Abstract

Our bodies are intricate ensembles of trillions of cells, and these building blocks are not generic like the bricks of a building, but rather are highly specialized. One characteristic of cells that distinguishes different types is their shape, from spherical, as in your circulating immune cells, to highly elongated, exemplified by the neurons that reach from our spines far into our legs. This project is aimed at understanding the mechanisms of cell shape change, which is crucial for many cell functions, including when a cell pinches into two after duplicating its contents. For 40 years, we have known that cell shape is maintained by some of the same cellular chemicals that cause our muscles to contract: actin, which forms long flexible polymers, and myosin, a biological motor that turns chemical energy into movement. Throughout these decades, substantial progress has been made in understanding how cells build actin polymers and turn on myosin motors, but less is known about how these essential events are attenuated. We reasoned that, just as the electronic governor on a heavy-duty truck limits its velocity, cells have ways of limiting actin-myosin work, to tune cell shape. In this project, we present several pieces of preliminary evidence of such cellular governors. We propose to determine the microscopic rearrangements that cause larger-scale cell shape changes, and define the chemicals that control these rearrangements. First, we demonstrate that the actin-myosin meshwork ring that pinches a cell in two does not go as fast as it can, but undergoes oscillations, speeding up and slowing down as it constricts. We routinely use powerful microscopes to observe living cells as they pinch in half, and measure the rearrangements that underlie these oscillations. Second, we will focus on the regulation of myosin, testing three distinct ideas about how its activity could be limited. Last, we present three new directions for the old field of studying cells pinching in half. To discover new candidate governors, we combined several technologies in ?fishing expedition? projects, which we have already completed. This unbiased but risky work laid well- substantiated groundwork for our functional studies of these new candidates. In sum, this project will take our field of cell pinching into novel territory, and will be relevant to the study of situations wherein cells purposefully arrest the pinching process, such as the generation of the specialized cells in your liver and heart muscle. Our findings will also contribute general principles of cell change shape, and thus help us understand normal development and diseases. Our discoveries may, in the long term, inform the development of therapies for pathologies involving cell shape regulation, such as cancers and blood diseases.

Public Health Relevance

Amy Shaub Maddox Project Narrative For a fertilized egg to become a person, or for tissues like the skin and digestive tract to be replenished due to wear and tear, cells must multiply. We are working to understand how one cell physically splits into two copies of itself. Knowing how cells normally multiply is key to treating cancer cells that grow abnormally, so our work will inform the development of anti-cancer drugs that target the tumor and not other tissues.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM102390-07
Application #
9389822
Study Section
Nuclear and Cytoplasmic Structure/Function and Dynamics Study Section (NCSD)
Program Officer
Gindhart, Joseph G
Project Start
2012-09-21
Project End
2021-08-31
Budget Start
2017-09-30
Budget End
2018-08-31
Support Year
7
Fiscal Year
2017
Total Cost
Indirect Cost

  Institution

Name
University of North Carolina Chapel Hill
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
608195277
City
Chapel Hill
State
NC
Country
United States
Zip Code
27599

  Publications

Descovich, Carlos Patino; Cortes, Daniel B; Ryan, Sean et al. (2018) Cross-linkers both drive and brake cytoskeletal remodeling and furrowing in cytokinesis. Mol Biol Cell 29:622-631
Fadero, Tanner C; Gerbich, Therese M; Rana, Kishan et al. (2018) LITE microscopy: Tilted light-sheet excitation of model organisms offers high resolution and low photobleaching. J Cell Biol 217:1869-1882
Lacroix, Benjamin; Letort, Gaëlle; Pitayu, Laras et al. (2018) Microtubule Dynamics Scale with Cell Size to Set Spindle Length and Assembly Timing. Dev Cell 45:496-511.e6
Rehain-Bell, Kathryn; Love, Andrew; Werner, Michael E et al. (2017) A Sterile 20 Family Kinase and Its Co-factor CCM-3 Regulate Contractile Ring Proteins on Germline Intercellular Bridges. Curr Biol 27:860-867
Ladouceur, A-M; Ranjan, Rajesh; Smith, Lydia et al. (2017) CENP-A and topoisomerase-II antagonistically affect chromosome length. J Cell Biol 216:2645-2655
Rehain, K; Green, R A; Bourdages, K G et al. (2017) Variations on a theme: Imaging cytokinetic and stable rings in situ using Caenorhabditis elegans. Methods Cell Biol 137:267-281
Dorn, Jonas F; Zhang, Li; Phi, Tan-Trao et al. (2016) A theoretical model of cytokinesis implicates feedback between membrane curvature and cytoskeletal organization in asymmetric cytokinetic furrowing. Mol Biol Cell 27:1286-99
Lacroix, Benjamin; Ryan, Joël; Dumont, Julien et al. (2016) Identification of microtubule growth deceleration and its regulation by conserved and novel proteins. Mol Biol Cell 27:1479-87
Rehain, Kathryn; Maddox, Amy Shaub (2015) Neuron migration: anillin protects leading edge actin. Curr Biol 25:R423-5
Sharif, Bedra; Fadero, Tanner; Maddox, Amy Shaub (2015) Anillin localization suggests distinct mechanisms of division plane specification in mouse oogenic meiosis I and II. Gene Expr Patterns 17:98-106

Showing the most recent 10 out of 13 publications