![Fig. 4. γ-IFN–induced increase of surface MHC class I expression is not affected by PML-specific RNA interference or by expression of PML mut ex3. / HEK293 cells were either untreated (left panel) or treated with 1000 U/ml γ-IFN (right panel) (time [t] = 0), and subsequently transfected with PML-specific siRNA duplex (middle row) or with GFP-PML mut ex3 (bottom row) (t = 6 hours). After 2 additional days (t = 54 hours), cells were processed for fluorescence microscopy and flow cytometry. Cells growing on glass coverslips were immunostained with anti-PML followed by GAM-Alexa 594 antibodies (red fluorescence, first and fourth columns) and counterstained with DAPI (blue fluorescence, second and fifth columns). Cells processed for flow cytometry were immunostained with anti–MHC class I mAb (W6.32) followed by GAM-PE. Histograms of MHC class I expression are shown for control and siRNA-transfected cell cultures, while bivariate dot plots of GFP fluorescence (x-axis) and MHC class I expression (y-axis) are reported for PML mut ex3–transfected cell cultures. Percentage of GFP-positive cells (ie, of PML mut ex3–transfected cells) is reported. The negative control of MHC class I expression, obtained using isotype-matched antibodies followed by GAM-PE, is shown in gray.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/101/9/10.1182_blood-2002-11-3335/4/h80934202004.jpeg?Expires=1724936405&Signature=Udyg56Lzz6RD3~C8inqyG4H7-Vvb05U92C5Ri0tB6rK7u55-~RvGCeB7DMlxvPIpgBW2xDnAsWqG0H~b3-BVz-J~5ZqApOqf-BKdWB9R4Nd1VXU5WbL6rcqOrftUDe8iltBKOdmecMRbz--L08zQV226Kpbc~AEKe~b7K7iFDeFl4ijROGc0NHLmpPLBe26EMq9vHyEttmnGAFrjH3KcM37kboDrdDiUN1hduHIqjgdUrCE5QsQOkVY-VCbpVpjR8zi4t~zafTJwYIXtwVVH-QIOV4jwOlPY1xfcVt--KaQDGWbftcQbFjNmwPbVWwm7B3MawRRTAaNJm5rXG83Leg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
γ-IFN–induced increase of surface MHC class I expression is not affected by PML-specific RNA interference or by expression of PML mut ex3.
HEK293 cells were either untreated (left panel) or treated with 1000 U/ml γ-IFN (right panel) (time [t] = 0), and subsequently transfected with PML-specific siRNA duplex (middle row) or with GFP-PML mut ex3 (bottom row) (t = 6 hours). After 2 additional days (t = 54 hours), cells were processed for fluorescence microscopy and flow cytometry. Cells growing on glass coverslips were immunostained with anti-PML followed by GAM-Alexa 594 antibodies (red fluorescence, first and fourth columns) and counterstained with DAPI (blue fluorescence, second and fifth columns). Cells processed for flow cytometry were immunostained with anti–MHC class I mAb (W6.32) followed by GAM-PE. Histograms of MHC class I expression are shown for control and siRNA-transfected cell cultures, while bivariate dot plots of GFP fluorescence (x-axis) and MHC class I expression (y-axis) are reported for PML mut ex3–transfected cell cultures. Percentage of GFP-positive cells (ie, of PML mut ex3–transfected cells) is reported. The negative control of MHC class I expression, obtained using isotype-matched antibodies followed by GAM-PE, is shown in gray.
