In many cell types, voltage-gate Ca2+ channels in the plasma membrane trigger intracellular Ca2+ release via ryanodine receptors (RyRs) in the endoplasmic reticulum. In skeletal muscle, a specialized form of this signaling occurs such that CaV1.1 (the principle subunit of the muscle Ca channel, also referred to as the 2+ DHPR) activates RyR1 (the skeletal RyR isoform) via a conformational interaction. A long-term goal of our research is to identify the minimum set of proteins needed for this conformational interaction, and to determine their sites of interaction with one another. Based on previous work and our own preliminary results we know that in addition to CaV1.1 and RyR1, two other proteins are required: a ?Stac? adaptor protein and junctophilin. Varying isoforms of all four proteins (CaVs, RyRs, Stacs and junctophilins) are also expressed in the nervous system and CaVs, RyRs and junctophilins are expressed in heart. Significantly, mutations of CaVs, RyRs and junctophilins give rise to inherited, human disorders of skeletal muscle, heart and the nervous system. Clearly understanding the pathogenesis of such disorders would benefit from a better understanding of how these proteins interact with one another, and a major focus of the proposed experiments is to achieve this understanding. Toward this end, we have developed a number of experimental tools, including a construct encoding only the cytoplasmic domain of RyR1 (?RyR1cyto? containing RyR1 residues 1-4300 but lacking the ~700 C-terminal residues that form the ion conducting pore and anchor RyR1 in the sarcoplasmic reticulum). Additionally, we have established the ability to obtain high level expression of CaV1.1 in non-muscle cells. With these and other results demonstrating feasibility, we propose to use cDNA expression in muscle and non- muscle cells, followed by patch clamping, confocal fluorescence microscopy, biochemistry and electron microscopy to pursue the following specific aims.
Aim 1. To use expression in tsA201 cells to define the determinants for interactions between skeletal, cardiac and neuronal isoforms of the Stac proteins, the junctophilins, and RyRs.
Aim 2. To exploit the differential methodological strengths of tsA201 and muscle cells for probing the molecular determinants of signaling between CaV1.1 and RyR1. Myotubes will be used to test the Stac isoform specificity for support of EC coupling and to test the role of the DHPR ?1 subunit. tsA201 cells will be used to determine how mutations affect CaV1.1 gating charge movements, and myotubes to probe proximities among constituents of the EC coupling apparatus.
Aim 3. To determine whether CaV1.1-RyR1 functional interactions can be reconstituted in tsA201 cells, either partially with RyR1cyto or entirely with full-length RyR1.

Public Health Relevance

Skeletal muscle contraction, which is essential for the ability to move and breathe, is triggered by an electrical signal. This process, termed excitation-contraction coupling, depends on two key proteins: the dihydropyridine receptor (DHPR) which is located in the membrane surrounding the muscle cell, and the ryanodine receptor (RyR1) located inside the cell. Mutations of these proteins, and another muscle protein called Stac3, result in serious muscle diseases in humans, including hypokalemic periodic paralysis and central core disease. In this project, we will define how the DHPR, Stac3 and RyR1 interact with one another and why mutations cause these human muscle diseases.

Agency
National Institute of Health (NIH)
Institute
National Institute of Arthritis and Musculoskeletal and Skin Diseases (NIAMS)
Type
Research Project (R01)
Project #
5R01AR070298-04
Application #
9739080
Study Section
Biophysics of Neural Systems Study Section (BPNS)
Program Officer
Boyce, Amanda T
Project Start
2016-07-01
Project End
2021-06-30
Budget Start
2019-07-01
Budget End
2020-06-30
Support Year
4
Fiscal Year
2019
Total Cost
Indirect Cost
Name
University of Colorado Denver
Department
Physiology
Type
Schools of Medicine
DUNS #
041096314
City
Aurora
State
CO
Country
United States
Zip Code
80045
Polster, Alexander; Perni, Stefano; Filipova, Dilyana et al. (2018) Junctional trafficking and restoration of retrograde signaling by the cytoplasmic RyR1 domain. J Gen Physiol 150:293-306
Polster, Alexander; Dittmer, Philip J; Perni, Stefano et al. (2018) Stac Proteins Suppress Ca2+-Dependent Inactivation of Neuronal l-type Ca2+ Channels. J Neurosci 38:9215-9227
Polster, Alexander; Nelson, Benjamin R; Papadopoulos, Symeon et al. (2018) Stac proteins associate with the critical domain for excitation-contraction coupling in the II-III loop of CaV1.1. J Gen Physiol 150:613-624
Perni, Stefano; Lavorato, Manuela; Beam, Kurt G (2017) De novo reconstitution reveals the proteins required for skeletal muscle voltage-induced Ca2+ release. Proc Natl Acad Sci U S A 114:13822-13827
Polster, Alexander; Nelson, Benjamin R; Olson, Eric N et al. (2016) Stac3 has a direct role in skeletal muscle-type excitation-contraction coupling that is disrupted by a myopathy-causing mutation. Proc Natl Acad Sci U S A 113:10986-91