Abstract

): Cytosolic Ca2+, the primary mediator of smooth muscle cell contraction, is controlled through a combination of Ca2+ release from endoplasmic reticulum (ER) Ca2+ stores and entry of Ca2+ across the plasma membrane (PM). Although there are differences in the relative roles of these two Ca2+ sources among different smooth muscle subtypes, intracellular Ca2+ stores play a crucial role in controlling the generation of Ca2+ signals in response to activation of phospholipase C-coupled receptors. Despite their importance, Ca2+ stores remain poorly defined and elusive entities within smooth muscle cells as well as most nonmuscle cell types. The objective is to study the function and organization of Ca2+ stores and their intricate relationship with the PM in the generation of Ca2+ signals. A central hypothesis to be evaluated is that direct coupling between Ca2 about stores and the PM is required in the activation of Ca2+ entry signals. The studies utilize a combination of established smooth muscle cell lines, primary cultures of aortic smooth muscle cells, and transfected model cell systems to assess the following questions: 1. What is the Nature of the Coupling Between Ca2+ Stores and the Plasma Membrane? Much evidence indicates that direct interactions between Ca2+ stores and PM mediate receptor-activated Ca2+ signaling events. Our objective is to probe the molecular components involved in this interaction. The specific hypothesis to be tested is that the InsP3 receptor is a central component in mediating this interaction. The experimental approach is to assess the role of different subtypes and molecular domains of the InsP3 receptor in mediating the coupling between ER and PM to activate store-operated Ca2+ entry channels. Experiments will investigate the molecular targets of the InsP3 receptor including members of the ubiquitously expressed TRP (transient receptor potential) family of receptor-activated cation entry channels and their role in mediating Ca2+ entry in response to store-depletion. 2. How are Ca2+ Stores Functionally Organized in Smooth Muscle Cells? Studies indicate that Ca2+ stores are organized in an intricate, heterogeneous, and dynamic network within cells.
Our aim i s to use a combination of biochemical, molecular, and cellular imaging approaches to probe the functional organization of Ca2+ stores. Central within this aim is to test the hypothesis that functionally identifiable coupling occurs between specific Ca2+ stores and discrete areas of the PM to mediate the activation of Ca2+ entry channels. The approach is to investigate the cellular components involved in this coupling, including the exocytotic machinery mediating trafficking and docking, and the role of cytoskeletal elements. Functional studies will be complemented with high-resolution imaging to spatially localize Ca2+ stores and Ca2+ signaling events. The studies represent a cohesive combination of cell biological and molecular approaches to determining how Ca2+ stores function to generate cytosolic Ca2+ signals - key to controlling the contractile responses and proliferation of smooth muscle cells. The mechanisms by which Ca2+ signals are generated is essential to understanding and modifying major vascular diseases involving functional aberrations or changes in the proliferation of vascular smooth muscle cells.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL055426-09
Application #
6703745
Study Section
Cell Development and Function Integrated Review Group (CDF)
Program Officer
Goldman, Stephen
Project Start
1996-03-01
Project End
2007-02-28
Budget Start
2004-03-01
Budget End
2007-02-28
Support Year
9
Fiscal Year
2004
Total Cost
$334,125
Indirect Cost

  Institution

Name
University of Maryland Baltimore
Department
Biochemistry
Type
Schools of Medicine
DUNS #
188435911
City
Baltimore
State
MD
Country
United States
Zip Code
21201

  Publications

Li, Changlin; Li, Jing; Cai, Xiangyu et al. (2011) Protein kinase D3 is a pivotal activator of pathological cardiac hypertrophy by selectively increasing the expression of hypertrophic transcription factors. J Biol Chem 286:40782-91
Li, Changlin; Cai, Xiangyu; Sun, Haili et al. (2011) The ?A isoform of calmodulin kinase II mediates pathological cardiac hypertrophy by interfering with the HDAC4-MEF2 signaling pathway. Biochem Biophys Res Commun 409:125-30
Mancarella, Salvatore; Wang, Youjun; Gill, Donald L (2011) Signal transduction: STIM1 senses both Ca²+ and heat. Nat Chem Biol 7:344-5
Wang, Youjun; Deng, Xiaoxiang; Mancarella, Salvatore et al. (2010) The calcium store sensor, STIM1, reciprocally controls Orai and CaV1.2 channels. Science 330:105-9
Mancarella, Salvatore; Wang, Youjun; Gill, Donald L (2009) Calcium signals: STIM dynamics mediate spatially unique oscillations. Curr Biol 19:R950-2
Graham, Sarah J L; Black, Melony J; Soboloff, Jonathan et al. (2009) Stim1, an endoplasmic reticulum Ca2+ sensor, negatively regulates 3T3-L1 pre-adipocyte differentiation. Differentiation 77:239-47
Hewavitharana, Thamara; Deng, Xiaoxiang; Wang, Youjun et al. (2008) Location and function of STIM1 in the activation of Ca2+ entry signals. J Biol Chem 283:26252-62
Soboloff, J; Spassova, M; Hewavitharana, T et al. (2007) TRPC channels: integrators of multiple cellular signals. Handb Exp Pharmacol :575-91
Spassova, Maria A; Soboloff, Jonathan; He, Li-Ping et al. (2006) STIM1 has a plasma membrane role in the activation of store-operated Ca(2+) channels. Proc Natl Acad Sci U S A 103:4040-5
Spassova, Maria A; Hewavitharana, Thamara; Xu, Wen et al. (2006) A common mechanism underlies stretch activation and receptor activation of TRPC6 channels. Proc Natl Acad Sci U S A 103:16586-91

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