Jean Claude Bernengo scite author profile

Jean Claude Bernengo

3Publications

97Citation Statements Received

70Citation Statements Given

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Affiliations

Claude Bernard University Lyon 1, Inserm, French National Centre for Scientific Research

Publications

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Measurements of Intracellular Mg2+ Concentration in Mouse Skeletal Muscle Fibers with the Fluorescent Indicator Mag-Indo-1

Csernoch

Bernengo

Szentesi

et al. 1998

Biophysical Journal

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Measurements of intracellular free magnesium concentration ([Mg2+]i) were performed on enzymatically isolated skeletal muscle fibers from mice, using the fluorescent ratiometric indicator mag-indo-1. An original procedure was developed to calibrate the dye response within the fibers: fibers were first permeabilized with saponin in the presence of a given extracellular magnesium concentration and were then embedded in silicone grease. The dye was then pressure microinjected into the saponin-permeabilized silicone-embedded fibers, and fluorescence was measured. The results show that for all tested [Mg2+], the value of the measured fluorescence ratio was higher than that found in aqueous solutions. Furthermore, the apparent binding curve that could be fit to the in vivo ratio data was shifted toward higher [Mg2+] by a factor of approximately 2. Using the in vivo calibration parameters, the mean resting [Mg2+]i was found to be 1.53 +/- 0.16 mM (n = 7). In an attempt to gain insight into the myoplasmic magnesium buffering capacity, we measured, together with mag-indo-1 fluorescence, the current elicited by the application of carbamylcholine (CCh) to the endplate of isolated fibers, in the presence of a high extracellular magnesium concentration. The results show that, under these conditions, a change in [Mg2+]i displaying a time course and amplitude qualitatively consistent with the CCh-induced inward current can be measured.

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Intracellular Ca2+ changes and Ca2+‐activated K+ channel activation induced by acetylcholine at the endplate of mouse skeletal muscle fibres.

Allard

Bernengo

Rougier

et al. 1996

The Journal of Physiology

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K+-rich external solution, using a pipette filled with Tyrode solution, external application of 0 1 mM ACh could induce a transient burst opening of channels carrying an outward current of an average amplitude of 4-6 + 0'2 pA at 0 mV (n = 8). 4. These channels were characterized as Ca2+-activated K+ channels. At 0 mV, in inside-out patches excised from the endplate membrane area, they displayed a conductance of 60 and 224 pS in the presence of Tyrode and K+-rich solution in the pipette, respectively. Halfmaximum activation was found for a [Ca2+]i close to 4 ,uM. The channels showed a typical voltage dependence. In outside-out patches these channels were shown to be blocked by 100 nM charybdotoxin (CTX). In fibres bathed in a Tyrode

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Photoacoustics as a tool for cutaneous permeation studies

Bernengo¹,

Gasquez²,

Falson-Rieg³

1998

High Temp.-High Press.

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