Figure 3
Figure 3. Plg deficiency delays clearance of apoptotic cells in vivo. (A-B) Cell Tracker Green CMFDA-labeled mouse apoptotic thymocytes were injected IV into Plg+/+ and Plg−/− mice. (A) Fluorescent microscopic images in duplicate (top and bottom panels are from 2 different Plg+/+ and 2 different Plg−/− mice) showing green-labeled apoptotic thymocytes trapped in the marginal zone of harvested spleens. Images with original magnification of ×20 were captured at room temperature under a Leica DMR upright microscope using an α Retiga EXi Cooled CCD camera and Image-Pro Plus software. The 4′,6 diamidino-2-phenylindole (blue) stains nuclei of splenic cells. Images are representative of 5 Plg+/+ and 5 Plg−/− mice. (B) Quantification of apoptotic thymocytes as areas of fluorescence in the spleens of Plg+/+ and Plg−/− mice. Bars are mean ± SD of average green fluorescence area per microscopic field. Three to 5 microscopic fields were counted from 5 mice per group. (C-D) Cell Tracker Green CMFDA-labeled apoptotic thymocytes were injected into the peritoneum of Plg+/+ or Plg−/− mice. Peritoneal cells were collected 1 hour postinjection and analyzed by flow cytometry. (C) A representative flow cytometry histogram comparing the fluorescence intensity of peritoneal lavage cells and showing the enhanced accumulation of thymocytes in Plg−/− mice compared with Plg+/+ mice. (D) Quantitative analysis of cells recovered from peritoneum of Plg+/+ or Plg−/− mice. Fluorescent cells with MFI are gated and MFI values derived from these cells are used in the calculation. Bars are mean ± SD of average green fluorescence (n = 3).

Plg deficiency delays clearance of apoptotic cells in vivo. (A-B) Cell Tracker Green CMFDA-labeled mouse apoptotic thymocytes were injected IV into Plg+/+ and Plg−/− mice. (A) Fluorescent microscopic images in duplicate (top and bottom panels are from 2 different Plg+/+ and 2 different Plg−/− mice) showing green-labeled apoptotic thymocytes trapped in the marginal zone of harvested spleens. Images with original magnification of ×20 were captured at room temperature under a Leica DMR upright microscope using an α Retiga EXi Cooled CCD camera and Image-Pro Plus software. The 4′,6 diamidino-2-phenylindole (blue) stains nuclei of splenic cells. Images are representative of 5 Plg+/+ and 5 Plg−/− mice. (B) Quantification of apoptotic thymocytes as areas of fluorescence in the spleens of Plg+/+ and Plg−/− mice. Bars are mean ± SD of average green fluorescence area per microscopic field. Three to 5 microscopic fields were counted from 5 mice per group. (C-D) Cell Tracker Green CMFDA-labeled apoptotic thymocytes were injected into the peritoneum of Plg+/+ or Plg−/− mice. Peritoneal cells were collected 1 hour postinjection and analyzed by flow cytometry. (C) A representative flow cytometry histogram comparing the fluorescence intensity of peritoneal lavage cells and showing the enhanced accumulation of thymocytes in Plg−/− mice compared with Plg+/+ mice. (D) Quantitative analysis of cells recovered from peritoneum of Plg+/+ or Plg−/− mice. Fluorescent cells with MFI are gated and MFI values derived from these cells are used in the calculation. Bars are mean ± SD of average green fluorescence (n = 3).

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