Abstract

Alpha-granules, the major secretory organelle of platelets, contain hundreds of proteins that are released upon activation. Interestingly, many of the stored proteins have seemingly opposite function, such as those with pro- or anti-angiogenic properties. A major unanswered question in platelet physiology is: Are platelets an active participant specifically releasing context-appropriate material from their -granules or are they random delivery devises? Here we address important aspects of that central question through three Specific Aims.
Specific Aim 1 : To test the hypothesis that human platelets contain a single major -granule population in which individual cargo proteins are packaged into distinct zones. Through the combined application of electron tomography, immunogold labeling, and super-resolution light microscopy, we will analyze a whole platelet both with respect to granule structure and protein distribution. Using these structural approaches, we will determine the extent of homogeneity, or heterogeneity, in structure and cargo protein distribution in the human -granule population.
Specific Aim 2 : To test the hypothesis that specialized -granule subdomains/extensions provide a spatial basis for differential membrane fusion/protein secretion to the plasma membrane/OCS in response to agonists. In this Aim, we apply the imaging approaches, from Aim 1, to characterize the structural basis on which platelet -granule secretion can support differential protein release. Our data and that of others suggest that differential release is a normal outcome of -granule secretion. To date, our Preliminary Data are consistent with a model in which important fusion machinery proteins such as the v- SNARE, VAMP-8, are concentrated over distinct subdomains of the -granule and hence may mediate subdomain specific fusion. Mouse platelets from gene knockouts will be facilitate experiments designed to reveal the accumulation of intermediates in granule release.
Specific Aim 3 : To test the hypothesis that VWF and/or cytoskeletal elements provides an organizing principle for platelet -granule structure and function. Reversible depolymerization of granule VWF has the therapeutic potential to modulate -granule secretion through affecting protein zoning and granule shape. The proposed research is both significant and innovative. Our overarching hypothesis of a granule organized structurally into specific subdomains designed for agonist-responsive secretion provides an innovative intellectual framework that drives experiments towards incisive answers. This framework can lead to revealing answers that would not come otherwise. Our experience in high-resolution imaging technology brings a novel toolset to the platelet field needed to definitively answer the central question raised. Our work will provide a reference framework for future therapeutic design.

Public Health Relevance

The proposed research will have a lasting impact because it provides answers to problems central to thrombosis and vascular health. We address the question: Are platelets an active participant specifically releasing context appropriate material from their ?-granules or are they random delivery devices? Our experimental answer to this question gives a framework for the development of new therapeutic approaches to bleeding, stroke and other vascular diseases.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
4R01HL119393-04
Application #
9068338
Study Section
Hemostasis and Thrombosis Study Section (HT)
Program Officer
Sarkar, Rita
Project Start
2013-08-01
Project End
2017-05-31
Budget Start
2016-06-01
Budget End
2017-05-31
Support Year
4
Fiscal Year
2016
Total Cost
Indirect Cost

  Institution

Name
University of Arkansas for Medical Sciences
Department
Physiology
Type
Schools of Medicine
DUNS #
122452563
City
Little Rock
State
AR
Country
United States
Zip Code
72205

  Publications

Joshi, Smita; Banerjee, Meenakshi; Zhang, Jinchao et al. (2018) Alterations in platelet secretion differentially affect thrombosis and hemostasis. Blood Adv 2:2187-2198
Pokrovskaya, Irina D; Joshi, Smita; Tobin, Michael et al. (2018) SNARE-dependent membrane fusion initiates ?-granule matrix decondensation in mouse platelets. Blood Adv 2:2947-2958
Yadav, Shilpi; Storrie, Brian (2017) The cellular basis of platelet secretion: Emerging structure/function relationships. Platelets 28:108-118
Yadav, Shilpi; Williamson, Jonathan K; Aronova, Maria A et al. (2017) Golgi proteins in circulating human platelets are distributed across non-stacked, scattered structures. Platelets 28:400-408
Storrie, Brian; Whiteheart, Sidney W (2017) Editorial: Platelet Secretion. Platelets 28:107
Banerjee, Meenakshi; Joshi, Smita; Zhang, Jinchao et al. (2017) Cellubrevin/vesicle-associated membrane protein-3-mediated endocytosis and trafficking regulate platelet functions. Blood 130:2872-2883
Kamykowski, Jeffrey A; Storrie, Brian (2017) Managing the Introduction of Super-Resolution Microscopy into a Core Facility. Methods Mol Biol 1663:15-19
Pokrovskaya, I D; Aronova, M A; Kamykowski, J A et al. (2016) STEM tomography reveals that the canalicular system and ?-granules remain separate compartments during early secretion stages in blood platelets. J Thromb Haemost 14:572-84
MacDonald, Laura; Baldini, Giulia; Storrie, Brian (2015) Does super-resolution fluorescence microscopy obsolete previous microscopic approaches to protein co-localization? Methods Mol Biol 1270:255-75
Storrie, Brian (2015) Defective platelet autocrine signaling in HPS. Blood 125:1515-6

Showing the most recent 10 out of 11 publications