540 binding by the B-cell populations shown in panel Bi, gated at t = 0 seconds and t = 400 seconds. Red lines, NOD B cells; blue lines, C57BL/10 B cells. (C) Results of 3 independent experiments equivalent to that in panel Bi but with lymph node cells derived from NOD (red lines) and DBA/2 (green lines) mice. (D) Calcium uptake in stimulated B cells. (Di) Lymphocytes from the C57BL/10 (red line) and NZW (blue line) mice were labeled with anti-CD19APC and anti-CD19PERCP antibodies respectively, mixed, incubated with 0.25 μM of the calcium-sensitive indicator Fluo-4AM for 10 minutes, washed, and stimulated with 0.2 μM calcimycin (arrow). Plots show Ca2+ uptake as a function of time. (Dii) Shows an equivalent experiment to that in panel Di but with lymph node cells derived from DBA/2 (red line) and NZW (blue line) mice.

A decrease in lipid packing precedes PS exposure in B cells. (A) Lymphocytes from C57BL/10 mice were labeled with anti-CD19APC antibody and preincubated with either 0.05 μM MC540 or AVFITC. Histograms show (mean fluorescence units) the rate of (Ai) MC540 binding or (Aii) PS exposure (binding of AV) by CD19+ B cells following stimulation with 3 μM (red lines), 2 μM (blue lines), or 1 μM (green lines) calcimycin. (Bi) Lymphocytes from C57BL/10 and NOD mice were labeled with anti-CD19APC and anti-CD19PERCP antibodies, respectively, mixed, and preincubated with 0.05 μM MC540. Panels show density plots of the rate of decrease in lipid packing (increased uptake of MC540) by B cells from C57BL/10 (left panel) and from NOD mice (center panel) in the same tube following stimulation with 2 μM calcimycin (arrows). The right panel shows an alternative plot of the same data plotted as the percentage of cells binding high levels of MC540 as a function of time. Red lines, NOD B cells; blue lines, C57BL/10 B cells. (Bii) Histograms of MC540 binding by the B-cell populations shown in panel Bi, gated at t = 0 seconds and t = 400 seconds. Red lines, NOD B cells; blue lines, C57BL/10 B cells. (C) Results of 3 independent experiments equivalent to that in panel Bi but with lymph node cells derived from NOD (red lines) and DBA/2 (green lines) mice. (D) Calcium uptake in stimulated B cells. (Di) Lymphocytes from the C57BL/10 (red line) and NZW (blue line) mice were labeled with anti-CD19APC and anti-CD19PERCP antibodies respectively, mixed, incubated with 0.25 μM of the calcium-sensitive indicator Fluo-4AM for 10 minutes, washed, and stimulated with 0.2 μM calcimycin (arrow). Plots show Ca2+ uptake as a function of time. (Dii) Shows an equivalent experiment to that in panel Di but with lymph node cells derived from DBA/2 (red line) and NZW (blue line) mice.

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