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Flow cytometric characterization of the chlorophyll contents and size distributions of plant protoplasts
Author(s) -
Galbraith David W.,
Harkins Kristi R.,
Jefferson Richard A.
Publication year - 1988
Publication title -
cytometry
Language(s) - English
Resource type - Journals
eISSN - 1097-0320
pISSN - 0196-4763
DOI - 10.1002/cyto.990090112
Subject(s) - protoplast , autofluorescence , chlorophyll , chloroplast , flow cytometry , botany , biology , chlorophyll a , chlorophyll fluorescence , nicotiana tabacum , fluorescence , biophysics , microbiology and biotechnology , biochemistry , physics , optics , gene
We have employed flow cytometry for the characterization of populations of protoplasts prepared from tobacco ( Nicotiana tabacum ) leaf tissues. We first investigated the possibility of using flow cytometric analysis of the emission of chlorophyll autofluorescence for measurement of the chlorophyll contents of leaf protoplasts. Defined numbers of leaf protoplasts were sorted according to different, nonoverlapping windows placed on the one‐dimensional histograms of chlorophyll autofluorescence emission. The amounts of cellular chlorophyll were measured in cell‐free extracts of these sorted protoplasts using fluorometry. A high degree of correlation (r 2 = 0.983) was observed between these two parameters. We then examined the distribution of protoplast diameters in these protoplast populations through the use of pulse‐width time‐of‐flight (TOF) analysis. Through sorting of protoplasts using a series of narrow, nonoverlapping TOF windows, we were able to demonstrate that the TOF parameter was linearly correlated with protoplast diameter, over the range of 15–55 μm (r 2 > 0.99). We also compared the use of fluorescein diacetate (FDA) fluorochromasia and chlorophyll autofluorescence as the source of fluorescent signals for TOF analysis. We found that the presence of chloroplasts introduced distortions into the measurement of apparent size afforded by TOF analysis of FDA fluorochromasia. These results are discussed in terms of the application of techniques of flow analysis and sorting for the measurement of gene expression within the various different cell types found in plant tissues and organs.

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