Fluorescence image cytometry for measurement of nuclear DNA content in surgical pathology

Abstract

A study was made on various methodological aspects of fluorescence image cytometry (FICM) for measurement of nuclear DNA content by using CCD cameras attached to an epifluorescence microscope. Cell nuclei of paraffin‐embedded specimens from mouse tissues and human prostate carcinomas were isolated and stained with 4′‐6‐diamidino‐2‐phenylindole (DAPI). We found that fluorescence fading, lamp stability, and the homogeneity of the illumination can easily be controlled. A camera with a signal‐to‐noise ratio of 53 dB gave a slightly more precise measurement than did a 46‐dB camera. The linearity of the analysis results was very good. The coefficient of variation of mouse kidney standard cells in the DNA histograms was about 5% and 7.4% in histograms of prostate carcinoma biopsies. Stained cell nuclei can be stored for long periods at −20°C without impairment of quality. Comparative measurements of ploidy by FICM and flow cytometry confirmed the accuracy of the FICM analyses. Thus, FICM appears to be an easy method for quantifying the DNA content of visually inspected cell nuclei in surgical pathology. © 1995 Wiley‐Liss, Inc.