Intracellular calcium regulation among subpopulations of rat dorsal root ganglion neurons

doi:10.1113/jphysiol.2006.116418

NEUROSCIENCE

Intracellular calcium regulation among subpopulations of rat dorsal root ganglion neurons

Shao-Gang Lu¹, Xiulin Zhang¹ and Michael S. Gold¹^,2^,3

¹ Department of Biomedical Sciences, Dental School
² Program in Neuroscience
³ Department of Anatomy and Neurobiology, Medical School, University of Maryland, Baltimore, Baltimore, MD 21201, USA

Abstract

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Abstract
Introduction
Methods
Results
Discussion
References

Primary afferent neurons are functionally heterogeneous. Todetermine whether this functional heterogeneity reflects, inpart, heterogeneity in the regulation of the concentration ofintracellular Ca²⁺ ([Ca²⁺]_i), the magnitude and decay of evokedCa²⁺ transients were assessed in subpopulations of dorsal rootganglion (DRG) neurons with voltage clamp and fura-2 ratiometricimaging. To determine whether differences in evoked Ca²⁺ transientsamong subpopulations of DRG neurons reflected differences inthe contribution of Ca²⁺ regulatory mechanisms, pharmacologicaltechniques were employed to assess the contribution of influx,efflux, release and uptake pathways. Subpopulations of DRG neuronswere defined by cell body size, binding of the plant lectinIB₄ and responsiveness to the algogenic compound capsaicin (CAP).Ca²⁺ transients were evoked with 30 mM K⁺ or voltage steps to0 mV. There were marked differences between subpopulations ofneurons with respect to both the magnitude and decay of theCa²⁺ transient, with the largest and most slowly decaying Ca²⁺transients in small-diameter, IB₄-positive, CAP-responsive neurons.The smallest and most rapidly decaying transients were in large-diameter,IB₄-negative and CAP-unresponsive DRG neurons. These differenceswere not due to a differential distribution of voltage-gatedCa²⁺ currents. However, these differences did appear to reflecta differential contribution of other influx, efflux, releaseand uptake mechanisms between subpopulations of neurons. Theseresults suggest that electrical activity in subpopulations ofDRG neurons will have a differential influence on Ca²⁺-regulatedphenomena such as spike adaptation, transmitter release andgene transcription. Significantly more activity should be requiredin large-diameter non-nociceptive afferents than in small-diameternociceptive afferents to have a comparable influence on theseprocesses.

(Received 3 July 2006; accepted after revision 24 August 2006; first published online 31 August 2006)
Corresponding author M. S. Gold: Department of Biomedical Sciences, University of Maryland Dental School, 666 West Baltimore Street, Baltimore, MD 21201, USA. Email: mgold{at}umaryland.edu

Introduction

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Abstract
Introduction
Methods
Results
Discussion
References

Primary afferent neurons are heterogeneous (Priestley et al. 2002).This heterogeneity has been well documented in afferent structure(i.e. termination patterns on both central and peripheral targets),neurochemistry (i.e. transmitter and receptor systems) and neurophysiology(i.e. adaptation properties and axon conduction velocity). Thisheterogeneity reflects the fact that primary afferent neuronssubserve a wide array of functions both afferent and efferentin an organ system that is also highly heterogeneous.

Calcium (Ca²⁺) acts as a second messenger within neurons toregulate a diverse array of physiological processes includingtransmitter release, changes in excitability, enzyme activityand gene expression (Berridge et al. 2000). Consequently, theconcentration of intracellular Ca²⁺ ([Ca²⁺]_i) is tightly regulatedand the mechanisms underlying its regulation are numerous (Berridge, 1998;Berridge et al. 2000; Thayer et al. 2002). Regulatory mechanismsinclude influx pathways (ion channels), efflux pathways (pumpsand exchangers), mechanisms underlying uptake and release fromintracellular stores (mitochondria and endoplasmic reticulum)and Ca²⁺-binding proteins. Results from previous studies indicatethat these regulatory mechanisms are differentially distributedamong subpopulations of sensory neurons. For example, inhibitionof Na⁺/Ca²⁺ exchanger by replacing extracellular Na⁺ with Li⁺results in an increase in resting [Ca²⁺]_i in most dorsal rootganglion (DRG) neurons, while a slowed decay of evoked Ca²⁺transients is only observed in a subpopulation of DRG neurons(Verdru et al. 1997). In addition, while mitochondria have beenshown to buffer ‘large’ Ca²⁺ loads in most DRG neurons(Werth & Thayer, 1994) they appear to influence the magnitudeand decay of evoked Ca²⁺ transients in specific subpopulationsof DRG neurons (Kostyuk et al. 1999). There also is evidencethat ‘calcium-induced calcium release’ (CICR) contributesto evoked Ca²⁺ transients in a subpopulation of rat DRG neurons(Shmigol et al. 1995b). Importantly, however, there has beenno systematic analysis of the regulation of [Ca²⁺]_i among subpopulationsof sensory neurons. Therefore, the present study was conductedin order to determine (1) whether there are differences amongsubpopulations of sensory neurons with respect to both restingand evoked increases in [Ca²⁺]_i; and (2) whether differencesin the regulation of [Ca²⁺]_i among subpopulations of sensoryneurons reflects a differential contribution of various [Ca²⁺]_i-regulatorymechanisms.

Standard fura-2 ratiometric techniques were employed in orderto monitor evoked changes in intracellular calcium level ofacutely dissociated DRG neurons. Pharmacological techniqueswere employed in order to assess the relative contribution ofvarious [Ca²⁺]_i regulatory mechanisms. Preliminary results fromthis study have been published elsewhere (Lu & Gold, 2005).

Methods

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Abstract
Introduction
Methods
Results
Discussion
References

Adult (240–340 g) male Sprague-Dawley rats (Harlan, Indianapolis,IN, USA) were used for this study. Rats were housed in the Universityof Maryland Dental School animal facility in groups of threeon a 12: 12 light dark schedule. Food and water are availablead libitum. All the experiments were approved by the Universityof Maryland Dental School Institution Animal Care and Use Committeeand performed in accordance with National Institutes of Healthguidelines as well as guidelines established by the InternationalAssociation of the Study of Pain for the use of laboratory animalsin research. Rats were deeply anaesthetized for both tissuelabelling and tissue harvest (details provided below). The depthof anaesthesia was assessed by monitoring for the presence orabsence of corneal reflexes and withdrawal responses to noxiouspinch of the handpaw. Respiration rate was also monitored. Supplementalanaesthesia was administered until animals were areflexive.Following tissue harvest, rats were killed by decapitation.

Chemicals and reagents

2-APB (2-aminoethoxydiphenylborate) and CPA (cyclopiazonic acid)were purchased from Calbiochem (La Jolla, CA, USA), DiI 1,1'-dioctadecyl-3,3,3',3'-tetramethylindocarbo-cyanineperchlorate was purchased from Invitrogen (Carlsbad, CA, USA).Fura-2 acetoxymethyl (AM) ester and pluronic were purchasedfrom TEF Laboratories (Austin, TX, USA). C28R2 conjugated toTAT to enable cell access was custom synthesized (GenScriptCorp, Scotch Pains, NJ, USA). All other chemicals were purchasedfrom Sigma-Aldrich (St Louis, MO, USA). Concentrations usedwere based on results from previous studies by other investigators.2-APB (100 µM), CCCP (carbonyl cyanide m-chlorophenylhydrazone, 10 µM), CPA (10 µM), ionomycin (10 µM),ryanodine (10 µM), fura-2 AM (2.5 µM) and pluronic(0.025%) were dissolved in DMSO (dimethyl sulfoxide) at concentrationsat least 1000x final, stored at –20°C, and then dilutedin bath solution immediately before use. C28R2 (2 µM),FITC-conjugated IB₄ (IB₄, 10 µg ml^–1), UTP (uridine5'-triphosphate, 100 µM) were dissolved in distilled waterat 1000x stocks. Capsaicin was dissolved in ethanol as a 1 mMstock. All other compounds were dissolved in bath solution directly.

Labelling of DRG neurons innervating the glabrous skin of the hindpaw

Prior to tissue harvest (>3 weeks), DRG neurons innervatingthe glabrous skin of the hindpaw were labelled with the retrogradetracer DiI. Labelling was performed as previously described(Gold & Traub, 2004). DiI was dissolved in DMSO (170 mgml^–1) and diluted 1: 10 in 0.9% of sterile saline. Diluteddye (10 µl) was injected subcutaneously under isofluraneanaesthesia with a 30 g injection needle; anaesthesia was inducedwith 6% isoflurane (Abbott Laboratories, North Chicago, IL,USA) and maintained with 1.5% isoflurane. DiI-labelled neuronswere easily identified under epifluorescence illumination witha Texas-red filter set.

Cell dissociation

Rats were deeply anaesthetized with a subcutaneous injectionof a mixture (1 ml kg^–1 of 55 mg ml^–1 ketamine,5.5 mg ml^–1 xylazine, and 1.1 mg ml^–1 acepromazine)(ketamine was from Fort Dodge Animal Health, Fort Dodge, WI,USA; xylazine and acepromazine were from Phoenix ScientificInc., St Joseph, MO, USA) and DRG neurons were prepared as previouslydescribed (Gold et al. 1996). Briefly, L_4–5 DRG ipsilateralto DiI injection were surgically removed, and desheathed inice-cold culture media composed of 90% minimal-essential-medium(MEM; Gibco BRL, Gaithersburg, MD, USA), 10% heat-inactivatedfetal bovine serum (FBS), 1x MEM vitamins and 1000 u ml^–1each of penicillin and streptomycin (MEM-COMP). DRG were incubated45 min at 37°C in 5 ml MEM containing 0.125% collagenaseP (Roche Bioscience, Palo Alto, CA, USA), 1x MEM vitamins and1000 u ml^–1 each of penicillin and streptomycin, and bubbledwith carbogen (95% O₂–5% CO₂). DRG were centrifuged at $~$ 400 g for 4 min, the collagenase solution was removed and thenreplaced 2.5 ml Ca²⁺- and Mg²⁺-free Hanks balanced salt solution(Gibco BRL, Gaithersburg, MD, USA) containing 0.25% trypsin(Worthington, Bristol, UK), 80 µg ml^–1 DNase and0.025% EDTA. Ganglia were mechanically dissociated in this solutionwith fire-polished pasteur pipettes and then incubated for 5min at 37°C. Trypsin activity was inhibited by the additionof 2.5 ml MEM-COMP containing 0.125% MgSO₄. Cell suspensionwas then centrifuged at $~$ 400 g for 4 min, resuspended with MEM-COMP,and plated onto glass coverslips, previously coated by a solutionof 5 µg ml^–1 mouse laminin (Gibco BRL, Gaithersburg,MD, USA) and 0.1 mg ml^–1 poly-L-ornithine. The cells wereincubated in MEM-COMP at 37°C, 3% CO₂, and 90% humidityfor 2 h, at which point they were transferred to a L-15 media(Gibco BRL, Gaithersburg, MD, USA) containing 10% FBS, 5 mMHepes and 5 mM glucose, and stored at room temperature. Allexperiments were performed within 8 h of tissue harvest.

Subclassification of DRG neurons

DRG neurons were subclassified on the basis of several criteria.These included cell body size, binding to the plant (Griffoniasimplicifolia) lectin isolectin B₄ (IB₄) and responsivenessto the algogenic compound capsaicin (CAP). Neurons were dividedinto small (<30 µm), medium (30–40 µm),and large ( $≥$ 40 µm) based on cell body diameter (Caffrey et al. 1992;Scroggs & Fox, 1992a) as measure with a calibrated eyepiecereticule. Based on the rough correlation between cell body sizeand axon conduction velocity (Harper & Lawson, 1985) aswell as previous anatomical and electrophysiological studiesperformed in vitro (Lawson, 2002), neurons with a small cellbody diameter are likely to be nociceptive afferents, whilethose with a large cell body diameter are likely to be non-nociceptiveafferents. Neurons with a medium cell body diameter are likelyto encompass both nociceptive and non-nociceptive afferents.IB₄ binding is a relatively simple way of identifying a uniquepopulation of afferents that appear to be involved in nociceptiveprocessing (Nagy & Hunt, 1982; Silverman & Kruger, 1990).IB₄-positive (IB₄+) neurons tend to give rise to unmyelinatedaxons, be devoid of the neuropeptides substance P and calcitoningene-related peptide (CGRP) and express a unique distributionof other receptors, including the ATP receptor P_2x3 (Vulchanova et al. 1998),which is thought to mediate the pain associated with tissuedamage. Finally, while not all nociceptive afferents are CAPresponsive (CAP+), CAP+ neurons are likely to be nociceptive,given that the only sensation associated with the cutaneousapplication of CAP is pain, and in naïve tissue CAP onlyactivates high-threshold C-fibre afferents (Martin et al. 1987).

Intracellular Ca²⁺ measurements

DRG neurons were loaded with 2.5 µM calcium indicatorfura-2 AM ester with 0.025% pluronic for 20 min at room temperatureas previously described (Thut et al. 2003). They were subsequentlylabelled with FITC-conjugated IB₄ (10 µg ml^–1 for10 min). Following fura-2 loading and IB₄ labelling, DRG neuronswere placed in a recording chamber and were continuously perfusedwith normal bath solution (mM: 130 NaCl, 3 KCl, 2.5 CaCl₂, 0.6MgCl₂, 10 Hepes, 10 glucose, pH adjusted with Tris base to 7.4,osmolality adjusted with sucrose to 325 mosmol l^–1). Forsome experiments, a ‘Ca²⁺-free’ bath solution wasemployed, which was the normal bath solution modified by theomission of CaCl₂, the addition of 0.1 mM EGTA and an increasein the concentration of MgCl₂ 3.1 mM. Fluorescence data wereacquired on a PC running Metafluor software (Molecular Devices,Sunnyvale, CA, USA) via a CCD camera (Roper Scientific, Trenton,NJ, USA, Model RTE/CCD 1300). The ratio (R) of fluorescenceemission (510 nm) in response to 340/380 nm excitation (controlledby a lambda 10-2 filter changer (Sutter Instruments CA, USA))was acquired at 1 Hz during drug applications. All drugs wereapplied via a gravity-fed chamber perfusion system except highK⁺ (30 mM), caffeine (10 mM), and capsaicin (500 nM), whichwere delivered by a computer-controlled fast perfusion system(switching time <50 ms; ALA Scientific Instruments, Westbury,NY, USA, Model DAD-12); normal bath (with 2.5 mM Ca²⁺) was appliedwith the fast perfusion system where indicated.

Intracellular free calcium concentration ([Ca²⁺]_i) was derivedfrom fluorescent ratios (R) following performance of in situcalibration experiments (Grynkiewicz et al. 1985; Kao, 1994)according to the following equation:

(1)
where K_d is the dissociation constant offura-2 for Ca²⁺ at room temperature (i.e. 224 nM); S_f2/S_b2 isthe fluorescence ratio of the emission intensity excited by380 nm signal in the absence of Ca²⁺ to that during the presenceof saturating Ca²⁺; R_min or R_max is the minimal or maximal fluorescenceratios, respectively. R_min was measured by perfusing the neuronswith nominally Ca²⁺-free bath solution containing 1.0 mM EGTAand 10 µM ionomycin with 10 mM Mg²⁺ for at least 40 min.R_max was obtained by perfusing neurons with standard bath solutioncontaining 20 mM Ca²⁺ and 10 µM ionomycin for a few minutes.Background values of F₃₄₀ and F₃₈₀ were collected by perfusingthe neurons with 50 µM digitonin for a few minutes. Valuesof S_f2/S_b2, R_min, or R_max were 15.51, 0.48, or 14.83 averagedover 65 neurons obtained from seven separate in situ calibrationexperiments performed over the time period during which allother experimental data was collected.

Electrophysiological recording

Whole-cell patch-clamp recordings were performed using an Axopatch200B amplifier (Molecular Devices, Sunnyvale, CA, USA) or EPC-9amplifier (HEKA Elektronik GmbH, Lambrecht, Germany). Seriesresistance was compensated (>80%) with amplifier circuitry.Data were acquired at 10 kHz and filtered at 2 kHz. Electrodes(1.8–3.0 M ${Omega}$ ) were filled with pipette solution (mM: 100Cs-Methansulphonate (MS), 5 Na-MS, 40 TEA-Cl, 1 CaCl₂, 2 MgCl₂,11 EGTA, 10 Hepes, 2 ATP-Mg, 1 GTP-Li); pH was adjusted to 7.2with Tris-base and osmolality was adjusted to 310 mosmol l^–1with sucrose. The bath solution was constructed to minimizeother currents in sensory neurons and contained (mM): 100 Choline-Cl,30 TEA-Cl, 2.5 CaCl₂, 0.6 MgCl₂, 10 Hepes, 10 Glucose; pH wasadjusted to 7.4 with Tris-base and osmolality was adjusted to325 mosmol l^–1 with sucrose. Neurons were held at –60mV. Voltage-gated Ca²⁺ currents were evoked with a series of60 ms command potentials from –80 to 60 mV in 5 mV incrementsteps following a 15 ms prepulse to –100 mV. Leak currentswere digitally subtracted using a P/–4 leak subtractionprotocol from a holding potential of –80 mV. For whole-cellcurrent-clamp recording, electrodes were filled with the pipettesolution mentioned above, but Cs⁺ and TEA⁺ were replaced byK⁺, and neurons were perfused with normal bath solution.

Intracellular Ca²⁺ measurements from voltage-clamped DRG neurons

The perforated-patch configuration of whole-cell patch clampwas used to assess Ca²⁺ transients evoked with voltage steps.For these experiments, pipette solution contained (mM): 30 KCl,55 K₂SO₄, 1 MgCl₂, 0.1 EGTA, 10 Hepes; pH was adjusted to 7.2with KOH and osmolality was adjusted to 310 mosmol l^–1with sucrose. Electrodes (1.8–3.0 M ${Omega}$ ) were dip-filled inthe pipette solution and subsequently back-filled with the samesolution but containing Amphotericin B (480 µg ml^–1,Sigma-Aldrich, St Louis, MO, USA) for perforation (Usachev et al. 1995).A series resistance of <20 M ${Omega}$ was achieved between 5 and 30min after seal formation which was compensated (about 60%) withamplifier circuitry. Ca²⁺ transients were evoked with depolarizationvoltage steps from –60 mV to 0 mV for 4000 ms, the sameduration used to apply high-K⁺ solution.

Statistical analysis

Data are expressed as mean ± S.E.M. Student's ttest and one-way ANOVA with the Holm–Sidak post hoc testwere used for simple comparisons between groups. For experimentsinvolving the application of test compounds, vehicle controlswere always included. Because we sought to assess the presenceof statistically significant influences of test compounds andthe possibility that there were differences between subpopulationsof sensory neurons with respect to the response to the testcompound (i.e. two main effects), as well as the interactionbetween the two, a two-way ANOVA was employed. Differences betweengroups were assessed with a Holm–Sidak post hoc test ifthere was a statistically significant interaction between maineffects. Statistical significance was assessed at P < 0.05.

Results

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Abstract
Introduction
Methods
Results
Discussion
References

Subpopulations of DRG neurons studied

Acutely dissociated DRG neurons from adult male rats were classifiedbased on the cell body diameter, IB₄ binding, CAP sensitivityand whether or not they innervated the glabrous skin of thehindpaw. Cell body diameter of DRG neurons was measured underbright-field illumination (Fig. 1Aa and d). DiI+ and IB₄+ DRGneurons were identified under epifluorescence illumination (Fig. 1Ab and c).CAP+ DRG neurons were identified at the end of experiments witha brief application of CAP (500 nM). Neurons considered CAP+demonstrated an increase in fura-2 fluorescent ratio >20%above baseline (Fig. 1Ae and f). A histogram of cell body diameteris shown in Fig. 1B, and 55% (127 out of 231), 25% (57 out of231) and 20% (47 out of 231) of all DRG neurons studied wereclassified as small, medium, and large. Consistent with previousobservations (Harper & Lawson, 1985), this histogram wasskewed, with the majority of neurons falling into the small-diametercategory; the median cell body diameter was 28.8 µm (with25.3 µm and 35.9 µm as 25th and 75th percentiles,respectively). 59% (136 out of 231) of neurons were IB₄+ and53% (123 out of 231) of neurons were CAP+. The majority of bothIB₄+ neurons (71%, 96 out of 136) and CAP+ neurons (69%, 85out of 123) were classified as small, while 28% (39 out of 136)and 1% (1 out of 136) of IB₄+ neurons and 29% (36 out of 123)and 2% (2 out of 123) of CAP+ neurons were classified as mediumand large, respectively. Thus, consistent with previous observations(Gold et al. 1996; Dirajlal et al. 2003), both IB₄+ and CAP+neurons were significantly smaller than IB_4– and CAP–neurons. Seventy-one per cent (97 out of 136) of IB₄+ neuronswere CAP+, while 79% (97 out of 123) of CAP+ neurons were IB₄+.

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Figure 1. Subpopulations of DRG neurons
A, photomicrographs of subpopulations of DRG neurons. Bright field images (a and d) were used to determine cell body diameter (scale bars: 50 µm). Under epifluorescence illumination, DiI- (b) and IB₄- (c) labelled neurons were identified in the field of neurons shown in a. The capsaicin sensitivity of the neurons shown in d was assessed with fura-2 microfluorimetry. Fura-2 fluorescence ratio is low at rest (e) and dramatically increased in a subpopulation of neurons (f) following application of capsaicin (500 nM). B, cell body diameter histogram of the total population of DRG neurons (n = 231, grey bars), IB₄-positive (IB4+) neurons (n = 136, black bars) and CAP-sensitive (CAP +) neurons (n = 123, white bars). Appoximately 70% IB₄+ and CAP+ DRG neurons had a small cell body diameter.

Twenty-three per cent (53 out 231) of the total population wereDiI+ neurons (i.e. cutaneous neurons innervating glabrous skinof the hindpaw), which comprised 19, 16 and 18 small, mediumand large neurons, respectively. The median cell body diameterof these cutaneous neurons was 31.23 µm (with 27.9 µmand 41.6 µm as 25th and 75th percentiles, respectively).Fifty-one per cent (27 out of 53) of cutaneous neurons wereIB₄+ and 49% (26 out of 53) were CAP+; 59% (16 out of 27) ofIB₄+ cutaneous neurons and 58% (15 out of 26) CAP+ cutaneousneurons were classified as small. Thirty-seven per cent (10out of 27) and 4% (1 out of 27) of IB₄+ cutaneous neurons, and38% (10 out of 26) and 4% (1 out of 26) of CAP+ cutaneous neuronswere classified as medium and large, respectively; 78% (21 outof 27) of IB₄+ cutaneous neurons were CAP+; 81% (21 out of 26)of CAP+ cutaneous neurons were IB₄+. There were no statisticallysignificant differences between cutaneous neurons and unlabelledneurons with respect to the distribution of neurons within subpopulations.

High-K⁺-induced Ca²⁺ transient in DRG neurons

A brief (4 s) application of 30 mM K⁺ (high K⁺) was used toevoke an increase in [Ca²⁺]_i subsequently referred to as a Ca²⁺transient. Representative recordings in Fig. 2A–C showevoked Ca²⁺ transients in small-, medium- and large-diameterDRG neurons, respectively. These evoked Ca²⁺ transients wereentirely dependent upon the presence of extracellular Ca²⁺ (Fig. 2D),as the 30 mM K⁺-evoked Ca²⁺ transients were completely abolishedin Ca²⁺-free bath solution in all small (7 of 7), medium (3of 3) and large (3 of 3) neurons tested. In order to determinethe extent of the depolarization induced by high K⁺, as wellas whether differences in resting membrane potential and/oradaptation properties could contribute to differences betweensubpopulations with respect to the magnitude and decay of evokedCa²⁺ transients, conventional whole-cell patch recordings weremade in current clamp (Fig. 2E). Resting membrane potentialwas –56.4 ± 4.3 (n = 10), –58.5 ±4.2 (n = 10) and –59.7 ± 3.1 (n = 7)in small-, medium- and large-diameter DRG neurons, respectively.Differences between groups were not statistically significant(P > 0.05, one way ANOVA). A 4 s application of 30 mM K⁺resulted in a rapid depolarization to a membrane potential atwhich the majority of neurons were rapidly ‘clamped’for the duration of the high-K⁺ application (Fig. 2E). Followingtermination of the high K⁺, resting membrane potential was rapidlyre-established. Action potentials were evoked by high-K⁺ applicationin 15 of 27 (56%) neurons tested, which included 8 of 10 small-diameterneurons, 7 of 10 medium-diameter neurons and 0 of 7 large-diameterneurons. Only one action potential was fired in 6 of the 15neurons in which any activity was observed. In four small-diameterneurons and one medium-diameter neuron in which more than oneaction potential was fired, overshooting action potentials werefollowed by high-frequency (44 ± 5 Hz) membrane potentialoscillations that decreased in amplitude to undetectable levelsover the initial period of membrane depolarization. The averagetime between the start of high-K⁺ application and the pointat which the membrane potential was effectively ‘clamped’at a depolarized potential was 773 ± 193 ms in all theneurons that fired more than a single spike yet demonstratedaccommodation during the high-K⁺ application. This durationwas 814 ± 173 (n = 6) and 528 ms (n = 1)in small- and medium-diameter neurons, respectively. Finally,in two neurons, the high-K⁺-evoked depolarization was associatedwith sustained action potential generation; the average instantaneousspike frequency was $~$ 7 Hz in one and $~$ 4 Hz in the other. Bothof these neurons were classified as medium-diameter neurons.Of the 25 neurons tested that did not fire sustained actionpotentials in response to 30 mM K⁺, the membrane potential waseffectively ‘clamped’ to –17 ± 1 mV,–19 ± 1 mV and –20 ± 1 mV in small,medium and large neuron groups, respectively. Differences betweengroups were not statistically significant (P > 0.05, one-wayANOVA).

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Figure 2. High-K⁺-evoked Ca²⁺ transients in DRG neurons
Ca²⁺ transients were evoked with a 4 s application of 30 mM K⁺ in typical small- (A), medium- (B) and large- (C) diameter DRG neurons. D, the high-K⁺-evoked Ca²⁺ transient is abolished in the presence of Ca²⁺-free bath solution. High K⁺ was applied at points indicated by black bars. Ca²⁺-free bath solution was applied for the time indicated with the continuous line. E, Response of a typical neuron under current clamp to 30 mM K⁺ (high K⁺). Voltage trace shows a rapid depolarization that was associated with the generation of two action potentials. The membrane potential was then stably ‘clamped’ at –21 mV for the remainder of the high-K⁺ application, after which membrane potential returned to baseline. Perforated-patch recording was used to study the magnitude and decay of Ca²⁺ transients evoked with a voltage step. Ca²⁺ transients evoked with a 4 s voltage step to 0 mV from a holding potential of –60 mV in typical small- (F), medium- (G) and large- (H) diameter neurons were similar to those evoked with 30 mM K⁺.

Differences among subpopulations of DRG neurons with respect to evoked Ca²⁺ transient

The resting [Ca²⁺]_i levels were 145 ± 4 (n = 127),129 ± 5 (n = 57) and 128 ± 4 nM (n =47) in small-, medium- or large-diameter DRG neurons, respectively.They were 138 ± 3 (n = 136) and 137 ± 4nM (n = 95) in IB₄+ and IB_4– neurons, respectively,and they were 135 ± 3 (n = 123) and 140 ±4 nM (n = 118) in CAP+ and CAP– DRG neurons, respectively.Differences between subpopulations were not statistically significant(P > 0.05, one-way ANOVA or Student's t test).

As shown in Fig. 3A, the magnitude of evoked Ca²⁺ transient,analysed as the difference between peak evoked Ca²⁺ and baseline( ${Delta}$ [Ca²⁺]_i), was largest in small- and smallest in large-diameterDRG neurons, respectively (n = 127, 57, and 47 for small-,medium-, and large-diameter neurons, respectively). Differencesbetween groups were statistically significant (P < 0.01,one-way ANOVA). The decay of evoked Ca²⁺ transient (Fig. 3A),analysed as time to 50% of peak (T₅₀), was slowest in small-and the fastest in large-diameter DRG neurons. Differences betweengroups were statistically significant (P < 0.01, one-wayANOVA). The magnitude was larger and the decay was longer inIB₄+ (n = 136) than in IB_4– (n = 95) DRG neurons,respectively (Fig. 3B), while magnitude and decay were largerand longer in CAP+ (n = 123) than in CAP– (n =118) DRG neurons, respectively (Fig. 3C). Differences betweengroups were statistically significant (P < 0.01, Student'st test). The evoked increase in [Ca²⁺]_i in subpopulations ofcutaneous DRG neurons (DiI+) was qualitatively and quantitativelysimilar to that observed in subpopulations of unlabelled DRGneurons as shown in Fig. 3D–F. Differences between subpopulationsof cutaneous neurons were statistically significant (P <0.05 or P < 0.01, one-way ANOVA or Student's t test). However,there were no statistically significant differences betweensubpopulations of unlabelled and DiI-labelled DRG neurons withrespect to the Ca²⁺ transients (P > 0.05, two-way analysisof variance). Because there were no differences between cutaneousand total DRG neurons with respect to the evoked Ca²⁺ transientswhen classified according to cell body diameter, IB₄ binding,and CAP responsiveness, DiI+ neurons were not analysed separatelyin subsequent experiments.

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Figure 3. Differential distributions of evoked Ca²⁺ transients among subpopulations of DRG neurons
A, the magnitude (left), analysed as ${Delta}$ [Ca²⁺]_i (peak value – baseline), and the decay (right), analysed as time to 50% of peak (T₅₀), of evoked Ca²⁺ transients were the largest in small-, and the smallest in large-diameter neurons (n = 127 in small-, 57 in medium-, and 47 in large-diameter cell groups). B, ${Delta}$ [Ca²⁺]_i (left) and T₅₀ (right) were larger in IB₄+ (n = 136) than in IB_4– (n = 95) neurons. C, ${Delta}$ [Ca²⁺]_i (left) and T₅₀ (right) were larger in CAP+ (n = 127) than in CAP– (n = 118) neurons. Data from A, B and C were from both unlabelled and DiI-labelled DRG neurons. Similar results were obtained in cutaneous DRG neurons (DiI-positive) innervating glabrous skin of the hindpaw (D, E and F). D, ${Delta}$ [Ca²⁺]_i and T₅₀ were the largest in small-, and the smallest in large-diameter cutaneous neurons (n = 19, 16, and 18 in small-, medium-, and large- diameter cell groups). E, ${Delta}$ [Ca²⁺]_i and T₅₀ were larger in IB₄+ (n = 27) than in IB_4– (n = 26) cutaneous neurons. F, ${Delta}$ [Ca²⁺]_i and T₅₀ were larger in CAP+ (n = 26) than in CAP– (n = 27) cutaneous neurons. Differences between groups were all statistically significant (*P < 0.05, **P < 0.01). Similar results were also obtained when Ca²⁺ transients were evoked with 4 s voltage steps from –60 to 0 mV in neurons under voltage clamp. ${Delta}$ [Ca²⁺]_i and T₅₀ were the largest in small-, and the smallest in large-diameter neurons (G, n = 10 in small-, 9 in medium- and 7 in large-diameter groups); They were larger in IB₄+ (n = 13) than in IB_4– (n = 13) DRG neurons (H) and they were larger in CAP+ (n = 17) than in CAP– (n = 9) DRG neurons (I). Statistically significant differences between groups are indicated (*P < 0.05, **P < 0.01).

In order to explore the possibility that IB₄ binding and CAPresponsiveness could be used to identify unique subpopulationsof small- and medium-diameter DRG neurons, these two criteria,as well as the combination of the two, were used to define subpopulationsof DRG neurons initially defined by cell body diameter. Table 1contains the results of this analysis, in which the magnitudeand decay of high-K⁺-evoked Ca²⁺ transients were compared betweensubpopulations of small-diameter DRG neurons. Table 2 containsthe results of this analysis for medium-diameter neurons. Insmall-diameter DRG neurons, evoked Ca²⁺ transients decayed moreslowly in IB₄+ neurons, while the magnitude of evoked transientswas larger in CAP– DRG neurons. Results of this analysisraise the possibility that there are large Ca²⁺ transients ina subpopulation of non-nociceptive small-diameter DRG neurons.However, the largest and most slowly decaying Ca²⁺ transientsin medium-diameter DRG neurons were present in putative nociceptors(i.e. IB₄+ and/or CAP+ neurons).

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Table 1. Ca²⁺ transients in subpopulations of small-diameter DRG neurons

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Table 2. Ca²⁺ transients in subpopulations of medium-diameter DRG neurons

The consistency of the high-K⁺-evoked changes in membrane potentialobserved in current clamp experiments could be used to argueagainst a role for excitability differences among DRG neuronsas an explanation for differences among subpopulations of DRGneurons with respect to magnitude and decay of high-K⁺-evokedCa²⁺ transients. However, in order to further address this issue,a group of neurons was studied in voltage clamp. The perforated-patchtechnique was employed in order to establish whole-cell access,while minimizing the impact of the recording on the intracellularmilieu (Horn & Marty, 1988). Resting [Ca²⁺]_i levels at aholding potential of –60 mV were similar to those observedin intact cells when subgrouped according to cell body diameter,IB₄ binding and CAP responsiveness (data not shown). A 4 s voltagestep from –60 mV to 0 mV was associated with an increasein [Ca²⁺]_i in all of neurons tested. Examples of Ca²⁺ transientsevoked with a 4 s voltage step to 0 mV in small-, medium- andlarger-diameter neurons are shown in Fig. 2F–H, respectively.The voltage-step-evoked increase in [Ca²⁺]_i in subpopulationsof DRG neurons was qualitatively and quantitatively similarto that observed in unclamped neurons in response to high K⁺(Fig. 3G–I). Differences between groups were statisticallysignificant (P < 0.05 or P < 0.01, one-way ANOVA or Student'st test). However, there were no statistically significant differencesbetween subpopulations of DRG neurons with respect to the Ca²⁺transients evoked with high K⁺ in unclamped neurons and voltagesteps in voltage-clamped neurons (P > 0.05, two-way analysisof variance).

Differences among subpopulations with respect to Ca²⁺ current density

Depolarization-induced increases in [Ca²⁺]_i in DRG neurons reflectan initial Ca²⁺ influx through voltage-gated Ca²⁺ channels (VGCC)(Shmigol et al. 1995b). In order to determine whether the differencesamong subpopulations of DRG neurons with respect to magnitudeand decay of high-K⁺-evoked Ca²⁺ transients reflect a differentialdensity of voltage-gated Ca²⁺ current, voltage-gated Ca²⁺ currentswere measured in subpopulations of cutaneous DRG neurons withwhole-cell voltage clamp. Currents were evoked as describedin Methods. High-voltage-activated Ca²⁺ current (HVACC) densitywas assessed by measuring peak Ca²⁺ current evoked at 0 mV (Fig. 4A)and dividing this value by cell capacitance. Typical I–Vcurves for Ca²⁺ currents evoked in small- ( ${blacksquare}$ ), medium- ( ${blacktriangleup}$ ) andlarge- (•) diameter DRG neurons are shown in Fig. 4B. Incontrast to high-K⁺-evoked increases in [Ca²⁺]_i, HVACC densitywas the smallest in small cells and the largest in large cells(Fig. 4C; n = 55, 41, and 19 for small-, medium-, andlarge-diameter neurons, respectively). The difference in HVACCdensity between small and large cells was statistically significant(P < 0.05, one-way ANOVA). There were no statistically significantdifferences between subpopulations of DRG neurons defined byIB₄ binding (Fig. 4D; n = 60 for IB₄+ and 48 for IB_4–neurons) and CAP sensitivity (Fig. 4E; n = 54 for CAP+and 37 for CAP– neurons) with respect to HVACC density(P > 0.05, Student's t test).

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Figure 4. Differential distribution of voltage-gated Ca²⁺ currents among subpopulations of DRG neurons
A, Ca²⁺ current traces evoked at 0 mV from a holding potential of –60 mV in typical small- (light grey), medium- (black) and large- (dark grey) diameter DRG neurons, respectively. Current traces shown in A were part of families of traces used to generate the I–V curves shown in B, where data from the small- (S, ${blacksquare}$ ), medium- (M, ${blacktriangleup}$ ) and large- (L, •) diameter DRG neurons are plotted. The large low-voltage-activated Ca²⁺ current (LVACC), or T-type Ca²⁺ current, apparent in I–V data from the medium-diameter neuron was observed in 6 out of 41 (15%) medium-, 3 out of 19 (16%) large- and 2 out of 55 (4%) small-diameter neurons. C, high-voltage-activated Ca²⁺ current (HVACC) densities (left) were the smallest in small-, and the largest in large-diameter neurons (n = 55, 41, and 19 in small-, medium-, and large-diameter cell groups). LVACC densities (right) were smallest in large-, and largest in medium-diameter neurons. D, they were larger in IB_4– (n = 60) than in IB₄+ (n = 48) neurons. E, they were larger in CAP– (n = 54) than in CAP + (n = 37) neurons. The currents at 0 mV or at –50 mV were divided by cell capacitance to yield the HVACC or LVACC density. Statistically significant differences between groups are indicated (*P < 0.05).

The presence of large (>100 pA) low-voltage-activated calciumcurrent (LVACC) or T-type Ca²⁺ current was observed in 6 outof 41 (15%) medium-, 3 out of 19 (16%) large- and 2 out of 55(4%) small-diameter neurons, respectively. Smaller (<100pA at –50 mV) LVACC were detectable in both small- andmedium-diameter DRG neurons. Differences between groups definedby cell body diameter were statistically significant (P <0.05, one-way ANOVA, Fig. 4C) with respect to LVACC density.There were no significant differences between groups definedby IB₄ binding (Fig. 4D) or capsaicin sensitivity (Fig. 4E)with respect to LVACC density (P > 0.05, Student's t test).

CICR via RyR but not IP₃R contributes to evoked Ca²⁺ transients in medium- and large-diameter, IB_4– and CAP– neurons

Results from previous studies suggest that Ca²⁺-induced Ca²⁺release (CICR), from internal stores via ryanodine receptors(RyRs), contributes to the magnitude and duration of evokedCa²⁺ transients in sensory neurons (Solovyova et al. 2002).Therefore, we sought to determine whether a differential distributionin the relative contribution of RyR-mediated CICR to high-K⁺-evokedCa²⁺ transients may contribute to observed differences amongsubpopulations of DRG neurons with respect to the magnitudeand decay of high-K⁺-evoked Ca²⁺ transients. After stable baselineresponses to high K⁺ were established, 10 µM ryanodinewas added to the cell perfusate. Repeated 8 s applications of10 mM caffeine were used to confirm block of RyRs. Neurons werethen stimulated again with high K⁺. Ryanodine alone had no influenceon resting [Ca²⁺]_i level. The change in evoked increase in [Ca²⁺]_iin the presence of ryanodine was calculated as a percentageof baseline according to following equation:

(2)

The change in the decay of the evoked increase in [Ca²⁺]_i wascalculated according to a similar equation:

(3)

Typical examples of evoked Ca²⁺ transients in small- (Fig. 5A)and large- (Fig. 5B) diameter DRG neurons were obtained before(continuous line) and during (dashed line) perfusion with normalbath solution containing 10 µM ryanodine. Two-way ANOVAof pooled data (Fig. 5D–F) revealed a significant drugeffect on both magnitude (P < 0.01) and decay (P < 0.05)of evoked Ca²⁺ transients in all subpopulations of neurons analysed.There was also a significant interaction between subpopulationand drug effects on the magnitude of evoked Ca²⁺ transientswhen neurons were grouped according to cell body size (P <0.01), IB₄ binding (P = 0.01) or CAP sensitivity (P <0.01). That is, inhibition of RyRs resulted in a reduction inthe magnitude of evoked increase in [Ca²⁺]_i in medium- (n =17) and large- (n = 10) diameter, IB_4– (n =27), and CAP– (n = 26) DRG neurons. There was alsoa significant interaction between subpopulation and drug effectson the decay of evoked Ca²⁺ transients in neurons grouped accordingto cell body size (P < 0.05). Of note, block of RyRs hadno statistically significant effect in small-diameter (n =24), IB₄+ (n = 24) and CAP+ (n = 25) subpopulationsof DRG neurons. Application of ryanodine vehicle (bath solutioncontaining 0.1% DMSO) had no significant influence on the magnitudeor decay of evoked Ca²⁺ transients (Fig. 5C–F).

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Figure 5. CICR via RyR contributes to evoked Ca²⁺ transients in large- and medium-cell body diameter, IB_4– and CAP– neurons
Typical evoked Ca²⁺ transients in small- (A) and large-diameter (B) DRG neurons were obtained before (continuous line) and during (dashed line) perfusion with normal bath solution containing 10 µM ryanodine. Note, prior to the second increase in [Ca²⁺]_i response, neurons were challenged with 10 mM caffeine repeatedly to establish block of RyRs. In order to determine the influence of ryanodine on the magnitude and decay of evoked Ca²⁺ transients, data were analysed as a percentage change from baseline which was determined for magnitude and decay as described in the text. Control neurons were treated with vehicle used to dissolve ryanodine (DMSO). C, An example of evoked Ca²⁺ transients from a large-diameter DRG neuron was obtained before and after perfusion with normal bath solution containing 0.1% DMSO. Pooled data for both control (filled bars) and drug-treated (open bars) neurons are plotted, illustrating the influence of ryanodine on the magnitude (left) and decay (right) of evoked Ca²⁺ transients in subpopulations of neurons defined by cell body size (D; n = 24 in small-, 17 in medium- and 10 in large-diameter cell groups), IB₄ binding (E; n = 24 in IB₄+ and 27 in IB_4– cell groups) and CAP sensitivity (F; n = 25 in CAP+ and 26 in CAP– cell groups). Data in each panel were analysed with a two-way ANOVA in order to assess the influence of subpopulation, drug treatment or an interaction between the two. Significant main effects associated with subpopulation and ryanodine were detected in each analysis. Post hoc analysis was performed if there was a significant interaction between main effects (subpopulation and ryanodine). Statistically significant differences between groups are indicated (*P < 0.05, **P < 0.01). Data for DMSO control were collected from 32 small-, 5 medium- and 6 large-diameter DRG neurons, which included 24 IB₄+, and 19 IB_4– neurons or 24 CAP+ and 19 CAP– neurons.

In addition to RyRs, there is evidence that IP₃ receptors mayalso be involved in Ca²⁺ release from internal stores (Svichar et al. 1997;Sanada et al. 2002; Solovyova & Verkhratsky, 2003). Therefore,the possibility that IP₃ receptors contribute to CICR in subpopulationsof DRG neurons was assessed. Bath application of 100 µM2-APB was used to block IP₃ receptors (Bootman et al. 2002).In order to confirm that this concentration of 2-APB was sufficientto block IP₃ receptor-mediated release of Ca²⁺, UTP was usedas a positive control because this compound has been shown toinduce IP₃-mediated increases in [Ca²⁺]_i via P₂Y receptors inDRG neurons (Ralevic & Burnstock, 1998; Sanada et al. 2002).An example of results obtained from this experiment is shownin Fig. 6A. A brief (1.0 s) application of 100 µM UTPwas used to evoke Ca²⁺ transients before (continuous line),during (short dashed line) and after (long dashed line) 2-APB(100 µM) perfusion. 2-APB clearly inhibited the increasein [Ca²⁺]_i induced by UTP. Examples of high-K⁺-evoked Ca²⁺ transientsin small and large neurons in the presence and absence of 100µM 2-APB are shown in Fig. 6B and C. Pooled data werefrom 37 small-, 12 medium-, and 14 large-diameter neurons (Fig. 6D),from 32 IB₄+ and 31 IB_4– neurons (Fig. 6E), and from 30CAP+ and 33 CAP– neurons (Fig. 6F). Blockade of IP₃ receptorsby 2-APB had no statistically significant effects on the magnitudeor decay of evoked Ca²⁺ transient in any of the subpopulationsof DRG neurons studied.

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Figure 6. IP₃ receptors do not appear to contribute to evoked Ca²⁺ transients in DRG neurons
A, UTP-evoked increases in [Ca²⁺]_i were significantly attenuated by 2-APB in a reversible manner. Similar results were obtained in four neurons which responded to UTP application. However, high-K⁺-evoked increase in [Ca²⁺]_i were not significantly influenced by 2-APB. Typical Ca²⁺ transients evoked in small- (B) and large- (C) diameter DRG neurons were obtained before (continuous line) and during (dashed line) perfusion with normal bath solution containing 100 µM 2-APB. The magnitude ( ${Delta}$ [Ca²⁺]_i) and decay (T₅₀) remained unchanged in all subpopulations of DRG neurons (D, E and F) during 2-APB treatment. Differences between groups were not statistically significant (P > 0.05). Data were collected from 37 small-, 12 medium- and 14 large-diameter DRG neurons, which included 32 IB₄+, and 31 IB_4– neurons or 30 CAP+ and 33 CAP– neurons.

SERCA plays a relatively large role in regulation of evoked Ca²⁺ transients in large-diameter, IB_4– and CAP– neurons

To further investigate the contribution of intracellular storesto the heterogeneity of evoked Ca²⁺ transients among DRG neurons,high-K⁺-evoked Ca²⁺ transients were assessed before and afterblock of sarco/endoplasmic reticulum calcium ATPase (SERCA)with CPA (Thayer et al. 2002). Typical examples of evoked Ca²⁺transients in small- (Fig. 7A) and large- (Fig. 7B) diameterDRG neurons were obtained before and during perfusion with normalbath solution containing 5 µM CPA. CPA induced an increasein both the magnitude and decay of evoked Ca²⁺ transients. Asexpected, CPA also caused an increase in resting [Ca²⁺]_i, whichdeclined to some extent after the initial application of thecompound, but did not return to the levels prior to CPA application.Two-way ANOVA of pooled data (Fig. 7C–E) revealed significant(P < 0.01) drug effects in all subpopulations of DRG neuronstested. There was also a significant interaction between subpopulationand drug effects on the magnitude of evoked Ca²⁺ transientswhen neurons were grouped according to cell body size (P <0.01) and CAP sensitivity (P < 0.01). Inhibition of SERCAby CPA caused the largest increase in the magnitude of the evokedCa²⁺ transient in large-diameter (Fig. 7C; n = 44 small-,9 medium- and 16 large-diameter neurons) and CAP– (Fig. 7E;n = 37 CAP+ and 32 CAP– neurons) DRG neurons. Asignificant interaction was also detected on the decay of theevoked Ca²⁺ transient when neurons were grouped according toIB₄ binding (P < 0.05); the influence of CPA was larger inIB₄+ (n = 40) compared to IB_4– (n = 29) DRGneurons (Fig. 7D).

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Figure 7. SERCA plays larger role in regulation of evoked Ca²⁺ transients in large-diameter, IB_4– and CAP– neurons
Typical evoked Ca²⁺ transients in small- (A) and large- (B) diameter DRG neurons were obtained before and during perfusion with normal bath solution containing 5 µM CPA, an inhibitor of sarco/endoplasmic reticulum Ca²⁺ ATPase. Pooled data for CPA-treated neurons are plotted, illustrating the influence of CPA on the magnitude (left) and decay (right) of evoked Ca²⁺ transients in subpopulations of neurons defined by cell body size (C, n = 44, 9, and 16 in small-, medium-, and large-diameter groups, respectively), IB₄ binding (D, n = 40 in IB₄+ and 29 in IB_4– groups) and CAP sensitivity (E, n = 37 in CAP+ and 32 in CAP– groups). Data from control neurons have been omitted for clarity. Data in each panel were analysed as in Figure 4 with a two-way ANOVA revealing significant main effects associated with subpopulation and CPA in each analysis. Post hoc analysis was performed if there was a significant interaction between main effects (subpopulation and CPA). Statistically significant differences between groups are indicated (** P < 0.01).

PMCA contributes minimally to the regulation of evoked Ca²⁺ transients in large-diameter, IB_4– and CAP– DRG neurons

Because Ca²⁺ efflux via plasma membrane Ca²⁺ ATPase (PMCA) mayinfluence both the magnitude and decay of evoked increases in[Ca²⁺]_i (Thayer et al. 2002), the contribution of PMCA to theregulation of evoked Ca²⁺ transients among subpopulation ofDRG neurons was determined. PMCA activity depends on directinteraction with calmodulin (Carafoli, 1992). It is thereforepossible to block PMCA activity by blocking calmodulin binding.A peptide inhibitor, C28R2, has been developed for such a purpose(Enyedi et al. 1991; Enyedi & Penniston, 1993), and wasused in the present study. C28R2 was commercially synthesizedand chemically cross-linked to the viral transduction protein,TAT. Ca²⁺ transients were evoked in neurons that were preincubated(30 min) with 2 µM TAT-C28R2. Data for drug treatmentwere collected from 32 small-, 15 medium- and 8 large-diameterneurons, which included 35 IB₄+ and 20 IB_4– neurons or30 CAP+ and 25 CAP– neurons. Control experiments wererun in parallel and involved coverslips of DRG neurons thatwere handled identically, except for the omission of C28R2.Data for control were collected from 22 small-, 13 medium- and11 large-diameter neurons, which included 20 IB₄+ and 26 IB_4–neurons or 20 CAP+ and 26 CAP– neurons. Two-way analysisof variance of pooled data (Fig. 8) revealed significant drugeffect on both the magnitude (P < 0.05) and decay (P <0.05) of evoked Ca²⁺ transients in each subpopulation of DRGneuron studied. There was a significant (P < 0.05) interactionbetween IB₄ binding and the influence of C28R2 on the magnitudeof the high-K⁺-evoked Ca²⁺ transients, which were larger inIB₄+ neurons in the presence of the drug than in IB_4–neurons. In order to determine whether the visual impressionthat C28R2 had little influence on large-diameter and IB_4–DRG neurons had statistical support, data were reanalysed asa percentage of control with one-way ANOVA (for size) or student'st tests (for IB₄ and CAP). Results of this analysis indicatedthat the influence of C28R2 was greater in medium-diameter (P< 0.05) and IB₄+ (P < 0.01) neurons than in larger-diameterneurons and IB_4– neurons, respectively.

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Figure 8. PMCA plays larger role in regulation of evoked Ca²⁺ transients in IB₄+ neurons
PMCA was blocked by 30 min preincubating neurons with the PMCA-specific peptide inhibitor C28R2 (2.0 µM). Control neurons were run in parallel. Pooled data for both control (filled bars) and drug treated (open bars) neurons are plotted, illustrating the influence of C28R2 on the magnitude (left) and decay (right) of evoked Ca²⁺ transients in subpopulations of neurons defined by cell body size (A), IB₄ binding (B) and CAP sensitivity (C). Data in each panel were analysed as in Fig. 4 with a two-way ANOVA revealing significant main effects associated with subpopulation and C28R2 in each analysis. Post hoc analysis was performed if there was a significant interaction between main effects (subpopulation and C28R2). Statistically significant differences between groups are indicated (*P < 0.05). Data for C28R2 treatment were collected from 32 small-, 15 medium- and 8 large-diameter DRG neurons, which included 35 IB₄+, and 20 IB_4– neurons, or 30 CAP+ and 25 CAP– neurons. Data for control were collected from 22 small-, 13 medium- and 11 large-diameter DRG neurons, which included 20 IB₄+, and 26 IB_4– neurons or 20 CAP+ and 26 CAP– neurons.

NCX contributes minimally to the regulation of evoked Ca²⁺ transients in large-diameter, IB_4– and CAP– neurons

Ca²⁺ efflux via plasma membrane Na⁺/Ca²⁺ exchangers (NCX) isanother mechanism that may influence the magnitude and decayof evoked Ca²⁺ transients. Therefore, the role of NCX in theregulation of evoked Ca²⁺ transients among subpopulation ofDRG neurons was assessed. NCX was inhibited by replacing extracellularNa⁺ with Li⁺ (Verdru et al. 1997). Examples of evoked Ca²⁺ transientsin small- (Fig. 9A) and large- (Fig. 9B) diameter DRG neuronswere obtained before and during perfusion with bath solutionin which Na⁺ had been replaced by Li⁺. Li⁺ did not change resting[Ca²⁺]_i. Two-way ANOVA revealed a significant drug effect onboth the magnitude (P < 0.05) and decay (P < 0.01) ofevoked Ca²⁺ transients in all three subpopulations of DRG neuronsanalysed. There were also significant interactions between subpopulationand drug effects on the magnitude of evoked Ca²⁺ transientswhen neurons were grouped according to IB₄ binding (P < 0.01)and CAP sensitivity (P < 0.01); Li⁺ had a larger effect onthe magnitude in IB₄+ (n = 31) and CAP+ (n = 29)neurons than in IB_4– (n = 19) and CAP– (n =21) neurons, respectively (Fig. 9D and E). In addition, a significantinteraction between subpopulation and drug effects on the decay(P < 0.01) of evoked Ca²⁺ transients was detected; post hocanalysis revealed that the Li⁺-induced increase in decay wasgreater (P < 0.05) in medium- than in large-diameter neurons(Fig. 9C; n = 28 in small-, 13 in medium- and 9 in large-cellgroups), in IB₄+ (P < 0.01) than in IB_4– neurons, andin CAP+ (P < 0.01) than in CAP– neurons (Fig. 9D and E).

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Figure 9. Na⁺/Ca²⁺ exchange regulates evoked Ca²⁺ transients in IB₄+ and CAP+ neurons
Typical evoked Ca²⁺ transients in small- (A) and large-diameter (B) DRG neurons were obtained before and during perfusion with bath solution in which Na⁺ had been replaced by Li⁺. Pooled data illustrating the influence of Li⁺ on the magnitude (left) and decay (right) of evoked Ca²⁺ transients in subpopulations of neurons defined by cell body size (C, n = 28, 13, and 9 in small-, medium-, and large-diameter groups, respectively), IB₄ binding (D, n = 31 in IB₄+ and 19 in IB_4– groups) and CAP sensitivity (E, n = 29 in CAP+ and 21 in CAP– groups). Data from control neurons were omitted for clarity. Data in each panel were analysed as in Fig. 4 with a two-way ANOVA revealing significant main effects associated with subpopulation and Li⁺ in each analysis. Post hoc analysis was performed if there was a significant interaction between main effects (subpopulation and Li⁺). Statistically significant differences between groups are indicated (*P < 0.05, ** P < 0.01).

Mitochondria regulate evoked Ca²⁺ transients in all subpopulations of DRG neurons

With both Ca²⁺ transporter (uniporter) and Na⁺/Ca²⁺ exchangers(MNCX), mitochondria may contribute to both uptake or releaseCa²⁺, and therefore are involved in the buffering of [Ca²⁺]_i.Bath application of 10 µM CCCP was used to disrupt mitochondrialproton gradient and block both uptake and release of Ca²⁺ frommitochondria (Kostyuk et al. 1999). Typical examples of evokedCa²⁺ transients in small- (Fig. 10A) and large- (Fig. 10B) diameterDRG neurons were obtained before and during perfusion with normalbath solution containing 10 µM CCCP. Pooled data are shownin Fig. 10C–E. Two-way ANOVA revealed a significant drugeffect on both the magnitude (P < 0.01) and decay (P <0.01) of evoked Ca²⁺ transients in all subpopulations of DRGneurons assessed. Furthermore, there was a significant interactionbetween the effects of subpopulation and drug with respect tothe influence of CCCP on the magnitude of evoked Ca²⁺ transientwhen neurons were analysed according to cell body size (P <0.01) and IB₄ binding (P < 0.05): the effects of CCCP werelarger in medium- (n = 6, P < 0.01) and large- (n =9, P < 0.01) diameter neurons than in small-diameter neurons(n = 18) (Fig. 10C) and in IB_4– (n = 15) neuronscompared to IB₄+ (n = 18) neurons (Fig. 10D, P < 0.01).CCCP also caused an initial increase in resting [Ca²⁺]_i, whichdeclined to some extent with time, but did not returned to thelevels prior to CCCP application.

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Figure 10. Mitochondria regulate evoked Ca²⁺ transients in all subpopulations of DRG neurons
Typical evoked Ca²⁺ transients in small- (A) and large- (B) diameter DRG neurons were obtained before and during perfusion with normal bath solution containing 10 µM CCCP, which disrupts mitochondrial proton gradient and blocks both uptake and release of Ca²⁺ from mitochondria. Pooled data illustrating the influence of CCCP on the magnitude (left) and decay (right) of evoked Ca²⁺ transients in subpopulations of neurons defined by cell body size (C, n = 18, 6, and 9 in small-, medium-, and large-diameter groups, respectively), IB₄ binding (D, n = 18 in IB₄+ and 15 in IB_4– groups) and CAP sensitivity (E, n = 14 in CAP+ and 19 in CAP– groups). Data from control neurons were omitted for clarity. Data in each panel were analysed as in Fig. 4 with a two-way ANOVA revealing significant main effects associated with subpopulation and CCCP in each analysis. Post hoc analysis was performed if there was a significant interaction between main effects (subpopulation and CCCP). Statistically significant differences between groups are indicated (** P < 0.01).

Differences among subpopulations with respect to store-operated Ca²⁺ entry

In addition to initial Ca²⁺ influx through VGCCs and consequentCa²⁺ release via RyRs from intracellular Ca²⁺ stores, store-operatedCa²⁺ entry (Usachev & Thayer, 1999) may also contributeto depolarisation-induced increase in [Ca²⁺]_i in DRG neurons.In order to determine whether the differences among subpopulationsof DRG neurons with respect to evoked Ca²⁺ transients reflecta difference in store-operated Ca²⁺ entry, store-operated Ca²⁺entry was measured in subpopulations of DRG neurons. Store-operatedCa²⁺ entry was induced by brief (20 s) application of normalbath solution (which contained 2.5 mM Ca²⁺) in DRG neurons 10min after depleting intracellular Ca²⁺ stores by treating neuronswith 10 µM CPA in Ca²⁺-free bath solution. Representativerecordings in Fig. 11A and B shows store-operated Ca²⁺ entryin small- and in large-diameter DRG neurons. Pooled data areplotted in Fig. 11C–E. The magnitude of the Ca²⁺ transientwas significantly larger in small- (n = 37) than in medium-(n = 15, P < 0.05) or large- (n = 12, p <0.05) diameter DRG neurons, and the decay of the Ca²⁺ transientwas significantly slower in small-diameter than in medium-diameterneurons (P < 0.05; one-way ANOVA). The magnitude of the Ca²⁺transient was larger (P < 0.01) and the decay slower (P <0.05) in IB₄+ (n = 39) and CAP+ (n = 36) DRG neuronsthan in IB_4– (n = 25) or CAP– (n = 28)neurons, respectively (Student's t test).

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Figure 11. Store-operated Ca²⁺ entry among subpopulations of DRG neurons
Store-operated Ca²⁺ entry was induced with a brief (20 s) application of bath solution containing 2.5 mM Ca²⁺ after the treatment of neurons with Ca²⁺-free solution containing 10 µM CPA. Shown in A and B are examples of such recordings made from small- (A) and large- (B) diameter DRG neurons. Pooled data illustrating the magnitude (left) and decay (right) of the Ca²⁺-induced increase in [Ca²⁺]_i in subpopulations of neurons defined by cell body size (C), IB₄ binding (D) and CAP sensitivity (E) are plotted. Data in C (n = 37, 15, and 12 in small-, medium-, and large-diameter groups, respectively) were analysed with a one-way ANOVA, while data in D (n = 39 in IB₄+ and 25 in IB_4– groups) and E (n = 36 in CAP+ and 28 in CAP– groups) were analysed with a Student t test. Statistically significant differences between groups are indicated (*P < 0.05, ** P < 0.01).

	Discussion

Top Abstract Introduction Methods Results Discussion References

This study constitutes the first systematic analysis of evokedCa²⁺ transients among subpopulations of DRG neurons. One ofthe most striking observations to arise from this analysis isthat while there are no statistically significant differencesamong subpopulations of DRG neurons with respect to resting[Ca²⁺]_i, there are marked differences among subpopulations withrespect to both the magnitude and decay of evoked Ca²⁺ transients.The magnitude of the evoked increase in [Ca²⁺]_i was the largest,and the decay was the slowest in small-diameter, IB₄+ and CAP+neurons while the magnitude was the smallest and the decay mostrapid in large-diameter, IB_4– and CAP– DRG neurons.Similar results were also observed in cutaneous DRG neurons(DiI+) innervating the hindpaw when classified according tocell body diameter, IB₄ binding or CAP responsiveness. Importantly,similar results were also observed if Ca²⁺ transients were evokedwith voltage steps. These observations suggested that thereare differences among subpopulations of DRG neurons with respectto the mechanisms underlying the regulation of [Ca²⁺]_i. Consequently,we assessed the contribution of a number of Ca²⁺ regulatorymechanisms to the magnitude and decay of evoked Ca²⁺ transientsamong subpopulations of DRG neurons. Results from this secondseries of experiments indicated that there are marked differencesbetween subpopulations of DRG neurons with respect to a numberof Ca²⁺ regulatory mechanisms including (1) voltage-gated Ca²⁺currents; (2) RyR-mediated CICR; (3) SERCA; (4) PMCA; (5) NCX;and (6) store-operated Ca²⁺ entry.

The majority of the results in this study were obtained fromintact (i.e. unclamped) neurons. It is important to point outthat the study of unclamped neurons may have influenced ourresults in two important ways. First, in unclamped neurons,there may be differences between subpopulations of neurons withrespect to resting membrane potential. Consistent with thissuggestion, there was a trend in the current-clamp data setsuggesting that the resting membrane potential was smallestin small-diameter neurons and largest in large-diameter neurons,and while the differences between groups in the present studywere not statistically significant, we have reported that thereare small, but significant differences between groups with respectto resting membrane potential (Gold et al. 1996). Resting membranepotential may influence high-K⁺-evoked Ca²⁺ transients in twogeneral ways: (1) by influencing the availability of voltage-gatedCa²⁺ channels, most dramatically low threshold, or T-type channelsthat are subject to steady-state inactivation; and (2) by influencingthe availability of channels that have an impact on the excitatoryresponse to membrane depolarisation, as both voltage-gated Na⁺current responsible for the upstroke of the action potentialand voltage-gated K⁺ currents that contribute to the downstrokeof the action potential as well as the duration of the afterhyperpolarizationare subject to steady-state inactivation. Second, variabilityin the action potential barrage and/or the time to membranepotential stabilization could have an impact on the magnitudeof Ca²⁺ influx during this period of membrane potential instability,as well as the number of Ca²⁺ channels mediating influx duringthe plateau phase of the high-K⁺-evoked membrane depolarization.Both of these factors may have contributed to variability inour data set as well as differences between subpopulations.Furthermore, it is possible that experimental manipulationsdesigned to assess the impact of various influx, efflux andrelease pathways, influenced resting membrane potential and/orspike adaptation, and therefore, may have had an indirect influenceon the magnitude and decay of the evoked Ca²⁺ transient. Conclusionsdrawn from these results are therefore made with caution.

While we acknowledge that the lack of clamp control may haveinfluenced the magnitude and decay of the high-K⁺-evoked Ca²⁺transient in DRG neurons, we believe that the lack of clampcontrol is unlikely to have contributed significantly to theobserved differences between subpopulations of DRG for the followingreasons. First, our current-clamp data suggest that ‘clampcontrol’ was surprisingly good in the majority of neuronsstudied as high K⁺ evoked more than two action potentials inonly half of the small-diameter neurons studied, less than one-thirdof the medium-diameter neurons and none of the large-diameterneurons. Sustained activity was only observed in two medium-diameterneurons. Second, if one assumed that high-K⁺-evoked action potentialsresulted in larger and more slowly decaying Ca²⁺ transients,one would predict that a subpopulation of small-diameter DRGneurons might have evoked Ca²⁺ transients that were similarto those observed in large-diameter DRG neurons. Yet the meanevoked increase in the lower quartile of small-diameter neurons(179 ± 11 nM), presumably reflecting small-diameter neuronsthat did not fire action potentials, was still statisticallysignificantly larger than that in larger-diameter neurons. Third,Ca²⁺ transients evoked with voltage steps resulted in mean datathat were qualitatively and quantitatively similar to thoseobserved with high-K⁺-evoked transients. And fourth, other investigatorshave also reported that evoked Ca²⁺ transients in unclampedDRG neurons are similar to evoked responses under voltage clamp(Werth et al. 1996; Usachev et al. 2002). It should also benoted the responses in unclamped neurons may be a better reflectionof Ca²⁺ regulation in vivo, given the potential deleteriousimpact associated with the electrical access necessary for voltageclamp.

Our results indicate that there is a differential distributionof voltage-gated Ca²⁺ current density among subpopulations ofDRG neurons. HVACC were present in the highest density in large-diameter,IB_4–, CAP– DRG neurons, and in the smallest densityin small-diameter, IB₄+, CAP+ DRG neurons. Thus, the distributionof HVACC cannot account for the differences among subpopulationswith respect to high-K⁺-evoked Ca²⁺ transients. Rather, theysuggest that if HVACC is the primary Ca²⁺ influx pathway responsiblefor initiating the Ca²⁺ transient in response to high K⁺, thenthere must be mechanisms to amplify Ca²⁺ transients in somesubpopulations of DRG neurons (i.e. small-diameter) and/or attenuateCa²⁺ transients in other subpopulations of DRG neurons (i.e.large-diameter). Because LVACC were the highest in density inmedium-, smaller in small- and