Axial tubule junctions control rapid calcium signaling in atria
Sören Brandenburg, … , W. Jonathan Lederer, Stephan E. Lehnart
Sören Brandenburg, … , W. Jonathan Lederer, Stephan E. Lehnart
Published September 19, 2016
Citation Information: J Clin Invest. 2016;126(10):3999-4015. https://doi.org/10.1172/JCI88241.
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Research Article Cardiology Cell biology

Axial tubule junctions control rapid calcium signaling in atria

Abstract

The canonical atrial myocyte (AM) is characterized by sparse transverse tubule (TT) invaginations and slow intracellular Ca2+ propagation but exhibits rapid contractile activation that is susceptible to loss of function during hypertrophic remodeling. Here, we have identified a membrane structure and Ca2+-signaling complex that may enhance the speed of atrial contraction independently of phospholamban regulation. This axial couplon was observed in human and mouse atria and is composed of voluminous axial tubules (ATs) with extensive junctions to the sarcoplasmic reticulum (SR) that include ryanodine receptor 2 (RyR2) clusters. In mouse AM, AT structures triggered Ca2+ release from the SR approximately 2 times faster at the AM center than at the surface. Rapid Ca2+ release correlated with colocalization of highly phosphorylated RyR2 clusters at AT-SR junctions and earlier, more rapid shortening of central sarcomeres. In contrast, mice expressing phosphorylation-incompetent RyR2 displayed depressed AM sarcomere shortening and reduced in vivo atrial contractile function. Moreover, left atrial hypertrophy led to AT proliferation, with a marked increase in the highly phosphorylated RyR2-pS2808 cluster fraction, thereby maintaining cytosolic Ca2+ signaling despite decreases in RyR2 cluster density and RyR2 protein expression. AT couplon “super-hubs” thus underlie faster excitation-contraction coupling in health as well as hypertrophic compensatory adaptation and represent a structural and metabolic mechanism that may contribute to contractile dysfunction and arrhythmias.

Authors

Sören Brandenburg, Tobias Kohl, George S.B. Williams, Konstantin Gusev, Eva Wagner, Eva A. Rog-Zielinska, Elke Hebisch, Miroslav Dura, Michael Didié, Michael Gotthardt, Viacheslav O. Nikolaev, Gerd Hasenfuss, Peter Kohl, Christopher W. Ward, W. Jonathan Lederer, Stephan E. Lehnart

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Figure 2

ATs and junctions with RyR2 clusters are common in human tissue.

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ATs and junctions with RyR2 clusters are common in human tissue. Dual-co...
Dual-color STED nanoscopy of 2 human LA tissue sections coimmunostained for Cav3 and RyR2. (A) Tissue section shows AMs aligned with capillaries (asterisks indicate the lumens). Magnified images (of red boxed area) show 1 Cav3-labeled AT membrane structure (arrowhead), which intersects with 6 transversal rows of RyR2 clusters delimited by the surface membrane on top. Scale bars: overview 10 μm; magnifications, 2 μm. (B) Intracellular high-power magnifications showing 2 parallel, axially aligned RyR2 cluster tracks, perpendicularly intersecting 6 transversal RyR2 rows. Arrowheads identify exemplary RyR2 clusters with typical axial couplon architectures. RyR2 clusters with elongated axial morphologies and Cav3-labeled structures are tightly spaced next to each other, indicating a functional role of AT-associated SR junctions. STED images are representative of 5 human LA samples. Scale bar: 2 μm.