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Dive into the research topics where Ran Zalk is active.

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Featured researches published by Ran Zalk.


Journal of Biological Chemistry | 2017

Amyloid β production is regulated by β2-adrenergic signaling-mediated post-translational modifications of the ryanodine receptor

Renaud Bussiere; Alain Lacampagne; Steven Reiken; Xiaoping Liu; Valerie Scheuerman; Ran Zalk; Cécile Martin; Frédéric Checler; Andrew R. Marks; Mounia Chami

Alteration of ryanodine receptor (RyR)-mediated calcium (Ca2+) signaling has been reported in Alzheimer disease (AD) models. However, the molecular mechanisms underlying altered RyR-mediated intracellular Ca2+ release in AD remain to be fully elucidated. We report here that RyR2 undergoes post-translational modifications (phosphorylation, oxidation, and nitrosylation) in SH-SY5Y neuroblastoma cells expressing the β-amyloid precursor protein (βAPP) harboring the familial double Swedish mutations (APPswe). RyR2 macromolecular complex remodeling, characterized by depletion of the regulatory protein calstabin2, resulted in increased cytosolic Ca2+ levels and mitochondrial oxidative stress. We also report a functional interplay between amyloid β (Aβ), β-adrenergic signaling, and altered Ca2+ signaling via leaky RyR2 channels. Thus, post-translational modifications of RyR occur downstream of Aβ through a β2-adrenergic signaling cascade that activates PKA. RyR2 remodeling in turn enhances βAPP processing. Importantly, pharmacological stabilization of the binding of calstabin2 to RyR2 channels, which prevents Ca2+ leakage, or blocking the β2-adrenergic signaling cascade reduced βAPP processing and the production of Aβ in APPswe-expressing SH-SY5Y cells. We conclude that targeting RyR-mediated Ca2+ leakage may be a therapeutic approach to treat AD.


Proceedings of the National Academy of Sciences of the United States of America | 2018

Single-channel recordings of RyR1 at microsecond resolution in CMOS-suspended membranes

Andreas J.W. Hartel; Peijie Ong; Indra Schroeder; M. Hunter Giese; Siddharth Shekar; Oliver B. Clarke; Ran Zalk; Andrew R. Marks; Wayne A. Hendrickson; Kenneth L. Shepard

Significance We present a method for measuring the conductance of ion channels at bandwidths up to 500 kHz by fabricating lipid membranes directly on the surface of a custom amplifier chip. We apply this approach to the RyR1 receptor, enabling us to identify additional closed states for calcium-dependent inactivation at microsecond temporal resolutions. Additional data analysis using extended beta distributions allows us to detect gating events as short as 35 ns, a timescale that approaches that of single-file ion translocation. These measurement techniques hold the promise of reaching timescales for studying the kinetics of ion channels, achievable now only with computer-based molecular dynamics simulations. Single-channel recordings are widely used to explore functional properties of ion channels. Typically, such recordings are performed at bandwidths of less than 10 kHz because of signal-to-noise considerations, limiting the temporal resolution available for studying fast gating dynamics to greater than 100 µs. Here we present experimental methods that directly integrate suspended lipid bilayers with high-bandwidth, low-noise transimpedance amplifiers based on complementary metal-oxide-semiconductor (CMOS) integrated circuits (IC) technology to achieve bandwidths in excess of 500 kHz and microsecond temporal resolution. We use this CMOS-integrated bilayer system to study the type 1 ryanodine receptor (RyR1), a Ca2+-activated intracellular Ca2+-release channel located on the sarcoplasmic reticulum. We are able to distinguish multiple closed states not evident with lower bandwidth recordings, suggesting the presence of an additional Ca2+ binding site, distinct from the site responsible for activation. An extended beta distribution analysis of our high-bandwidth data can be used to infer closed state flicker events as fast as 35 ns. These events are in the range of single-file ion translocations.


Annual Review of Biochemistry | 2007

Modulation of the ryanodine receptor and intracellular calcium

Ran Zalk; Stephan E. Lehnart; Andrew R. Marks


Nature | 2015

Structure of a mammalian ryanodine receptor

Ran Zalk; Oliver B. Clarke; Amedee des Georges; Robert A. Grassucci; Steven Reiken; Filippo Mancia; Wayne A. Hendrickson; Joachim Frank; Andrew R. Marks


Cell Metabolism | 2011

Ryanodine Receptor Oxidation Causes Intracellular Calcium Leak and Muscle Weakness in Aging

Daniel C. Andersson; Matthew J. Betzenhauser; Steven Reiken; Albano C. Meli; Alisa Umanskaya; Wenjun Xie; Takayuki Shiomi; Ran Zalk; Alain Lacampagne; Andrew R. Marks


Cell | 2016

Structural Basis for Gating and Activation of RyR1.

Amedee des Georges; Oliver B. Clarke; Ran Zalk; Qi Yuan; Kendall J. Condon; Robert A. Grassucci; Wayne A. Hendrickson; Andrew R. Marks; Joachim Frank


Acta Neuropathologica | 2017

Post-translational remodeling of ryanodine receptor induces calcium leak leading to Alzheimer’s disease-like pathologies and cognitive deficits

Alain Lacampagne; Xiaoping Liu; Steven Reiken; Renaud Bussiere; Albano C. Meli; Inger Lauritzen; Andrew F. Teich; Ran Zalk; Nathalie Saint; Ottavio Arancio; Charlotte Bauer; Fabrice Duprat; Clark A. Briggs; Shreaya Chakroborty; Grace E. Stutzmann; Michael L. Shelanski; Frédéric Checler; Mounia Chami; Andrew R. Marks


Biophysical Journal | 2017

Functional Study of the Ryanodine Receptor Type 1 using Cryo-Electron Microscopy

Amedee des Georges; Oliver B. Clarke; Ran Zalk; Qi Yuan; Kendall J. Condon; Robert A. Grassucci; Wayne A. Hendrickson; Andrew R. Marks; Joachim Frank


Archive | 2016

Structure of rabbit RyR1 (EGTA-only dataset, class 1)

Oliver B. Clarke; A. des Georges; Ran Zalk; Andrew R. Marks; Wayne A. Hendrickson; Joachim Frank


Archive | 2016

Structure of rabbit RyR1 (Caffeine/ATP/Ca2+ dataset, class 1&2)

Oliver B. Clarke; A. des Georges; Ran Zalk; Andrew R. Marks; Wayne A. Hendrickson; Joachim Frank

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Albano C. Meli

University of Montpellier

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Amedee des Georges

City University of New York

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