Abstract
Methods of cell preparation and quantitative flow cytometric cell sorting were developed for precise measurements of the incorporated radioactivity in cells labelled with [ 14C]-valine and fractionated as a function of their fluorescence intensity after staining with fluorescein-iso-thiocyanate (FITC). FITC fluorescence intensity of exponentially growing NHIK 3025 cells was found to be directly proportional to cellular protein content as measured by saturation-labelling with [ 14C]-valine. Protein synthesis as measured by 14C incorporation after pulse-labelling was found to increase nearly proportionally with cellular protein content. The deviations from proportionality were not greater than 6%, but yet found to be significant since the measurement error corresponded to only 2% standard deviation.
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