The Golgi-resident protease Kex2 acts in conjunction with Prm1 to facilitate cell fusion during yeast mating

doi:10.1083/jcb.200609182

Published online
doi:10.1083/jcb.200609182
The Journal of Cell Biology, Vol. 176, No. 2, 209-222
The Rockefeller University Press, 0021-9525 $30.00
© Heiman et al.

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The Golgi-resident protease Kex2 acts in conjunction with Prm1 to facilitate cell fusion during yeast mating

Maxwell G. Heiman, Alex Engel, and Peter Walter

¹ Howard Hughes Medical Institute and ² Department of Biochemistry and Biophysics, University of California, San Francisco, San Francisco, CA 94158

Correspondence to Peter Walter: pwalter{at}biochem.ucsf.edu

The molecular machines that mediate cell fusion are unknown.Previously, we identified a multispanning transmembrane protein,Prm1 (pheromone-regulated membrane protein 1), that acts duringyeast mating (Heiman, M.G., and P. Walter. 2000. J. Cell Biol.151:719–730). Without Prm1, a substantial fraction ofmating pairs arrest with their plasma membranes tightly apposedyet unfused. In this study, we show that lack of the Golgi-residentprotease Kex2 strongly enhances the cell fusion defect of Prm1-deficientmating pairs and causes a mild fusion defect in otherwise wild-typemating pairs. Lack of the Kex1 protease but not the Ste13 proteaseresults in similar defects. ${Delta}$ kex2 and ${Delta}$ kex1 fusion defects weresuppressed by osmotic support, a trait shared with mutants defectivein cell wall remodeling. In contrast, other cell wall mutantsdo not enhance the ${Delta}$ prm1 fusion defect. Electron microscopy of ${Delta}$ kex2-derived mating pairs revealed novel extracellular blebsat presumptive sites of fusion. Kex2 and Kex1 may promote cellfusion by proteolytically processing substrates that act inparallel to Prm1 as an alternative fusion machine, as cell wallcomponents, or both.

M.G. Heiman's present address is The Rockefeller University,New York, NY 10021.

Abbreviations used in this paper: PRM, pheromone-regulated membraneprotein; WT, wild type.

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