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PLANT PHYSIOLOGY , Vol 113, Issue 1 269-279, Copyright © 1997 by American Society of Plant Biologists
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GENE REGULATION AND MOLECULAR GENETICS |
Activation of Plant Plasma Membrane Ca2+-Permeable Channels by Race-Specific Fungal Elicitors
A. Gelli, V. J. Higgins and E. Blumwald
Department of Botany, University of Toronto, 25 Willcocks Sreet, Toronto, Ontario, Canada M5S 3B2
The response of plant cells to invading pathogens is regulated by
fluctuations in cytosolic Ca2+ levels that are mediated by Ca2+-permeable
channels located at the plasma membrane of the host cell. The mechanisms by
which fungal elicitors can induce Ca2+ uptake by the host cell were
examined by the application of conventional patch-clamp techniques.
Whole-cell and single-channel experiments on tomato (Lycopersicon
esculentum L.) protoplasts revealed a race-specific fungal elicitor-induced
activation of a plasma membrane Ca2+-permeable channel. The presence of the
fungal elicitor resulted in a greater probability of channel opening.
Guanosine 5[prime]-[[beta]-thio]diphosphate, a GDP analog that locks
heterotrimeric G-proteins into their inactivated state, abolished the
channel activation induced by the fungal elicitor, whereas guanosine
5[prime][[gamma]-thio]triphosphate, a nonhydrolyzable GTP analog that locks
heterotrimeric G-proteins into their activated state, produced an effect
similar to that observed with the fungal elicitor. Mastoparan, which
stimulates GTPase activity, mimicked the effect of GTP[[gamma]]S. The
addition of HA1004 (a protein kinase inhibitor) in the presence of the
elicitor totally abolished channel activity, whereas okadaic acid (a
protein phosphatase inhibitor) moderately enhanced channel activity,
suggesting that the activation of the channel by fungal elicitors is
modulated by a heterotrimeric G-protein-dependent phosphorylation of the
channel protein.
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