Visualization of exocytosis during sea urchin egg fertilization using confocal microscopy

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JOURNAL ARTICLES

Visualization of exocytosis during sea urchin egg fertilization using confocal microscopy

M Terasaki
Laboratory of Neurobiology, NINDS, NIH, Bethesda, MD 20892, USA.

A Ca2+ wave at fertilization triggers cortical granule exocytosis in sea urchin eggs. New methods for visualizing exocytosis of individual cortical granules were developed using fluorescent probes and confocal microscopy. Electron microscopy previously provided evidence that cortical granule exocytosis results in the formation of long-lived depressions in the cell surface. Fluorescent dextran or ovalbumin in the sea water seemed to label these depressions and appeared by confocal microscopy as disks. FM 1-43, a water-soluble fluorescent dye which labels membranes in contact with the sea water, seemed to label the membrane of these depressions and appeared as rings. In double-labeling experiments, the disk and ring labeling by the two types of fluorescent dyes were coincident to within 0.5 second. The fluorescent labeling is coincident with the disappearance of cortical granules by transmitted light microscopy, demonstrating that the labeling corresponds to cortical granule exocytosis. Fluorescent labeling was simultaneous with an expansion of the space occupied by the cortical granule, and labeling by the fluorescent dextran was found to take 0.1-0.2 second. These results are consistent with, and reinforce the previous electron microscopic evidence for, long-lived depressions formed by exocytosis; in addition, the new methods provide new ways to investigate cortical granule exocytosis in living eggs. The fluorescence labeling methods were used with the Ca2+ indicator Ca Green-dextran to test if Ca2+ and cortical granule exocytosis are closely related spatially and temporally. In any given region of the cortex, Ca2+ increased relatively slowly.(ABSTRACT TRUNCATED AT 250 WORDS)

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				A. Wemhoner, M. Frick, P. Dietl, P. Jennings, and T. Haller A Fluorescent Microplate Assay for Exocytosis in Alveolar Type II Cells J Biomol Screen, April 1, 2006; 11(3): 286 - 295. [Abstract] [PDF]

				A. M. Sokac and W. M. Bement Kiss-and-Coat and Compartment Mixing: Coupling Exocytosis to Signal Generation and Local Actin Assembly Mol. Biol. Cell, April 1, 2006; 17(4): 1495 - 1502. [Abstract] [Full Text] [PDF]

				A. C. Millard, M. Terasaki, and L. M. Loew Second Harmonic Imaging of Exocytosis at Fertilization Biophys. J., June 1, 2005; 88(6): L46 - L48. [Abstract] [Full Text] [PDF]

				E. Voronina and G. M. Wessel {beta}{gamma} subunits of heterotrimeric G-proteins contribute to Ca2+ release at fertilization in the sea urchin J. Cell Sci., December 1, 2004; 117(25): 5995 - 6005. [Abstract] [Full Text] [PDF]

				M. Terasaki, L. L. Runft, and A. R. Hand Changes in Organization of the Endoplasmic Reticulum during Xenopus Oocyte Maturation and Activation Mol. Biol. Cell, April 1, 2001; 12(4): 1103 - 1116. [Abstract] [Full Text]

				M. Nezuo, H. Shogomori, M. Hoshi, T. Yamamoto, T. Teshima, T. Shiba, and K. Chiba Developmental changes in localization of the main ganglioside during sea urchin embryogenesis Glycobiology, November 1, 2000; 10(11): 1243 - 1247. [Abstract] [Full Text] [PDF]

				D. Raucher and M. P. Sheetz Membrane Expansion Increases Endocytosis Rate during Mitosis J. Cell Biol., February 8, 1999; 144(3): 497 - 506. [Abstract] [Full Text] [PDF]

				K. Becker and N. Hart Reorganization of filamentous actin and myosin-II in zebrafish eggs correlates temporally and spatially with cortical granule exocytosis J. Cell Sci., January 1, 1999; 112(1): 97 - 110. [Abstract] [PDF]

				M. Terasaki Imaging of Echinoderm Fertilization Mol. Biol. Cell, July 1, 1998; 9(7): 1609 - 1612. [Full Text]

				G.-Q. Bi, R. L. Morris, G. Liao, J. M. Alderton, J. M. Scholey, and R. A. Steinhardt Kinesin- and Myosin-driven Steps of Vesicle Recruitment for Ca2+-regulated Exocytosis J. Cell Biol., September 8, 1997; 138(5): 999 - 1008. [Abstract] [Full Text] [PDF]