CSM News Electronic Edition Volume 4, number 9 March 11, 1995 Please submit abstracts of your papers as soon as they have been accepted for publication by sending them to CSM-News@worms.cmsbio.nwu.edu. Back issues of CSM-News, the CSM Reference database and other useful information is available by anonymous ftp from worms.cmsbio.nwu.edu [165.124.233.50], via Gopher at the same address, or by World Wide Web at the URL "http://worms.cmsbio.nwu.edu/dicty.html" =============== Announcements =============== Dietmar Manstein has deposited the sequences of several new and potentially useful Dicty vectors with the archive. These sequences are available in the directory /pub/dicty/Vector_Sequences =========== Abstracts =========== OVEREXPRESSION OF MYOSIN MOTOR DOMAINS IN DICTYOSTELIUM DISCOIDEUM: SCREENING OF TRANSFORMANTS AND PURIFICATION OF THE AFFINITY TAGGED PROTEIN Dietmar J. Manstein and Deborah M. Hunt National Institute for Medical Research, The Ridgeway, Mill Hill, London NW7 1AA, U.K. Journal of Muscle Research and Cell Motility, in press Summary The eukaryotic organism Dictyostelium discoideum has become one of the organisms of choice for the over-expression of recombinant myosins and myosin fragments. Here, we describe a protocol that facilitates the screening of cells that have been transformed with myosin expression constructs and allows the rapid purification of recombinant myosins. Depletion of cellular ATP is used to recruit most of the endogenous and recombinant myosin into a rigor-like complex with actin. Following cell lysis the insoluble actomyosin complex is precipitated by centrifugation, washed, and Mg2+-ATP is added to extract the recombinant protein from the pellet. More than 90% of the protein in the resulting supernatant corresponds to actin, myosin, and the recombinant myosin fragments. Therefore, it is easy to detect any differences in expression level between individual myosin constructs on SDS-polyacrylamide gels. Additionally, the dependence of expression on external factors, such as cell density, can be readily determined. Furthermore, the presence of a band corresponding to the recombinant protein indicates that the overexpressed protein has at least some of the functional properties that are characteristic for a myosin motor. This rapid and selective extraction protocol can also be utilised to facilitate the purification of recombinant myosin motors on a preparative scale and has proved particularly useful in the purification of myosin head fragments, that are tagged with histidine residues, by Ni2+-chelate chromatography. ----------------------------------------------------------------------- Amoeboid gametes and fertilization in Dictyostelium: Gamete and pronuclear fusion are mediated by calmodulin and its binding proteins Danton H. O'Day, Keith E. Lewis, Michael A. Lydan Department of Zoology, University of Toronto, Erindale College, 3359 Mississauga Road, Mississauga, ON L5L 1C6 CANADA In: Advances in Spermatozoal Taxonomy and Phylogeny. B.G.M. Jamieson, J. Ausio & J.-L. Justine (Editors), Memoires du Museum National d'Histoire Naturelle, Paris (1995) Abstract The gametes of Dictyostelium discoideum are tiny amoeboid cells which contain a small condensed nucleus. Gamete formation is calcium-independent and inhibited by calmodulin function. Accumulated data suggests that the gametes are a source of sexual pheromone that promotes sexual cell fusion. Time-lapse videomicroscopy has revealed that gametes are highly motile compared to non-gametic cells and, when two gametes contact, fusion results in the formation of a binucleate cell. Within each binucleate, pronuclear migration, swelling and fusion occur as the cytoplasmic volume of the cell increases dramatically producing a zygote giant cell. Gamete fusion is calcium-dependent and involves at least one membrane-bound, GlycNAc-containing glycoprotein (gp138). Fertilization is mediated by the dual signal transduction pathway involving calcium and protein kinase C. Of particular importance is the downstream role of calmodulin (CaM) and its binding proteins (CaMBPs). A putative CaM Kinase III activity and two, as yet unidentified CaMBPs (i.e., CaMBP-48, CAMBP-91) are developmentally regulated and temporally associated with the events of cell and pronuclear fusion in D. discoideum. Fertilization is terminated by a feed-back mechanism involving an autoinhibitor that is secreted by the zygote giant cells. This low molecular weight, hydrophoic, heat-stable autoinhibitor inhibits both cell and pronuclear fusion by preventing the interaction of CaM with its binding proteins. These results are discussed in terms of fertilization and signal transduction involving calmodulin and its binding proteins in higher animals. ------------------------------------------------------------------------ [End CSM News, volume 4, number 9]