Abstract

We are using the giant single cell of the early Drosophila embryo (500 um x 150 um) as a model system in which to examine the biochemical basis for selected aspects of cytoplasmic organization. An understanding of the highly organized cytoplasm in this unusual cell will be required to understand the spatially patterned cell determination processes that underlie its development into a complex multicellular organism. Our approach centers on a study of the cytoskeletal proteins that organize the syncytial cytoplasm. The cytoskeleton is very complicated, and our major goal is to analyze the function of a few of the major multiprotein complexes involved in molecular detail. We also wish to develop methods for identifying and isolating more minor cytoskeletal proteins that are suspected to localize selected mRNAs (such as bicoid mRNA) or proteins to specific regions of the egg cortex. Most of our research plans begin by exploiting two affinity chromatography procedures that have taken us several years to develop to a satisfactory state: actin filament-affinity chromatography and microtubule-affinity chromatography. These procedures have been validated by experiments with known proteins that bind to actin filaments and microtubules. When used to fractionate extracts of early (pre-gastrula) Drosophila embryos, they enable more than 40 (actin filament columns) and 60 (micro- tubule columns) different proteins to be selected and purified. The antibodies that have thus far been produced to these proteins and used to stain embryos suggest that most of the proteins isolated by affinity chromatography are associated with their respective cytoskeletal network (actin filament or microtubule) inside the cell. The main problem now is to make a wise selection of individual proteins to purify to homogeneity and study in detail. This selection is being made after considering the results of cytological localizations, antibody injections into embryos to block function, and biochemical fractionation that identify protein complexes and activities. We have thus far selected for detailed study a 205 kilodalton microtubule-binding protein that is released from microtubules with ATP and localizes to centrosomes, and a 230 kilodalton actin-binding protein whose monoclonal antibody interferes with nuclear spacing when injected into Drosophila embryos. In addition, we have been purifying to homogeneity several intermediate filament-type proteins that are present in large amounts in the syncytial stage embryo.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM023928-12
Application #
3271966
Study Section
Molecular Cytology Study Section (CTY)
Project Start
1977-08-01
Project End
1993-06-30
Budget Start
1989-07-01
Budget End
1990-06-30
Support Year
12
Fiscal Year
1989
Total Cost
Indirect Cost

  Institution

Name
University of California San Francisco
Department
Type
Schools of Medicine
DUNS #
073133571
City
San Francisco
State
CA
Country
United States
Zip Code
94143

  Publications

Liu, Ling; Su, Xiaoyang; Quinn 3rd, William J et al. (2018) Quantitative Analysis of NAD Synthesis-Breakdown Fluxes. Cell Metab 27:1067-1080.e5
Groen, Aaron C; Mitchison, Timothy J (2016) Purification and Fluorescent Labeling of Tubulin from Xenopus laevis Egg Extracts. Methods Mol Biol 1413:35-45
Özlü, Nurhan; Qureshi, Mohammad H; Toyoda, Yusuke et al. (2015) Quantitative comparison of a human cancer cell surface proteome between interphase and mitosis. EMBO J 34:251-65
Coughlin, Margaret; Groen, Aaron C; Mitchison, Timothy J (2014) Electron microscopy of microtubule cytoskeleton assembly in vitro. Methods Mol Biol 1117:259-71
Mitchison, Timothy J; Nguyen, Phuong; Coughlin, Margaret et al. (2013) Self-organization of stabilized microtubules by both spindle and midzone mechanisms in Xenopus egg cytosol. Mol Biol Cell 24:1559-73
Kueh, Hao Yuan; Niethammer, Philipp; Mitchison, Timothy J (2013) Maintenance of mitochondrial oxygen homeostasis by cosubstrate compensation. Biophys J 104:1338-48
Hu, Chi-Kuo; Ozlu, Nurhan; Coughlin, Margaret et al. (2012) Plk1 negatively regulates PRC1 to prevent premature midzone formation before cytokinesis. Mol Biol Cell 23:2702-11
Hu, Chi-Kuo; Coughlin, Margaret; Mitchison, Timothy J (2012) Midbody assembly and its regulation during cytokinesis. Mol Biol Cell 23:1024-34
Zhang, Xin; Wang, Wenchao; Bedigian, Anne V et al. (2012) Dopamine receptor D3 regulates endocytic sorting by a Prazosin-sensitive interaction with the coatomer COPI. Proc Natl Acad Sci U S A 109:12485-90
Maiuri, Paolo; Terriac, Emmanuel; Paul-Gilloteaux, Perrine et al. (2012) The first World Cell Race. Curr Biol 22:R673-5

Showing the most recent 10 out of 70 publications