Actin‐mediated surface motility during sea urchin fertilization
- 1 January 1983
- journal article
- Published by Wiley in Cell Motility
- Vol. 3 (5), 513-524
- https://doi.org/10.1002/cm.970030518
Abstract
The sea urchin egg at fertilization is an ideal model in which to study actin‐mediated surface activity. Electron microscopy of unfertilized eggs demonstrates the presence of thousands of well‐arrayed short microvilli, which appear supported by cytochalasin‐sensitive actin oligomers as detected with rhodamine‐labeled phalloidin staining of permeabilized eggs. At insemination, the previously short microvilli elongate and cluster around the successful sperm during incorporation. Phalloidin staining demonstrates a tremendous recruitement of polymerized actin into the site of sperm incorporation, resulting in the formation of the fertilization cone. Fertilization of cytochalasin‐treated eggs results in the normal activation of the metabolic and bioeletric events, but sperm incorporation does not occur since the localized actin assembly required for fertilization cone formation is precluded. After sperm incorporation, the entire fertilized surface is restructured, as a result of a massive polymerization of actin to produce a burst in microvillar elongation. Addition of cytochalasin to eggs immediately following sperm incorporation demonstrates the recruitment of actin assembly for the proper progression through the first cell cycle. During normal cell divison, the egg surface retains the long microvilli. The furrow which forms at cytokinesis does not appear as a unique new structure, but rather as a reorganization of the cortical microfilaments. Quantitative fluorescence microscopy argues against an increase in microfilaments during early cytokinesis. At the latest stages of cytokinesis, a thickening of the cortical actin is noted, which could possibly be interpreted as a contractile ring. A minor basal level of actin assembly with numerous nucleation sites in unfertilized eggs and a tremendous but localized assembly of microfilaments surrounding the sperm during incorporation, followed by a massive global microfilament assembly event to elongate the fertilized egg microvilli resulting later in the reorganization of these microfilaments to produce the forces necessary for cytokinesis, highlight the utility of the study of sea urchin eggs at fertilization for understanding actin‐membrane interactions.Keywords
This publication has 30 references indexed in Scilit:
- Microtubule‐containing detergent‐extracted cytoskeletons in sea urchin eggs from fertilization through cell division: Antitubulin immunofluorescence microscopyCell Motility, 1983
- State of actin during the cycle of cohesiveness of the cytoplasm in parthenogenetically activated sea urchin eggExperimental Cell Research, 1982
- Anti-tubulin immunofluorescence microscopy of microtubules present during the pronuclear movements of sea urchin fertilizationDevelopmental Biology, 1981
- In vivo staining of cytoskeletal actin by autointernalization of nontoxic concentrations of nitrobenzoxadiazole-phallacidin.The Journal of cell biology, 1981
- IONIC TRIGGERS IN THE FERTILIZATION OF SEA URCHIN EGGSAnnals of the New York Academy of Sciences, 1980
- pH regulates the polymerization of actin in the sea urchin egg cortex.The Journal of cell biology, 1979
- Polarized bundles of actin filaments within microvilli of fertilized sea urchin eggs.The Journal of cell biology, 1977
- Changes in the topography of the sea urchin egg after fertilization.The Journal of cell biology, 1976
- The Site of Spermatozoon Entrance in the Unfertilized Egg of Discoglossus pictus (Anura): An Electron Microscope StudyBiology of Reproduction, 1975
- Methods for removal of the vitelline membrane of sea urchin eggs: I. Use of dithiothreitol (Cleland Reagent)Experimental Cell Research, 1970