Publication | Open Access
Ca<sup>2+</sup>, Annexins, and GTP Modulate Exocytosis from Maize Root Cap Protoplasts
156
Citations
35
References
1998
Year
Plant PhysiologyBotanyGlycobiologyCytoskeletonRoot Cap CellsCellular PhysiologyPlant DevelopmentPlant Molecular BiologyCell CapacitancePlant CytologyCell PhysiologyPlant BiologyBiochemistryCell BiologyCell WallBiologyDevelopmental BiologyNatural SciencesGtp Modulate ExocytosisPlant Cell CultureMedicineCa2+ BuffersExtracellular Matrix
Protoplasts isolated from root cap cells of maize were shown to secrete fucose-rich polysaccharides and were used in a patch-clamp study to monitor changes in whole-cell capacitance. Ca2+ was required for exocytosis, which was measured as an increase in cell capacitance during intracellular dialysis with Ca2+ buffers via the patch pipette. Exocytosis was stimulated significantly by small increases above normal resting [Ca2+]. In the absence of Ca2+, protoplasts decreased in size. In situ hybridization showed significant expression of the maize annexin p35 in root cap cells, differ-entiating vascular tissue, and elongating cells. Dialysis of protoplasts with maize annexins stimulated exocytosis at physiological [Ca2+], and this could be blocked by dialysis with antibodies specific to maize annexins. Dialysis with milli-molar concentrations of GTP strongly inhibited exocytosis, causing protoplasts to decrease in size. GTPgammaS and GDPbetaS both caused only a slight inhibition of exocytosis at physiological Ca2+. Protoplasts were shown to internalize plasma membrane actively. The results are discussed in relation to the regulation of exocytosis in what is usually considered to be a constitutively secreting system; they provide direct evidence for a role of annexins in exocytosis in plant cells.
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