Abstract

The major goal of mitosis is to distribute the genetic material accurately between the two daughter cells. Defects in meiosis or mitosis lead to aneuploidy, which is a significant cause of birth defects and is a hallmark of tumorigenesis. Proper spindle function relies on precise spatial and temporal control of microtubule (MT) dynamics and the integration of forces of motor proteins. Defects in regulated MT dynamics lead to spindle multi-polarity, improper kinetochore-MT attachments, delayed mitotic progression, and improper chromosome segregation. Despite the generation of an extensive parts list for the spindle, a major unanswered question is to understand how MT dynamics and motor protein activity are spatially and temporally regulated to ensure proper spindle architecture and function. This has been due, in part, to a lack of appropriate tools that could be used to relate key regulatory biochemical events to where those events are controlled spatially in the spindle. Our recent implementation of new FRET-based biosensors combined with FLIM and super resolution microscopy is now enabling us to address this important question. In this proposal we will: 1) Define how MT sliding is spatially modulated to control spindle organization by reconstituting MT sliding, and using FLIM imaging of novel intermolecular FRET reporters. These experiments will establish a paradigm for how the spatial control of motor activity contributes to the global organization of the spindle and will also define the critical features of XCTK2 that contribute to pole focusing and could be targeted for therapeutic development for treatment of tumors with centrosome amplification. 2) Define how Aurora B kinase modulates protein conformation, targeting, and function of the mitotic kinesin MCAK by testing how the CT of MCAK modulates conformation and activity. We will use Xenopus spindle assembly assays with various MCAK CT mutants and Fluorescence Lifetime Imaging of our MCAK biosensors to define where and when this conformational regulation occurs. This work will define spatial control mechanisms for the control of MCAK that will also serve as a model for regulation of protein activity by kinase networks. 3) Define how the integration of spatially distinct MT populations contributes to mitotic fidelity by testing the model that excess polymerization of non-kinetochore MTs increases mal-attached kinetochores and reduces mitotic fidelity. 3D-SIM super-resolution imaging of chromosome- MT interactions after kinesin knockdown will allow us to visualize how loss of these proteins lead to mal- oriented chromosomes. In vitro reconstitution assays using single molecule imaging and PALM/STORM will define how different MT dynamics regulators cooperatively control plus-end dynamics. Together these studies will bridge the gap in knowledge between how biochemical activities in vitro impact spindle structure and function in vivo.

Public Health Relevance

The faithful segregation of genetic material by the mitotic spindle to daughter cells is essential for the survival of an organism. The spindle is composed of microtubules and associated proteins that are utilized to attach the chromosomes to the spindle and to ensure their accurate segregation. Elucidating the mechanisms by which chromosomes are aligned and segregated will provide important insight into the accurate control of genomic fidelity, a process that goes awry in numerous proliferative diseases, such as cancer.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM059618-16
Application #
9132266
Study Section
Nuclear and Cytoplasmic Structure/Function and Dynamics Study Section (NCSD)
Program Officer
Deatherage, James F
Project Start
1999-08-01
Project End
2018-08-31
Budget Start
2016-09-01
Budget End
2017-08-31
Support Year
16
Fiscal Year
2016
Total Cost
Indirect Cost

  Institution

Name
Indiana University-Purdue University at Indianapolis
Department
Biochemistry
Type
Schools of Medicine
DUNS #
603007902
City
Indianapolis
State
IN
Country
United States
Zip Code
46202

  Publications

Huang, Yuejia; Li, Teng; Ems-McClung, Stephanie C et al. (2018) Aurora A activation in mitosis promoted by BuGZ. J Cell Biol 217:107-116
Bisson-Filho, Alexandre W; Hsu, Yen-Pang; Squyres, Georgia R et al. (2017) Treadmilling by FtsZ filaments drives peptidoglycan synthesis and bacterial cell division. Science 355:739-743
Zong, Hailing; Carnes, Stephanie K; Moe, Christina et al. (2016) The far C-terminus of MCAK regulates its conformation and spindle pole focusing. Mol Biol Cell 27:1451-64
Chen, Shengyao; Stout, Jane R; Dharmaiah, Sathiya et al. (2016) Transient endoreplication down-regulates the kinesin-14 HSET and contributes to genomic instability. Mol Biol Cell 27:2911-23
Walczak, Claire E; Zong, Hailing; Jain, Sachin et al. (2016) Spatial regulation of astral microtubule dynamics by Kif18B in PtK cells. Mol Biol Cell 27:3021-3030
Weaver, Lesley N; Ems-McClung, Stephanie C; Chen, Sez-Hon R et al. (2015) The Ran-GTP gradient spatially regulates XCTK2 in the spindle. Curr Biol 25:1509-14
Pannu, Vaishali; Rida, Padmashree C G; Ogden, Angela et al. (2015) HSET overexpression fuels tumor progression via centrosome clustering-independent mechanisms in breast cancer patients. Oncotarget 6:6076-91
Weaver, Lesley N; Walczak, Claire E (2015) Spatial gradients controlling spindle assembly. Biochem Soc Trans 43:7-12
Yount, Amber L; Zong, Hailing; Walczak, Claire E (2015) Regulatory mechanisms that control mitotic kinesins. Exp Cell Res 334:70-7
Huang, Rong; Oh, Hyunju; Arrendale, Allison et al. (2013) Intracellular targets for a phosphotyrosine peptidomimetic include the mitotic kinesin, MCAK. Biochem Pharmacol 86:597-611

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