Joshua N. Edwards scite author profile

Key pointsr Current methods do not allow a quantitative description of Ca 2+ movements across the tubular (t-) system membrane without isolating the membranes from their native skeletal muscle fibre.r Here we present a fluorescence-based method that allows determination of the t-system [Ca 2+ ] transients and derivation of t-system Ca 2+ fluxes in mechanically skinned skeletal muscle fibres. Differences in t-system Ca 2+ -handling properties between fast-and slow-twitch fibres from rat muscle are resolved for the first time using this new technique.r The method can be used to study Ca 2+ handling of the t-system and allows direct comparisons of t-system Ca 2+ transients and Ca 2+ fluxes between groups of fibres and fibres from different strains of animals. AbstractThe tubular (t-) system of skeletal muscle is an internalization of the plasma membrane that maintains a large Ca 2+ gradient and exchanges Ca 2+ between the extracellular and intracellular environments. Little is known of the Ca 2+ -handling properties of the t-system as the small Ca 2+ fluxes conducted are difficult to resolve with conventional methods. To advance knowledge in this area we calibrated t-system-trapped rhod-5N inside skinned fibres from rat and

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Toward the roles of store-operated Ca2+ entry in skeletal muscle

Launikonis

Murphy

Edwards

2010

Pflugers Arch - Eur J Physiol

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Store-operated Ca(2+) entry (SOCE) has been found to be a rapidly activated robust mechanism in skeletal muscle fibres. It is conducted across the junctional membranes by stromal interacting molecule 1 (STIM1) and Orai1, which are housed in the sarcoplasmic reticulum (SR) and tubular (t-) system, respectively. These molecules that conduct SOCE appear evenly distributed throughout the SR and t-system of skeletal muscle, allowing for rapid and local control in response to depletions of Ca(2+) from SR. The significant depletion of SR Ca(2+) required to reach the activation threshold for SOCE could only be achieved during prolonged bouts of excitation-contraction coupling (EC coupling) in a healthy skeletal muscle fibre, meaning that this mechanism is not responsible for refilling the SR with Ca(2+) during periods of fibre quiescence. While Ca(2+) in SR remains below the activation threshold for SOCE, a low-amplitude persistent Ca(2+) influx is provided to the junctional cleft. This article reviews the properties of SOCE in skeletal muscle and the proposed molecular mechanism, assesses its potential physiological roles during EC coupling, namely refilling the SR with Ca(2+) and simple balancing of Ca(2+) within the cell, and also proposes the possibility of SOCE as a potential regulator of t-system and SR membrane protein function.

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Cardiac alternans and intracellular calcium cycling

Edwards

Blatter

2014

Clin Exp Pharma Physio

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Cardiac alternans refers to a condition in which there is a periodic beat-to-beat oscillation in electrical activity and the strength of cardiac muscle contraction at a constant heart rate. Clinically, cardiac alternans occurs in settings that are typical for cardiac arrhythmias and has been causally linked to these conditions. At the cellular level, alternans is defined as beat-to-beat alternations in contraction amplitude (mechanical alternans), action potential duration (APD; electrical or APD alternans), and Ca2+ transient amplitude (Ca2+ alternans). The cause of alternans is multifactorial, however alternans always originate from disturbances of the bi-directional coupling between membrane voltage (Vm) and intracellular calcium ([Ca2+]i). Bi-directional coupling refers to the fact that in cardiac cells, Vm depolarization and the generation of action potentials cause the elevation of [Ca2+]i that is required for contraction (a process referred to as excitation-contraction coupling), the changes of [Ca2+]i on the other hand control Vm because important membrane currents are Ca2+-dependent. Evidence is mounting that alternans is ultimately caused by disturbances of cellular Ca2+ signaling. Here we review how two key factors of cardiac cellular Ca2+ cycling - the release of Ca2+ from internal stores and the capability of clearing the cytosol from Ca2+ after each beat - determine the conditions under which alternans occurs. The contributions from key Ca2+ handling proteins - surface membrane channels, ion pumps and transporters, and internal Ca2+ release channels - are discussed.

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O₂^•−production at 37°C plays a critical role in depressing tetanic force of isolated rat and mouse skeletal muscle

Edwards¹,

Macdonald²,

Poel³

et al. 2007

American Journal of Physiology-Cell Physiology

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To find out whether the decrease in muscle performance of isolated mammalian skeletal muscle associated with the increase in temperature toward physiological levels is related to the increase in muscle superoxide (O(2)(*-)) production, O(2)(*-) released extracellularly by intact isolated rat and mouse extensor digitorum longus (EDL) muscles was measured at 22, 32, and 37 degrees C in Krebs-Ringer solution, and tetanic force was measured in both preparations at 22 and 37 degrees C under the same conditions. The rate of O(2)(*-) production increased marginally when the temperature was increased from 22 to 32 degrees C, but increased fivefold when the temperature was increased from 22 to 37 degrees C in both rat and mouse preparations. This increase was accompanied by a marked decrease in tetanic force after 30 min incubation at 37 degrees C in both rat and mouse EDL muscles. Tetanic force remained largely depressed after return to 22 degrees C for up to 120 min. The specific maximum Ca(2+)-activated force measured in mechanically skinned fibers after the temperature treatment was markedly depressed in mouse fibers but was not significantly depressed in rat muscle fibers. The resting membrane and intracellular action potentials were, however, significantly affected by the temperature treatment in the rat fibers. The effects of the temperature treatment on tetanic force, maximum Ca(2+)-activated force, and membrane potential were largely prevented by 1 mM Tempol (4-hydroxy-2,2,6,6-tetramethylpiperidine-1-oxyl), a membrane-permeable superoxide dismutase mimetic, indicating that the increased O(2)(*-) production at physiological temperatures is largely responsible for the observed depression in tetanic force at 37 degrees C by affecting the contractile apparatus and plasma membrane.

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Activation and propagation of Ca²⁺ release from inside the sarcoplasmic reticulum network of mammalian skeletal muscle

Cully

Edwards

Launikonis

2014

The Journal of Physiology

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Skeletal muscle fibres are large and highly elongated cells specialized for producing the force required for posture and movement. The process of controlling the production of force within the muscle, known as excitation-contraction coupling, requires virtually simultaneous release of large amounts of Ca(2+) from the sarcoplasmic reticulum (SR) at the level of every sarcomere within the muscle fibre. Here we imaged Ca(2+) movements within the SR, tubular (t-) system and in the cytoplasm to observe that the SR of skeletal muscle is a connected network capable of allowing diffusion of Ca(2+) within its lumen to promote the propagation of Ca(2+) release throughout the fibre under conditions where inhibition of SR ryanodine receptors (RyRs) was reduced. Reduction of cytoplasmic [Mg(2+)] ([Mg(2+)]cyto) induced a leak of Ca(2+) through RyRs, causing a reduction in SR Ca(2+) buffering power argued to be due to a breakdown of SR calsequestrin polymers, leading to a local elevation of [Ca(2+)]SR. The local rise in [Ca(2+)]SR, an intra-SR Ca(2+) transient, induced a local diffusely rising [Ca(2+)]cyto. A prolonged Ca(2+) wave lasting tens of seconds or more was generated from these events. Ca(2+) waves were dependent on the diffusion of Ca(2+) within the lumen of the SR and ended as [Ca(2+)]SR dropped to low levels to inactivate RyRs. Inactivation of RyRs allowed re-accumulation of [Ca(2+)]SR and the activation of secondary Ca(2+) waves in the persistent presence of low [Mg(2+)]cyto if the threshold [Ca(2+)]SR for RyR opening could be reached. Secondary Ca(2+) waves occurred without an abrupt reduction in SR Ca(2+) buffering power. Ca(2+) release and wave propagation occurred in the absence of Ca(2+)-induced Ca(2+) release. These observations are consistent with the activation of Ca(2+) release through RyRs of lowered cytoplasmic inhibition by [Ca(2+)]SR or store overload-induced Ca(2+) release. Restitution of SR Ca(2+) buffering power to its initially high value required imposing normal resting ionic conditions in the cytoplasm, which re-imposed the normal resting inhibition on the RyRs, allowing [Ca(2+)]SR to return to endogenous levels without activation of store overload-induced Ca(2+) release. These results are discussed in the context of how pathophysiological Ca(2+) release such as that occurring in malignant hyperthermia can be generated.

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GIGANTEA is a component of a regulatory pathway determining wall ingrowth deposition in phloem parenchyma transfer cells of Arabidopsis thaliana

et al. 2010

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SUMMARYTransfer cells are specialised transport cells containing invaginated wall ingrowths that generate an amplified plasma membrane surface area with high densities of transporter proteins. They trans-differentiate from differentiated cells at sites at which enhanced rates of nutrient transport occur across apo/symplasmic boundaries. Despite their physiological importance, little is known of the molecular mechanisms regulating construction of their intricate wall ingrowths. We investigated the genetic control of wall ingrowth formation in phloem parenchyma transfer cells of leaf minor veins in Arabidopsis thaliana. Wall ingrowth development in these cells is substantially enhanced upon exposing plants to high-light or cold treatments. A hierarchical bioinformatic analysis of public microarray datasets derived from the leaves of plants subjected to these treatments identified GIGANTEA (GI) as one of 46 genes that are commonly up-regulated twofold or more under both high-light and cold conditions. Histological analysis of the GI mutants gi-2 and gi-3 showed that the amount of phloem parenchyma containing wall ingrowths was reduced 15-fold compared with wild-type. Discrete papillate wall ingrowths were formed in gi-2 plants but failed to develop into branched networks. Wall ingrowth development in gi-2 was not rescued by exposing these plants to high-light or cold conditions. In contrast, over-expression of GI in the gi-2 background restored wall ingrowth deposition to wild-type levels. These results indicate that GI regulates the ongoing development of wall ingrowth networks at a point downstream of inputs from environmental signals.

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Joshua N. Edwards

Ultra-rapid activation and deactivation of store-operated Ca2+ entry in skeletal muscle

Upregulation of store-operated Ca²⁺ entry in dystrophic mdx mouse muscle

A quantitative description of tubular system Ca²⁺ handling in fast‐ and slow‐twitch muscle fibres

Toward the roles of store-operated Ca2+ entry in skeletal muscle

Cardiac alternans and intracellular calcium cycling

O₂^•−production at 37°C plays a critical role in depressing tetanic force of isolated rat and mouse skeletal muscle

Activation and propagation of Ca²⁺ release from inside the sarcoplasmic reticulum network of mammalian skeletal muscle

GIGANTEA is a component of a regulatory pathway determining wall ingrowth deposition in phloem parenchyma transfer cells of Arabidopsis thaliana

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Joshua N. Edwards

Ultra-rapid activation and deactivation of store-operated Ca2+ entry in skeletal muscle

Upregulation of store-operated Ca2+ entry in dystrophic mdx mouse muscle

A quantitative description of tubular system Ca2+ handling in fast‐ and slow‐twitch muscle fibres

Toward the roles of store-operated Ca2+ entry in skeletal muscle

Cardiac alternans and intracellular calcium cycling

O2•−production at 37°C plays a critical role in depressing tetanic force of isolated rat and mouse skeletal muscle

Activation and propagation of Ca2+ release from inside the sarcoplasmic reticulum network of mammalian skeletal muscle

GIGANTEA is a component of a regulatory pathway determining wall ingrowth deposition in phloem parenchyma transfer cells of Arabidopsis thaliana

Contact Info

Product

Resources

About

Upregulation of store-operated Ca²⁺ entry in dystrophic mdx mouse muscle

A quantitative description of tubular system Ca²⁺ handling in fast‐ and slow‐twitch muscle fibres

O₂^•−production at 37°C plays a critical role in depressing tetanic force of isolated rat and mouse skeletal muscle

Activation and propagation of Ca²⁺ release from inside the sarcoplasmic reticulum network of mammalian skeletal muscle