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THE PLANT CELL, Vol 1, Issue 1 53-63, Copyright © 1989 by American Society of Plant Biologists
Expression of a Chimeric Polygalacturonase Gene in Transgenic rin (Ripening Inhibitor) Tomato Fruit Results in Polyuronide Degradation but not Fruit Softening
J. J. Giovannoni, D. DellaPenna, A. B. Bennett and R. L. Fischer
Division of Molecular Plant Biology, University of California, Berkeley, California 94720
Tomato fruit ripening is accompanied by extensive degradation of pectic
cell wall components. This is thought to be due to the action of a single
enzyme, polygalacturonase, whose activity is controlled, at least in part,
at the level of gene expression. At the onset of tomato fruit ripening,
polygalacturonase enzyme activity, mRNA levels, and relative rate of gene
transcription all increase dramatically. To elucidate the role of
polygalacturonase during tomato fruit ripening, we utilized a pleiotropic
genetic mutation, rin, that blocks many aspects of ripening, including the
activation of polygalacturonase gene transcription. The polygalacturonase
structural gene was ligated to a promoter that is inducible in mature rin
fruit and inserted into the fruit genome, and plants were regenerated. This
allowed expression of the polygalacturonase gene in transgenic rin fruit at
a time corresponding to ripening in wild-type fruit. Expression of this
gene resulted in the accumulation of active polygalacturonase enzyme and
the degradation of cell wall polyuronides in transgenic rin fruit. However,
no significant effect on fruit softening, ethylene evolution, or color
development was detected. These results indicate that polygalacturonase is
the primary determinant of cell wall polyuronide degradation, but suggest
that this degradation is not sufficient for the induction of softening,
elevated rates of ethylene biosynthesis, or lycopene accumulation in rin
fruit.
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