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The Journal of Neuroscience, April 11, 2007, 27(15):4008-4013; doi:10.1523/JNEUROSCI.3278-06.2007
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Brief Communications
Actin Filaments Mediate Mechanical Gating during Osmosensory Transduction in Rat Supraoptic Nucleus Neurons
Zizhen Zhang, Alexandra N. Kindrat, Reza Sharif-Naeini, andCharles W. Bourque Centre for Research in Neuroscience, Montreal General Hospital and McGill University, Montreal, Quebec, Canada H3G 1A4
Abstract
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Abstract
Introduction
Osmosensory transduction is a bidirectional process displayed by neurons involved in the control of thirst and antidiuretic hormone release, and is therefore crucial for body fluid homeostasis. Although this mechanism is known to involve the activation of nonselective cation channels during hypertonicity-evoked shrinking, and the inhibition of these channels during hypotonicity-evoked swelling, the basis for this regulation is unknown. Here, we investigated this process using whole-cell patch-clamp recordings from neurons acutely isolated from the supraoptic nucleus of adult rats. The mechanosensitivity index, defined as the ratio of conductance change to normalized volume change, was quantitatively equivalent whether cell volume was increased or decreased by changes in extracellular fluid osmolality, or by changes in pipette pressure. Moreover, responses induced by hyperosmotic or hypo-osmotic media could be reversed by increasing or decreasing pipette pressure, respectively. The mechanosensitivity index was significantly reduced in neurons treated with cytochalasin-D, a compound that promotes the depolymerization of actin filaments. Conversely, cells treated with jasplakinolide, a compound that promotes actin polymerization, showed a significant increase in mechanosensitivity index. Finally, the depolarizing and excitatory effects of hypertonic stimuli were significantly enhanced by jasplakinolide and reduced by cytochalasin-D. We conclude that osmosensory transduction in these neurons is a reversible mechanical process that depends on an intact actin cytoskeleton, and the sensitivity of the transducer appears to vary in proportion with the density of actin filaments.
Key words: hypothalamus; supraoptic nucleus; electrophysiology; osmoreceptor; actin cytoskeleton; vasopressin
Introduction
Osmosensory neurons in the CNS of mammals detect changes in plasma osmolality caused by temporal differences in the intake or loss of salt and water. In vivo, the electrical activity of these neurons is generally increased by hyperosmolality and inhibited by hypo-osmolality (Bourque et al., 1994), and information encoded by these responses modulates thirst and antidiuretic hormone release to promote hydromineral balance (Denton et al., 1996
Materials and Methods
Preparation and perfusion of isolated cells. MNCs were acutely isolated from adult (100–200 g) male Long–Evans rats as reported previously (Zhang and Bourque, 20031 mm3) containing the SON were then cut and incubated for 90 min in oxygenated PIPES solution (33.5 °C), pH 7.0, containing 0.7 mg/ml trypsin (type XI; Sigma, St. Louis, MO). Blocks were transferred to a trypsin-free PIPES solution, pH 7.4 (22°C), and dispersed as required. Cell suspensions were plated onto plastic Petri dishes and used within 30–120 min. Dishes were mounted on an inverted phase contrast microscope (Diaphot; Nikon, Tokyo, Japan) and perfused with a HEPES-buffered saline containing (in mM) 75 Na2SO4, 3 KCl, 1 MgCl2, 10 HEPES, 1 CaCl2, and 10 glucose. Different amounts of mannitol were added to adjust osmolality. Osmotic steps were applied using a gravity system delivering solutions at a rate of 1.0–1.2 ml/min–1. A fast stepper device (SF-77B; Warner Instruments, Hamden, CT) was used to switch between the adjacent barrels of a three-barrel glass assembly to minimize time lag (<20 ms) when changing solutions. Excess solution was sucked away through a vacuum system.
Measurements of relative cell volume. We determined relative changes in cell volume from measurements of maximal cross-sectional area (CSA; from digitized images) (Zhang and Bourque, 2003
Electrophysiological recording. Cells were patch clamped with glass pipettes (1.2 mm outer diameter glass; A-M Systems, Carlsborg, WA) containing a solution, pH 7.2, comprising (in mM) 120 K gluconate, 10 HEPES, 1 MgCl2, and 1 EGTA. Whole-cell recordings were performed using an Axopatch-1D amplifier (Molecular Devices, Union City, CA). Pipette pressure was monitored via a digital pressure transducer (model PM015D; World Precision Instruments, Sarasota, FL) and controlled via an air-filled syringe. Changes in volume caused by given changes in pipette pressure differed significantly from cell to cell and, generally, varied as a sensitive and inverse function of pipette resistance (i.e., tip diameter). Membrane current (direct current, –2 kHz) was digitized (10 kHz) via a digidata 1200B interface coupled to a computer running Clampex 8 (Molecular Devices). Whole-cell capacitance and series resistance were compensated electronically. Voltage ramps (–100–0 mV; 20 mV/s) were commanded to determine steady-state whole-cell current–voltage (I–V) relationships. All data were stored on a computer for off-line analysis.
Treatment of cells with JSK and Cyt-D. Stock solutions of cytochasin D (Cyt-D) (78–100 mM in DMSO; Sigma) or jasplakinolide (JSK; 1 mM in DMSO; Invitrogen, Eugene, OR) were separated into 1 µl aliquots and stored at –20°C in plastic vials. For each experiment, a fresh 1 µl aliquot of drug or DMSO was well mixed into 400 µl of oxygenated PIPES solution, yielding concentrations of 195–250 µM Cyt-D and 2.5 µM JSK in 0.25% DMSO. Enzyme-treated tissue blocks were then placed and triturated in this solution and plated onto 4–5 plastic Petri dishes. Dishes containing drug treated cells (30–60 min after plating) were then flooded with HEPES recording solution just before recording was to begin.
Statistics. All values are reported as mean ± SEM. Comparisons of the means between groups were made using Student's t test or ANOVA (SigmaStat 2.1; SPSS, Chicago, IL) as indicated. Differences between the means were considered significant when p < 0.05. Where differences were found by ANOVA and Dunn's test for multiple comparisons was performed post hoc to identify specific distinctions (p < 0.05).
Results
If osmosensory transduction is attributable primarily to a mechanical regulation of SIC channels, then this process should be quantitatively equivalent when induced by changes in cell volume provoked by osmotic perturbations and by changes in hydrostatic pressure applied under isotonic conditions. To test this hypothesis, whole-cell voltage-clamp recordings were made from MNCs acutely isolated from the supraoptic nucleus of adult rats. Cells were challenged with osmotic stimuli (in the absence or presence of mannitol) or changes in hydrostatic pressure (applied to the inside of the recording pipette), and synchronous values of normalized cell volume (nV) and membrane conductance were determined at different time points by digital imaging and steady-state I–V analysis. As reported previously (Oliet and Bourque, 1993aG) vary inversely with cell volume. To obtain a positive numerical index of transducer sensitivity, values of
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Figure 1. Volume modulation of cation current by osmotic and hydrostatic pressure. A, Steady-state I–V relationships measured from isolated MNCs (VH = –70 mV) exposed to hypotonic (left) and hypertonic solutions (right). Note that the stimuli respectively reduce and increase slope conductance. B, Relationships between changes in slope conductance (
If the mechanical gating of SIC channels is solely responsible for osmosensory transduction, then it should be possible to interrupt and reverse the osmotic modulation of the channels by a mechanically induced recovery of cell volume. Indeed, the decrease in membrane conductance associated with hypotonic swelling could be reversed by reducing cell volume via the application of negative pressure to the recording pipette (Fig. 2A). Conversely, the increase in membrane conductance provoked by hypertonic shrinking could be reversed by inflating the cell via an increase in pipette pressure (Fig. 2B). We also attempted to reverse the effects of mechanically evoked changes in cell volume by antagonistic osmotic stimuli. Whereas we could readily reverse suction-evoked increases in conductance by exposing the cell to a hypotonic solution (n = 6) (data not shown), we could not maintain stable whole-cell recordings long enough to examine the effects of hypertonicity on the reduced conductance provoked during sustained increases in pipette pressure. Linear regression analysis of data obtained from individual cells was then performed to determine the slope of the relationship between
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Figure 2. Reversal of osmosensory transduction by hydrostatic pressure. A, Plot showing values of membrane conductance (G) and nV observed in an isolated MNC exposed to a sustained hypotonic stimulus (–60 mosmol/kg, gray area). After 110 s, negative pressure (bar, –50 mmHg) was applied to the recording pipette. Note that this procedure reversed the effects of the hypotonic stimulus on nV and G. B, Plot showing values of G and nV observed in a cell exposed to a sustained hypertonic stimulus (+60 mosmol/kg, gray area). After 100 s, positive pressure (bar, +30 mmHg) was applied to the recording pipette. Note that this procedure reversed the effects of the hypertonic stimulus on nV and G. C, Bar graphs showing mean values of transducer sensitivity observed when hydrostatic pressure and osmotic stimuli were used to initiate (onset, open bars) or reverse (reversal, filled bar) the modulation of membrane cation conductance by changes in cell volume. No significant difference was observed (p > 0.05; two-way ANOVA).
Previous studies have indicated that filamentous actin (F-actin) can either participate in the gating of mechanosensitive channels (Su et al., 2000
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Figure 3. Role of F-actin in mechanotransduction. A, Whole-cell current recordings (VH = –60 mV) from isolated MNCs exposed to Cyt-D (middle), vehicle (control, top), or JSK (bottom). Vertical deflections are current responses to hyperpolarizing steps (–20 mV) applied every 5 s to monitor G. In each case, negative pressure (
Finally, to determine whether F-actin is necessary for osmosensory transduction, we examined the effects of Cyt-D and JSK on the current-clamp responses of MNCs to a hyperosmotic challenge (+60 mosmol/kg; 60–80 s). As illustrated in Figure 4A, excitatory responses to this stimulus were smaller in Cyt-D treated cells (n = 20) and larger in JSK treated cells (n = 11) than in vehicle-treated controls (n = 15). Indeed, although osmotically evoked changes in cell volume were equivalent in the three groups (Fig. 4B) (p = 0.973), significant differences were observed in the magnitude of the depolarizing osmoreceptor potentials and excitatory responses observed under the three conditions. Specifically, Cyt-D significantly reduced the average amplitude of the osmoreceptor potentials (0.6 ± 0.8 mV in Cyt-D vs 8.1 ± 1.3 mV in control; p < 0.001) and the increase in firing rate (+0.3 ± 0.2 Hz in Cyt-D vs + 1.6 ± 0.5 Hz in control; p < 0.05) induced by the hyperosmotic stimulus. Conversely, JSK significantly enhanced both the osmoreceptor potential (+12.5 ± 1.4 mV; p = 0.013) and the excitatory effect (+3.1 ± 0.7 Hz; p = 0.012) of the hyperosmotic stimulus.
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Figure 4. F-actin is required for osmosensory transduction. A, Whole-cell current-clamp recordings from isolated MNCs subjected to hypertonic stimuli (bar; +60 mosmol/kg). The traces show representative recordings taken from cells treated with vehicle (control, top), Cyt-D (middle), and JSK (bottom). In all traces, the spikes are truncated and the dashed line indicates –55 mV. B, Bar graphs showing that mean (±SEM) osmoreceptor potentials (depolarization measured at 60 s; middle) and excitation (increase in firing observed between 50 and 70 s compared with control; right) were significantly reduced by Cyt-D and significantly enhanced by JSK, whereas no difference was noted in the amount of shrinking evoked by the osmotic stimulus (p = 0.923; measured 60 s after stimulus onset; left). *p < 0.05.
Discussion
Osmosensory transduction is a mechanical event
Our experiments revealed that the sensitivity of the relationship between cell volume and membrane cation conductance was quantitatively equivalent whether the volume of MNCs was modulated by osmotic stimuli, or by changes in pipette pressure applied under isotonic conditions. Although the maximal amplitudes of the stimuli used in our experiments provoked changes in cell volume that exceeded those that occur under physiological conditions, it is important to note that the inverse relationship between membrane conductance and cell volume could be clearly detected with volume changes of 2–3% (Fig. 1B), well within the physiological range (Zhang and Bourque, 2003Actin filaments mediate mechanical coupling during osmosensory transduction
Previous studies have established that elements of the cytoskeleton are attached to the plasma membrane via links to a variety of membrane-associated proteins (Revenu et al., 2004Molecular basis for mechanical control of SIC channels during osmosensory transduction
The molecular mechanism that underlies the modulation of SIC channels during osmosensory transduction remains unknown and may involve proteins other than F-actin and the SIC channel itself. Although our results cannot exclude the possibility that an actin-dependent mechanically gated biochemical step is involved in the osmotic modulation of SIC channels, such a process would have to be bidirectional, and rapidly reversible, because the time course of mechanotransduction mirrored that of the changes in cell volume. Alternately, it remains possible that volume-dependent modulation of SIC channel activity reflects the intrinsic mechanosensitivity of these channels (Oliet and Bourque, 1993a
Footnotes
Received July 31, 2006; revised March 5, 2007; accepted March 6, 2007.This work was supported by Canadian Institutes of Health Research (CIHR) Operating and Senior Investigator Awards and by a James McGill Research Chair to C.W.B. In addition, A.N.K. was the recipient of studentship awards from the Fonds pour la Formation de Chercheurs et l'Aide à la Recherche of Quebec and from the McGill University Health Center Research Institute (MUHCRI). R.S.-N. was the recipient of doctoral awards from the CIHR and the Heart and Stroke Foundation of Canada (HSFC), and Z.Z. was the recipient of studentship awards from the MUHCRI and the HSFC.
Correspondence should be addressed to Dr. Charles W. Bourque, Division of Neurology, Room L7-216, Montreal General Hospital, 1650 Cedar Avenue, Montreal, Quebec, Canada H3G 1A4. Email: charles.bourque{at}mcgill.ca
Copyright © 2007 Society for Neuroscience 0270-6474/07/274008-06$15.00/0
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