Abstract

Signal transduction within the central nervous system involves the recognition of neurotransmitter or neuromodulator by a specific receptor and the subsequent activation (or inhibition) of a cellular event. These cellular events (ion translocation, neurotransmitter release etc.) are often mediated by second messengers, which are evoked as a result of receptor occupancy. This laboratory has been interested in the adenylate cyclase system for some time, and the proposed research represents an attempt to identify aspects of adenylate cyclase regulation which may be restricted to neural cells. One locus of this regulation is the ability of cytoskeletal components (specifically tubulin) to modify the adenylate cyclase system by direct transfer or GTP to the regulatory G proteins. The physical and biochemical link between tubulin and the adenylate cyclase system will be probed in a number of reconstitution studies. These studies will be performed on nitrocellulose or in phospholipid vesicles, and will test for physical interaction and/or nucleotide exchange between tubulin and G proteins. The former studies will be designed to determine the portion of the tubulin molecule responsible for the association with G proteins as well as the domains of tubulin responsible for nucleotide exchange. Specific antibodies, proteolytic digestion and synthetic peptides will be used to make these determinations. The hydrolysis resistant photoaffinity GTP analog, AAGTP will be used to probe the nucleotide exchange process between tubulin and G proteins as well as among G protein species. Physical interaction among G proteins (including tubulin) will be examined in membranes with the use of cross-linking agents, including a novel, nucleotide based crosslinker. The photoreceptor G protein system will be used to probe the kinetics of the nucleotide exchange process within a less complex system, and antibodies against a specific region of the photoreceptor G protein (transducin) will be used as well. If possible a newly discovered 32 KDa protein will be purified and characterized. Finally, the relevance of this protein, as well as G protein interaction and nucleotide exchange established in a permeable cell system. Greater understanding of the mechanisms whereby neurotransmitter signals are mediated will lead to a better understanding of human mental function and dysfunction.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Mental Health (NIMH)
Type
Research Project (R01)
Project #
2R01MH039595-05
Application #
3377469
Study Section
Neurosciences Research Review Committee (BPN)
Project Start
1984-12-01
Project End
1990-11-30
Budget Start
1989-02-01
Budget End
1989-11-30
Support Year
5
Fiscal Year
1989
Total Cost
Indirect Cost

  Institution

Name
University of Illinois at Chicago
Department
Type
Overall Medical
DUNS #
121911077
City
Chicago
State
IL
Country
United States
Zip Code
60612

  Publications

Cocchi, Massimo; Bernroider, G; Rasenick, Mark et al. (2017) Document of Trapani on animal consciousness and quantum brain function: A hypothesis. J Integr Neurosci 16:S99-S103
Schappi, Jeffrey M; Krbanjevic, Aleksandar; Rasenick, Mark M (2014) Tubulin, actin and heterotrimeric G proteins: coordination of signaling and structure. Biochim Biophys Acta 1838:674-81
Saengsawang, Witchuda; Rasenick, Mark M (2013) Heterotrimeric G proteins and microtubules. Methods Cell Biol 115:173-89
Davé, Rahul H; Saengsawang, Witchuda; Lopus, Manu et al. (2011) A molecular and structural mechanism for G protein-mediated microtubule destabilization. J Biol Chem 286:4319-28
Jarzynka, Michael J; Passey, Deepshikha K; Johnson, David A et al. (2009) Microtubules modulate melatonin receptors involved in phase-shifting circadian activity rhythms: in vitro and in vivo evidence. J Pineal Res 46:161-71
Allen, John A; Yu, Jiang Z; Dave, Rahul H et al. (2009) Caveolin-1 and lipid microdomains regulate Gs trafficking and attenuate Gs/adenylyl cyclase signaling. Mol Pharmacol 76:1082-93
Dave, Rahul H; Saengsawang, Witchuda; Yu, Jiang-Zhou et al. (2009) Heterotrimeric G-proteins interact directly with cytoskeletal components to modify microtubule-dependent cellular processes. Neurosignals 17:100-8
Roychowdhury, Sukla; Rasenick, Mark M (2008) Submembraneous microtubule cytoskeleton: regulation of microtubule assembly by heterotrimeric Gproteins. FEBS J 275:4654-63
Donati, Robert J; Dwivedi, Yogesh; Roberts, Rosalinda C et al. (2008) Postmortem brain tissue of depressed suicides reveals increased Gs alpha localization in lipid raft domains where it is less likely to activate adenylyl cyclase. J Neurosci 28:3042-50
Layden, Brian T; Saengsawang, Witchuda; Donati, Robert J et al. (2008) Structural model of a complex between the heterotrimeric G protein, Gsalpha, and tubulin. Biochim Biophys Acta 1783:964-73

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