NoteThis protocol describes semi-automated cell counts using fluorescently labeled cells, a hemocytometer and ImageJ software. The hemocytometer is not needed if you have already calibrated the areas of images taken with your microscope and camera. Our setup automatically imports images in iPhoto and loads them into Photoshop with a double-click. However, you could also import and crop the images directly into ImageJ if you prefer.MaterialsCells in mediaEtOH1x P.I. (100 µg propidium iodide / mL PBS)HemocytometerU.V. fluorescent microscope with cameraComputer with ImageJ and image cropping software.ProcedureFix Cells by diluting them 50% in EtOH.1. To an eppendorf add 0.1 mL cells in PBS or media2. Add 0.1 mL of 100% EtOH while vortexing.3. Spin at 3,000 RPM x1 min.4. Aspirate off supernatant and respend cells in 0.1 mL of 1x P.I. Mix, incubate 2 min. Photograph cells on u.v. microscope5. Add 10 µL of stained cells to Hemocytometer.6. Place on U.V. microscope. (If the cells are too crowded then you may need to further dilute them in P.I. or PBS)7. Photograph 1 large square of hemocytometer with brightfield.8. Without moving the stage or changing the zoom, photograph the same area under u.v. light with red filter. Import and crop photo (e.g. using iPhoto and Photoshop)9. Import photos from the camera to the computer (e.g. with iPhoto). Double click an image to open image in Photoshop.10. In Photoshop, use the marquee tool measure the size of large square of the brightfield hemocytometer image.