Electrical Synapses Mediate Signal Transmission in the Rod Pathway of the Mammalian Retina

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The Journal of Neuroscience, December 15, 2002, 22(24):10558-10566

Electrical Synapses Mediate Signal Transmission in the Rod Pathway of the Mammalian Retina
Margaret Lin Veruki and Espen Hartveit
University of Bergen, Department of Anatomy and Cell Biology, N-5009 Bergen, Norway

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the retina, AII (rod) amacrine cells are essential for integrating rod signals into the cone pathway. In addition to beinginterconnected via homologous gap junctions, these cells makeextensive heterologous gap junctions with ON-cone bipolar cells(BCs). These gap junctions are the pathway for transfer of rodsignals to the ON-system. To investigate the functional propertiesof these gap junctions, we performed simultaneous whole-cell recordingsfrom pairs of AII amacrine cells and ON-cone bipolar cells inthe in vitro slice preparation of the rat retina. We demonstratestrong electrical coupling with symmetrical junction conductance(~1.2 nS) and very low steady-state voltage sensitivity. However,signal transmission is more effective in the direction from AIIamacrine cells to ON-cone bipolar cells than in the other direction.This functional rectification can be explained by a correspondingdifference in membrane input resistance between the two cell types.Signal transmission has low-pass filter characteristics with increasingattenuation and phase shift for increasing stimulus frequency.Action potentials in AII amacrine cells evoke distinct electricalpostsynaptic potentials in ON-cone bipolar cells. Strong and temporallyprecise synchronization of subthreshold membrane potential fluctuationsare commonlyobserved.

Key words: gap junctions; electrical synapses; rod pathway; AII amacrine cells; bipolar cells; retina; synaptic transmission

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Networks of inhibitory interneurons in several regions of the CNS are extensively interconnected by electrical synapses. Themajor structural elements of these synapses are gap junctions,specialized intercellular contacts formed by a family of transmembraneproteins termed connexins (Kumar and Gilula, 1996). Most of theelectrical synapses are formed by gap junctions between neuronsof the same type (homologous gap junctions). In contrast, heterologouscoupling might be relatively rare (Galarreta and Hestrin, 2001).The retina provides striking examples of populations of neuronsthat make both homologous and heterologous gap junctions, suchas AII (rod) amacrine cells. AII amacrine cells are essentialfor integrating rod signals into the cone pathway and are interconnectedby gap junctions (Kolb and Famiglietti, 1974), thereby forminga network of electrically coupled neurons (Veruki and Hartveit,2002). In addition to these homologous gap junctions, AII amacrinecells make extensive heterologous gap junctions with ON-cone bipolarcells (BCs) (Kolb and Famiglietti, 1974; McGuire et al., 1984;Strettoi et al., 1992, 1994; Chun et al., 1993). These connectionsare the pathway through which rod signals are conveyed to theON-system. There is strong evidence that the neuron-specific connexin36is expressed by AII amacrine cells and is the subunit of the homologousgap junctions (Feigenspan et al., 2001; Mills et al., 2001). Importantly,the heterologous gap junctions made with ON-cone bipolar cellsare thought to be heterotypic, because ON-cone bipolar cells donot seem to express connexin36 (Feigenspan et al., 2001; Millset al., 2001). Although the electrical synapses between AII amacrinecells were analyzed recently in detail (Veruki and Hartveit, 2002),little is known about the functional characteristics and preciserole of electrical synapses between AII amacrine cells and ON-conebipolar cells. For example, is the electrical junction conductancelarge enough that action potentials in AII amacrine cells canbe transmitted to bipolar cells? Are the synapses symmetricalor is there evidence for rectification? What are the consequencesof the difference in cell size and membrane input resistance betweenAII amacrine cells and bipolar cells? To which extent will theelectrical synapses synchronize the membrane potentials betweenAII amacrine cells and bipolar cells? As a first step toward unravelingthe operational characteristics of this microcircuit, we haveperformed simultaneous dual recordings from pairs of such cellsin an in vitro slice preparation of the rat retina. We demonstratestrong, bidirectional electrical coupling between AII amacrinecells and ON-cone bipolar cells with identical conductances foreach direction of coupling. However, the coupling coefficientfor transmission from AII amacrine cells to ON-cone bipolar cellsis considerably larger than for transmission in the other direction.This functional rectification can be explained by a correspondingdifference in membrane input resistance between the two typesof cells. We also demonstrate that action potentials in AII amacrinecells evoke discrete electrical postsynaptic potentials (PSPs)in ON-cone bipolar cells. Finally, the strong electrical couplingacts to tightly synchronize both oscillatory and non-oscillatorysubthreshold membrane potential fluctuations between AII amacrinecells and ON-cone bipolarcells.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Albino rats (4-7 weeks postnatal) were deeply anesthetized with halothane in oxygen and killed by cervical dislocation (procedureapproved under the surveillance of the Norwegian Animal ResearchAuthority). Detailed accounts of the methods, including preparationof retinal slices, have been published previously (Hartveit, 1997;Veruki and Hartveit, 2002). Anesthesia, dissection, and preparationof slices were done under normal room illumination. During recording,the room lights were dimmed moderately for the purpose of observingmonitor displays better. Thus, we consider the slices to be lightadapted.

The extracellular perfusing solution was bubbled continuously with 95% O₂-5% CO₂ and had the following composition (in mM):125 NaCl, 25 NaHCO₃, 2.5 KCl, 2.5 CaCl₂, 1 MgCl₂, 10 glucose,pH 7.4 (20-24°C). In relaxation experiments with measurement ofthe steady-state voltage sensitivity of the electrical junctionconductance, the extracellular solution contained 2.5 mM Co²⁺ (replacing an equimolar concentration of Ca²⁺) and 300 nM TTX to block voltage-gated membrane currents. TTXwas also added in experiments with application of sinusoidal stimulito study frequency dependence of electrical coupling. The recordingpipettes (4-6 M $Omega$ for amacrine cells; 6-9 M $Omega$ for bipolar cells)were filled with a solution containing (in mM): 140 K-gluconate,5 HEPES, 1 CaCl₂, 1 MgCl₂, 5 EGTA, 4 Na₂ATP, 0.5 GTP. In relaxationexperiments (see above), the recording pipette solution contained(in mM): 125 CsCl, 4 NaCl, 5 HEPES, 1 CaCl₂, 1 MgCl₂, 5 EGTA,15 tetraethylammonium chloride, 4 Na₂ATP, 0.5 GTP. For both intracellularsolutions, Lucifer yellow was added (1 mg/ml), and pH was adjustedto 7.3 with KOH or CsOH. The holding potentials were correctedon-line for liquid junctionpotentials.

Antagonists of chemical synaptic transmission were added directly to the external solution. The concentrations of the drugswere as follows (in µM): 30 3-((RS)-2-carboxypiperazin-4-yl)-propyl-1-phosphonicacid (Tocris Cookson, Bristol, UK), 10 6-cyano-7-nitroquinoxaline-2,3-dione(Tocris Cookson), 10 bicuculline methchloride (Tocris Cookson),500 picrotoxin (Sigma-Aldrich, St. Louis, MO), 1 strychnine (ResearchBiochemicals, Natick,MA).

Dual whole-cell recordings were made with an EPC9/2 amplifier (HEKA Elektronik, Lambrecht, Germany). The fast current-clampfeedback circuitry of the EPC9/2 was used in all current-clamprecordings. For some voltage-clamp experiments, the digital-analogconverter-stimulus template corresponded to the digitization ofa previously recorded action potential (Veruki and Hartveit, 2002).The series resistance in both cells was regularly monitored byapplying a series of 10 mV hyperpolarizing voltage pulses. Theaverage series resistance was 16 ± 1 (SEM) M $Omega$ for amacrine cells(n = 18) and 17 ± 2 M $Omega$ for bipolar cells (n = 18). Cells withseries resistance >40 M $Omega$ were excluded fromanalysis.

Data analysis was performed with PulseFit (HEKA Elektronik), Igor Pro (WaveMetrics, Lake Oswego, OR), AxoGraph (Axon Instruments,Union City, CA), and DataView (Dr. W. J. Heitler, University ofSt. Andrews, UK). To calculate the electrical junction conductance(G_j), we assumed an equivalent-circuit model and corrected forerrors introduced by non-zero series resistance and finite membraneresistance (Veruki and Hartveit, 2002). In relaxation experimentswith measurement of the steady-state voltage sensitivity of theelectrical junction conductance, the voltage steps (applied tothe presynaptic cell) were 10 sec in duration from a holding potentialof $-$ 50 mV to voltages between $-$ 120 and +10 mV (10 mV steps). LargerV_j steps could not be performed because they compromised the integrityof the cells. The time course of postsynaptic current traces wasestimated by curve fitting with a monoexponential function, I(t)= Aexp( $-$ t/ $tau$ ) + I_ss, where I(t) is the current as a function oftime, $tau$ is the time constant, I_ss is the steady-state currentamplitude, and the instantaneous current at time 0 (I₀) is equalto the sum of A and I_ss. The steady-state junctional conductanceat each V_j was normalized to the instantaneous conductance atthe same voltage, and the resulting G_j,ss values (calculated asI_ss/I₀) were plotted as a function of V_j.

Normalized cross-correlograms of continuous membrane potential recordings were calculated as the correlation of the two recordsdivided by the number of points and the SD of each voltage record.Accordingly, the cross-correlation amplitude can vary between+1 and $-$ 1 and depends only on the degree of synchrony betweenthe voltage records and not on their absolute amplitude. Sliding,color-coded two-dimensional (2D) cross-correlograms of pairs ofvoltage records of duration T seconds were calculated from consecutivepairs of data segments, each of 500 msec duration, and shifted100 msec forward in time relative to the previous segment. Eachsegment was mean-subtracted before calculating the cross-correlation,which is therefore mathematically equivalent to the cross-covariance.A matrix was then constructed in which consecutive 1D cross-correlationfunctions constitute consecutive columns with time running alongthe x-axis and the time lag of the correlation function runningalong the y-axis. The normalized correlation amplitude was codedby color. The time-averaged cross-correlogram was calculated asthe average of each row of the 2D cross-correlogram. All cross-correlogramswere calculated with the bipolar cell as the nonreference celland the AII amacrine cell as the referencecell.

Statistical analyses were performed with Student's two-tailed t tests, with a level of significance of p < 0.05 (unpaired,unless otherwise stated). Data are presented as means ± SEM (n= number of cells or cellpairs).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of AII amacrine and ON-cone bipolar cells in retinal slices

All recordings were aimed at pairs of AII amacrine cells and presumed ON-cone bipolar cells in rat retinal slices (Fig. 1).Although AII amacrine cells constitute a homogeneous populationof cells (Wässle et al., 1993), ON-cone bipolar cells are a heterogeneousgroup encompassing four to five cell types (Euler et al., 1996;Hartveit, 1997). Although it is not possible to target ON-conebipolar cells for recording with absolute confidence, the cellbodies of these cells tend to be located distally in the innernuclear layer but proximally to the cell bodies of the rod bipolarcells (Euler and Wässle, 1995). All cells were filled with Luciferyellow, and at the end of each recording, fluorescence microscopyallowed visualization of both cells (Fig. 1, bottom). Cells wereclassified by direct, visual observation of fluorescent imagesat the microscope. In this way it was possible to visually traceand identify the processes belonging to each cell. In some cases,it was necessary to withdraw the pipette from the AII amacrinecell. This led to a rapid leakage of Lucifer yellow and stronglyreduced the staining of this cell, such that the bipolar cellcould be observed in isolation and then classified properly. Inaddition, each cell pair was carefully drawn by hand, and somecell pairs were photographed at a series of focal planes (Hartveit,1997). For AII amacrine cells, the morphological characteristicsincluded lobular appendages and arboreal dendrites. For bipolarcells, they included a dendrite ascending to the outer plexiformlayer and an axon descending to the inner plexiform layer witha branching pattern and stratification level of the axon terminalsystem specific for each type. ON-cone bipolar cells were identifiedas having axons stratifying in stratum 3 (S3), S4, or S5 of theinner plexiform layer and were classified according to the followingcriteria (Euler and Wässle, 1995; Hartveit, 1997). Type 5 and6 cells have narrowly stratifying axon terminals located directlydistal (type 5) or directly proximal (type 6) to the inner cholinergicband, which can be visualized regularly as an optically denseband with differential interference contrast optics (Euler andWässle, 1995). Type 7 cells have a more diffusely stratifyingaxon terminal, centered at the same level as the axon terminalof type 6 cells (approximately at the border between S3 and S4).Type 8 cells have an axon terminal that branches proximally inS4 and descends into S5. We did not record from type 9 cone bipolarcells. OFF-cone bipolar cells were identified as having axon terminalsstratifying in S1 or S2 of the inner plexiform layer. Rod bipolarcells were identified by one or two larger swellings at the axonterminal in S5.

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Figure 1. Visualization of simultaneously recorded AII amacrine cells and ON-cone bipolar cells. Top two panels, An AII amacrine cell (bottom arrows) and a type 7 ON-cone bipolar cell (top arrows) in an in vitro slice from rat retina, visualized with infra-red differential interference contrast videomicroscopy. In the left panel, the ON-cone bipolar cell is in focus; in the right panel, the AII amacrine cell is in focus. Bottom, Composite fluorescence photomicrograph of same cell pair after filling with Lucifer yellow. The level of stratification of the axon terminal of the ON-cone bipolar cell is indicated by an arrow. Scale bars, 10 µm.

Electrical coupling of AII amacrine cells and ON-cone bipolar cells

With a pair of cells in whole-cell voltage clamp, we tested for electrical coupling by applying voltage commands to one celland recording the current responses in both cells. A cell is referredto as presynaptic when it is the cell in which an experimentalmanipulation is initiated and as postsynaptic when it respondsto a membrane potential change in the presynaptic cell (Nolanet al., 1999). Application of a hyperpolarizing voltage step evokedan inward current in the presynaptic cell, and when cells wereelectrically coupled it also evoked an outward current in thepostsynaptic cell (Fig. 2A,B). Application of a depolarizing voltagestep evoked an outward current in the presynaptic cell and aninward current in the postsynaptic cell (Fig. 2A,B). Recordingswere performed in the presence of antagonists of chemical neurotransmittersto isolate the effects of electrical coupling from chemical synaptictransmission (see Materials and Methods). In addition, where appropriate,experiments were repeated in control solution without antagoniststo verify that the results obtained did not depend on blockedchemical synaptic transmission as such. For all cell pairs, theelectrical coupling was reciprocal.

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Figure 2. Junction conductance of electrical synapses between AII amacrine cells and ON-cone bipolar cells. A, With a cell pair in voltage clamp (V_h = $-$ 60 mV), 300 msec voltage pulses (V) of $-$ 20, $-$ 10, and +15 mV are applied to the AII amacrine cell while current responses are recorded from both cells (I_AII and I_BC). Hyperpolarizing pulses applied to the AII amacrine cell result in inward currents in this cell and outward currents in the bipolar cell (type 7). A depolarizing pulse in the AII amacrine cell results in an outward current in this cell and an inward current in the bipolar cell. Here and in subsequent figures, the recording configuration is drawn with the AII amacrine cell on the left and the ON-cone bipolar cell on the right. B, Same as in A, but voltage pulses are applied to the bipolar cell (V). C, Current-voltage relationship for the junctional current (I_j) versus the junctional voltage (V_j) for cell pair in A and B; voltage pulses (from $-$ 20 to +20 mV, 5 mV increments) applied to AII amacrine cell (as in A). The data points have been fit with a straight line (slope = G_j). D, Same as in C, but voltage pulses applied to bipolar cell (as in B). E, Comparison of G_j in each direction indicates nonrectifying electrical coupling [G_{j (BC} _AII) for bipolar cell presynaptic; G_{j (AII} _BC) for AII amacrine cell presynaptic]. The dashed line has a slope of 1 [G_{j (BC} _AII) = G_{j (AII} _BC)]. F, Relaxation experiments to determine steady-state voltage sensitivity of electrical junction conductance between two coupled cells. Experimental paradigm as in A and B, but presynaptic voltage pulses are 10 sec in duration ( $-$ 60 to +60 mV, 10 mV increments). Traces illustrate postsynaptic current responses (I_AII) with voltage pulses applied to the bipolar cell (left, type 8) and postsynaptic current responses (I_BC) with voltage pulses applied to the AII amacrine cell (right). Note that for larger amplitude voltage pulses, there is slight decay of postsynaptic currents toward a (non-zero) steady-state level. Dashed lines indicate baseline current. G, Plot of steady-state junctional conductance (G_j,ss) as a function of V_j. G_j,ss at each V_j is plotted as mean ± SEM. Data points are normalized to the instantaneous value at each V_j. Data for each direction of coupling are plotted separately, with either an AII amacrine cell ( $open circle$ ) or a bipolar cell () postsynaptic.

A total of 31 AII amacrine-ON-cone bipolar cell pairs displayed electrical coupling as described above. After fluorescencemicroscopy and visualization with Lucifer yellow, all cell pairswere observed to be in potential physical contact with each otheras judged by overlap between the arboreal dendrites of the AIIamacrine cell and the arborization of the axon terminal of theON-cone bipolar cell. The ON-cone bipolar cells were classified(Euler and Wässle, 1995) as type 5 (n = 3), type 6 (n = 3), type7 (n = 15), and type 8 (n = 7). We also recorded two coupled pairsin which the bipolar cell was either a type 5 or 6 and one coupledpair in which the bipolar cell could not be visualized adequately.Two AII amacrine-ON-cone bipolar cell pairs did not display electricalcoupling and subsequently, after visualization, were found tohave nonoverlapping processes. We also recorded from cell pairsin which only one member of the pair was either an AII amacrinecell or an ON-cone bipolar cell. Electrical coupling was neverobserved between suchcells.

Electrical junction conductance

With both cells in voltage clamp, we estimated the junction conductance (G_j) by applying a series of voltage commands to thepresynaptic cell and recording the evoked currents in both thepresynaptic and the postsynaptic cell (Fig. 2A,B). The junctioncurrent (I_j) versus junction voltage (V_j) relationship, correctedfor non-zero series resistance and finite membrane input resistance,was linear (Fig. 2C,D), indicating that G_j was independent ofV_j over the range of voltages (±20 mV) and pulse durations (500msec) tested. Accordingly, G_j was measured as the slope of a straightline fitted to the I-V relation [1362 pS (Fig. 2C); 1399 pS (Fig.2D)]. The junctional conductance was very similar for both directionsof coupling (Fig. 2E). The mean G_j was 1203 ± 158 pS for couplingfrom AII amacrine cells to ON-cone bipolar cells (n = 18 cellpairs; range, 102-3353 pS) and 1206 ± 148 pS for coupling fromON-cone bipolar cells to AII amacrine cells (range, 109-3124 pS).When the cell pairs were classified according to the type of bipolarcell in each pair (n = 16 cell pairs), the mean G_j values wereas follows (G_j averaged for both directions of coupling): 106and 646 pS (type 5), 596 and 1379 pS (type 6), 1233 ± 83 pS (type7; n = 7), and 1414 ± 460 pS (type 8; n = 5). There was no statisticallysignificant difference between type 7 and type 8 cell pairs (p= 0.66). Type 5 and type 6 cell pairs were not included in thestatistical comparisons because of limited sample sizes. G_j wasquite stable over the duration of recording (typically 20-30min).

Voltage sensitivity of electrical junction conductance

The voltage sensitivity of the steady-state electrical junction conductance (G_j,ss) was examined by applying 10-sec-long voltagepulses to the presynaptic cell and measuring the evoked currentin the postsynaptic cell. The transjunctional voltage (V_j) wasvaried from $-$ 70 or $-$ 60 mV to +60 mV. Within this voltage range,there was little dependence of G_j,ss on V_j. Figure 2F shows postsynapticcurrent families in an AII amacrine cell and an ON-cone bipolarcell, while voltage pulses were applied to the corresponding presynapticcell. For V_j < $-$ 40 mV and V_j > +40 mV, there was slight relaxationof the postsynaptic current. Figure 2G shows the resulting G_j,ssversus V_j for data pooled from three to six cell pairs. Becauseof the limited range of V_j values tested, no attempt was madeto fit the G_j,ss versus V_j data to a Boltzmann relationship (Sprayet al., 1981).

Coupling coefficient

In current clamp, a current step in the presynaptic cell evoked a presynaptic and postsynaptic voltage change of the samepolarity, as expected for transmission via electrical synapses(Fig. 3A,B). For each cell pair and for each direction of coupling,a coupling coefficient was calculated as the ratio of the voltagechange in the noninjected cell to that in the injected cell. Whenthe two directions of coupling were compared, coupling was foundto be consistently asymmetric (Fig. 3C). The mean steady-statecoupling coefficient in the direction AII $right-arrow$ ON-cone bipolar cellwas 0.61 ± 0.04 (n = 9 cell pairs), whereas the mean steady-statecoupling coefficient in the direction ON-cone bipolar cell $right-arrow$ AIIwas 0.30 ± 0.03 (same nine cell pairs). To quantify the apparentrectification, we calculated the ratio of the higher to the lowercoupling coefficient for each cell pair (i.e., the K ratio) (Nolanet al., 1999). The mean K ratio was 2.2 ± 0.2. This rectificationcannot be accounted for by the junction conductance, which wassymmetrical (Fig. 2E). An alternative explanation for the asymmetricalcoupling coefficient is a difference in membrane input resistance(reflecting the difference in cell size) between the two coupledcells (441 ± 36 M $Omega$ for AII amacrine cells; 1030 ± 112 M $Omega$ for ON-conebipolar cells). We investigated this by plotting the K ratio foreach coupled pair against the ratio of postsynaptic to presynapticmembrane input resistances (calculated in the direction of thelarger coupling coefficient) (Fig. 3D). The result suggests thatthe asymmetry of coupling coefficients can be well accounted forby the difference in membrane input resistance. For seven of thesecoupled cell pairs, we repeated the measurements in control solutionwithout blockers. There was no statistically significant differencein the K ratio between the two conditions (K ratio with blockers,1.8 ± 0.2; K ratio without blockers, 1.7 ± 0.2; p = 0.3; pairedt test). Thus, the asymmetry did not depend on the presence ofblockers of chemical synaptic transmission.

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Figure 3. Estimation of coupling coefficients between electrically coupled cells. A, With both cells in current clamp, 500 msec current pulses (I) of $-$ 50, $-$ 25, and +50 pA are applied to the AII amacrine cell while voltage responses are recorded from both cells (V_AII, V_BC). Injection of negative current results in hyperpolarization of both cells, and injection of positive current results in depolarization of both cells. B, Same as in A, but current pulses of $-$ 20, $-$ 10, and +20 pA are applied to the bipolar cell (type 6). C, Comparison of coupling coefficients in each direction indicates apparent rectification for all cell pairs (BC $right-arrow$ AII for bipolar cell presynaptic; AII $right-arrow$ BC for AII amacrine cell presynaptic). The straight line has a slope of 1 (i.e., coupling coefficient is the same in both directions). D, Relation between apparent rectification (K ratio) and input resistance ratio. The continuous line represents the values expected when pairs of cells are connected by asymmetrical coupling coefficients and input resistances, but symmetrical G_j. The horizontal and vertical dashed lines represent values expected when pairs of cells have identical coupling coefficients and input resistances, respectively.

Frequency dependence of electrical synaptic transmission

Electrical coupling between nerve cells can have the functional characteristics of a low-pass filter (Bennett, 1977). To investigatethis we applied sinusoidal current stimuli of varying frequency(1-100 Hz) to electrically coupled cell pairs while recordingthe voltage modulation in both cells (Fig. 4A,B). For each frequencywe calculated the coupling coefficient and the phase shift forboth directions of coupling (Veruki and Hartveit, 2002). The couplingcoefficient at each frequency was normalized to the coupling coefficientfor steady-state responses in the same direction for the samecell pair. The signal transmission in both directions of couplinghad clear low-pass characteristics, with increasing attenuationand phase shift for increasing stimulus frequency. Furthermore,the transmission characteristics for each direction of couplingclosely mirrored each other (Fig. 4C).

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Figure 4. Electrical coupling between AII amacrine cells and ON-cone bipolar cells displays transmission characteristics of a low-pass filter. A, B, Increasing phase lag and response attenuation between the voltage oscillations evoked in the presynaptic and postsynaptic cells of a coupled pair when injecting sinusoidal current stimuli of increasing frequency in the presynaptic cell. A, AII amacrine cell presynaptic (current stimulus 100 pA peak-to-peak amplitude) and bipolar cell (type 6) postsynaptic (each trace is the average of 3-9 sweeps). Horizontal calibration bar indicates duration of one stimulus period (250 msec for 4 Hz, 25 msec for 40 Hz, and 10 msec for 100 Hz; A, B). B, Same as in A, but bipolar cell presynaptic (current stimulus 30 pA peak-to-peak amplitude) and AII amacrine cell postsynaptic (each trace is the average of 3-9 sweeps). C, Bode plot showing frequency dependence of response attenuation (coupling coefficient normalized to steady-state coupling coefficient) and phase lag of sinusoidal voltage response for both directions of coupling (n = 6 cell pairs).

Electrical postsynaptic potentials and signal transmission between coupled cells

Spike generation between pairs of AII amacrine cells can be synchronized precisely, and there is evidence that spikes canbe transmitted through electrical synapses between these cells(Veruki and Hartveit, 2002). The question therefore arises whetherelectrical synapses between AII amacrine cells and ON-cone bipolarcells allow for a similar transmission of spikes. Although AIIamacrine cells can generate TTX-sensitive spikes (Boos et al.,1993; Veruki and Hartveit, 2002), we did not observe similar spikesgenerated by ON-cone bipolar cells in situ.

For electrically coupled cell pairs, we observed that spontaneous action potentials in the AII amacrine cell evoked slow depolarizationsin the ON-cone bipolar cell (Fig. 5A). There were no failures.Adding TTX blocked action potentials in AII amacrine cells andthe corresponding depolarizations in ON-cone bipolar cells (Fig.5B). Figure 5C shows a series of traces with postsynaptic depolarizationsin an ON-cone bipolar cell aligned by a spike in the presynapticcell (AII). The postsynaptic depolarizations had an average amplitudeof 2.0 ± 0.1 mV (range, 1.1-3.0 mV; n = 40 responses), a 10-90%rise time of 2.6 ± 0.1 msec (range, 1.3-5.8 msec), and a latencyfrom the presynaptic spike of 0.32 ± 0.02 msec (range, 0.04-0.65msec). The latency was determined as the time interval betweenthe maximum slope of the presynaptic action potential (measuredas the peak of the first derivative of that waveform) and theonset of the postsynaptic depolarization (measured as 5% of thepeak amplitude). The low variability of the postsynaptic depolarizationsand the absence of failures suggest that the connection was monosynapticand that the depolarizations corresponded to electrical PSPs.The average coupling coefficient (ratio between the amplitudeof the postsynaptic depolarization and the amplitude of the presynapticspike) was 0.22. This was lower than the steady-state couplingcoefficient between the same cell pair, which was 0.61, consistentwith frequency-dependent attenuation of transmission. Similarobservations and quantitative measurements of electrical PSPswere made for a total of eight cell pairs. The mean peak amplitudewas 1.6 ± 0.3 mV (range, 0.1-2.8 mV), the mean 10-90% rise timewas 2.2 ± 0.4 msec (range, 1.2-4.2 msec), and the mean latencyfrom the presynaptic spike was 0.37 ± 0.09 msec (range, 0.15-0.78msec). The mean coupling coefficient was 0.18 ± 0.06 (range, 0.02-0.49).

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Figure 5. Transmission of action potentials from AII amacrine cells and electrical PSPs in ON-cone bipolar cells. A, Spontaneous activity of a simultaneously recorded, electrically coupled cell pair. Spikes in the AII amacrine cell occur together with slower depolarizations in the ON-cone bipolar cell (type 7). B, TTX blocks spiking in the AII amacrine cell and corresponding subthreshold depolarizations in the ON-cone bipolar cell. C, Left, Recording configuration, both cells in current clamp. Right, Overlaid spontaneous activity (Control) traces of AII amacrine cell and bipolar cell aligned by a spike in the AII amacrine cell (n = 6). Same cell pair as A. D, Left, Recording configuration; AII amacrine cell voltage clamped with prerecorded action potential waveform and bipolar cell in current clamp. Right, Overlaid evoked activity traces of AII amacrine cell and bipolar cell aligned by a simulated spike in the AII amacrine cell (n = 6); recorded in the presence of TTX. Same cell pair as A. E, Spontaneous activity of a simultaneously recorded, electrically coupled cell pair. Note simultaneously occurring subthreshold depolarizations (vertical arrows) in the AII amacrine cell and the bipolar cell (type 8), presumably evoked by spiking activity in other AII amacrine cells independently coupled to both cells. A spike in the AII amacrine cell evokes an additional subthreshold depolarization in the bipolar cell. F, Spontaneous activity of simultaneously recorded, electrically coupled cell pairs (left, type 6 bipolar cell; middle and right, type 7 bipolar cell, same cell pair). Note subthreshold depolarizations (vertical arrows) in the AII amacrine cell (left) or the bipolar cell (middle and right) unaccompanied by corresponding depolarizations in the other cell of the pair.

The transmission characteristics between electrically coupled AII amacrine cells and cone bipolar cells were studied by applicationof simulated action potentials as voltage-clamp templates. Afterrecording a series of electrical PSPs evoked by spontaneous presynapticaction potentials in the AII amacrine cells (Fig. 5C), we addedTTX to the extracellular solution, changed the recording configurationof the AII amacrine cell from current clamp to voltage clamp,and applied a previously recorded action potential as a voltage-clampcommand. The postsynaptic depolarizations evoked by the simulatedaction potential were similar to those evoked by spontaneous actionpotentials (Fig. 5D). To quantify the comparison, we measuredthree response parameters: latency, coupling coefficient, and10-90% rise time of the postsynaptic depolarization. There wasno significant difference between the values of each of the threeparameters compared between control and TTX conditions (p > 0.16;n = 6 cell pairs; paired t test for each response parameter).This suggests that voltage-gated I_Na does not influence the couplingcharacteristics or the time course of the postsynaptic responseand that the transmission of action potentials from AII amacrinecells to ON-cone bipolar cells can be explained by a passive,electrotonicmechanism.

Although our recordings were from pairs consisting of one AII amacrine cell and one bipolar cell, we sometimes observed indirectevidence for electrical coupling to other cells, making it likelythat electrical coupling encompasses a more extensive networkof cells. In the example shown in Figure 5E, an ON-cone bipolarcell displayed an electrical PSP corresponding to an action potentialin a simultaneously recorded AII amacrine cell. In addition, bothcells displayed correlated subthreshold depolarizations, presumablyelectrical PSPs caused by action potentials in other AII amacrinecells connected independently to the recorded cells. In othercases, presumed electrical PSPs occurred only in the AII amacrinecell of a coupled pair (Fig. 5F, left) or only in the ON-conebipolar cell of a coupled pair (Fig. 5F, middle and right), suggestingthat they were caused by spikes in other AII amacrine cells coupledpredominantly (or exclusively) to only one of the recordedcells.

Subthreshold membrane potential synchronization and oscillation

Electrical synapses are able to mediate temporally precise synchronization not only of action potentials but of subthresholdmembrane potential fluctuations as well (Galarreta and Hestrin,2001; Veruki and Hartveit, 2002). An important question is thereforewhether such patterns of synchronization can be observed betweenAII amacrine cells and ON-cone bipolar cells. For a quantitativeanalysis, we constructed sliding-window, 2D cross-correlogramsbetween pairs of simultaneously recorded cells. The 2D cross-correlogramsin Figure 6B were calculated from 15-sec-long, continuous voltagerecords from a pair of electrically coupled cells (Fig. 6A) andshow strong, continuous synchronization of membrane potentialfluctuations. This was observed both in the control condition(Fig. 6A, top, B, left) and in the combined presence of antagonistsof chemical synaptic transmission, TTX and Co²⁺ (replacing Ca²⁺ in the external solution) (Fig. 6A, bottom, B, right). The time-averagedcross-correlogram for each condition is shown in Figure 6D (left,blue traces; top row control, bottom row with blockers). For each2D cross-correlogram, we calculated the peak amplitude, peak location(relative to zero time delay), and half-width duration of each(1D) cross-correlogram as a function of recording time. The peakamplitude was taken as a measure of synchrony. For both recordingconditions, the variability in synchrony over time was minimal,with a mean value of 0.824 ± 0.004 (n = 148 1D cross-correlograms)in the control condition and 0.763 ± 0.006 with blockers. Thepeak amplitude of the time-averaged cross-correlograms was locatedvery close to zero time delay, and there was little fluctuationin the location of the peak as a function of time (Fig. 6C). Thisindicates a consistent, near-zero time shift between the membranepotential fluctuations in the two cells. In the control condition,the location of the peak was +2.8 ± 0.1 msec (Fig. 6C, left),indicating that the AII amacrine cell led and the ON-cone bipolarcell followed (see Materials and Methods). In the combined presenceof antagonists, TTX and Co²⁺, the location of the peak reversed ( $-$ 2.3 ± 0.1 msec) (Fig. 6C,right), indicating that the AII amacrine cell no longer led thebipolar cell. Further experiments attributed this effect to thepresence of TTX (see below).

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Figure 6. Synchronous subthreshold membrane potential fluctuations during spontaneous activity. A, Spontaneous activity of a pair of simultaneously recorded, electrically coupled cells (AII amacrine cell, blue; cone bipolar cell type 7, red) in control solution (top) and in the presence of antagonists of chemical synaptic transmission, TTX and Co²⁺ (bottom). B, Sliding 2D cross-correlograms for 15 sec continuous recordings of same cell pair as in A (left, control condition; right, with blockers). Horizontal axis, Time at the center of the 0.5 sec sliding window; vertical axis, time lag from the center (zero time delay) of the window. The normalized correlation amplitude is coded by color (bar, right). Period of recordings in A is indicated by solid horizontal lines. C, Location of peak amplitude in 2D cross-correlograms in B (left, control condition; right, with blockers). D, One-dimensional cross-correlograms (top row, control condition; bottom row, with blockers): time-averaged normal (blue) and shuffled (red) cross-correlograms (left); cross-correlograms centered at time points corresponding to arrows 1, 2, and 3 in B (control condition); cross-correlograms centered at time points corresponding to arrows 4, 5, and 6 in B (with blockers).

Two-dimensional cross-correlograms were constructed for a total of 16 cell pairs in control solution. The average peak amplitudeof time-averaged cross-correlograms was 0.74 ± 0.03 (range, 0.53-0.91),and the average location of the peak was +3.2 ± 0.5 msec (range,+0.3 to +8.8 msec). In the presence of antagonists of chemicalsynaptic transmission, the average peak amplitude was 0.73 ± 0.04(n = 17), and after adding TTX along with the antagonists it was0.72 ± 0.04 (n = 13). The location of the peak amplitude did notchange significantly in the presence of antagonists of chemicalsynaptic transmission (p = 0.11; paired t test; n = 16), but inthe additional presence of TTX the average location of the peakchanged from +3.3 ± 0.6 to $-$ 1.6 ± 1.3 msec (p = 0.004; pairedt test; n = 13). As a control, we constructed shuffled cross-correlogramswith segments for the second cell chosen in random order withrespect to the first cell. Additionally, cross-correlograms wereconstructed from pairs of AII amacrine cells and either rod bipolarcells or OFF-cone bipolar cells (n = 5; recorded in the presenceof antagonists of chemical synaptic transmission). We never observedconsistent peaks in shuffled (Fig. 6D, left, red traces) or noncoupledcross-correlograms (data notshown).

For most cell pairs the cross-correlograms indicated that the strong synchronization was accompanied by discrete periods ofmarkedly oscillatory membrane potential fluctuations. The degreeof oscillation varied over time with continuous synchronizationalternating between oscillatory (Fig. 6D, top, panels 2 and 3)and non-oscillatory activity (Fig. 6D, top, panel 1), evidenceof marked short-term dynamics in network activity. The periodof oscillation was typically 100-300 msec. In the presence ofblockers, synchronization still alternated between oscillatory(Fig. 6C, bottom, panels 4 and 5) and non-oscillatory activity(Fig. 6D, bottom, panel 6). This suggests that oscillatory synchronizationdoes not depend on chemical neurotransmission, Na⁺-dependent action potentials, or voltage-gated Ca²⁺currents.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

There is increasing evidence for the widespread existence of gap junctions, functionally corresponding to electrical synapses,in several regions of the CNS (Galarreta and Hestrin, 2001). Inthe retina, homologous and heterologous gap junctions were detecteddecades ago and have been assigned a role both in pathways fortransfer of visual signals and in networks of neurons thoughtto be important for adjustment of visual sensitivity and spatialresolution. Electrical synapses between AII amacrine cells andON-cone bipolar cells are considered essential for the flow ofvisual signals in the retina under dark-adapted conditions (Kolband Famiglietti, 1974; Bloomfield and Dacheux, 2001). To investigatefunctional aspects of this microcircuit, we have used simultaneousdual recording to directly demonstrate and functionally characterizestrong electrical coupling between AII amacrine cells and ON-conebipolar cells. The electrical synapses have symmetrical junctionconductances with very low voltage sensitivity, mediate sign-conservingsignaling, and show a strong propensity to synchronize membranepotential fluctuations. There is strong functional rectificationwith preferential transmission of membrane potential changes fromAII amacrine cells to ON-cone bipolar cells. Action potentialsin AII amacrine cells evoke distinct electrical PSPs in ON-conebipolar cells. Electrical coupling was detected between AII amacrinecells and every type of bipolar cell proposed to correspond toON-cone bipolar cells (Euler et al., 1996; Hartveit, 1997), exceptON-cone bipolar cell type 9, which is rare (Euler and Wässle,1995; Hartveit, 1997) and was not recorded in the present study.The experiments were performed in mature tissue, thus excludingthe possibility that the observations are unique to a particulardevelopmental stage in maturation of the neuronaltissue.

We believe that the observed electrical coupling between AII amacrine cells and ON-cone bipolar cells is caused by flow ofcurrent through gap junctions. The observed responses have thefunctional properties expected for electrical coupling mediatedby gap junctions (Bennett, 1977). We observed electrical couplingonly in cell pairs with overlapping processes. Finally, we neverobserved electrical coupling when either an AII amacrine cellor an ON-cone bipolar cell was recorded simultaneously with anyother type of cell (except when recording from pairs of AII amacrinecells) (Veruki and Hartveit, 2002), regardless of whether thecells were in potential physical contact. Our estimate of theelectrical junction conductance will be influenced by severalsources of error that to some extent could cancel each other.On the one hand, the existence of indirect pathways of couplingbetween two monosynaptically coupled cells will tend to overestimatethe true junction conductance. On the other hand, our measurementsinclude the cytoplasmic resistance along the processes of eachcoupled cell, and this will tend to underestimate the true junctionconductance.

Morphological investigations at the ultrastructural level have identified a structural asymmetry of the gap junctions betweenAII amacrine cells and ON-cone bipolar cells (Strettoi et al.,1992), and it has been speculated that this is related to a functionalasymmetry of the corresponding electrical synapses (Vaney, 1997).Recently, this idea was challenged by studies suggesting thattracer coupling between AII amacrine cells and ON-cone bipolarcells was bidirectional (Trexler et al., 2001) and that depolarizingresponses to photopic visual signals may be conveyed to AII amacrinecells (Xin and Bloomfield, 1999). Alternatively, it was suggestedthat the structural asymmetry could reflect some form of regulationof the signal transmission between AII amacrine cells and ON-conebipolar cells (Strettoi et al., 1992). In the present study, witha light-adapted slice preparation, we demonstrate directly thatthe electrical junction conductance was consistently symmetricand the steady-state voltage-sensitivity was very low (withinthe physiologically relevant range examined). The functional characteristicsof the electrical coupling seem well suited for efficient transferof visual signals between the two cell types. The strong asymmetryof coupling coefficients indicates that transmission will be moreeffective in the direction from AII amacrine cells to ON-conebipolar cells. This functional rectification could be a consequenceof the corresponding difference in membrane input resistance betweenthe two cell types (reflecting the difference in cell size). Thelow coupling coefficient for transmission from ON-cone bipolarcells to AII amacrine cells could also be a mechanism to preventextensive cross-talk between different types of ON-cone bipolarcells electrically coupled to the same AII amacrine cell. It islikely, however, that the degree of coupling could be regulatedby changes in the electrical junction conductance through activationof intracellular second messenger systems. Although changes intracer coupling need not reflect corresponding changes in electricalcoupling, there is indeed evidence that tracer coupling betweenAII amacrine cells and bipolar cells is under modulatory control,possibly related to network switching between rod and cone pathwaysassociated with light adaptation (Mills and Massey, 1995). Itwas proposed that the gap junctions between AII amacrine cellsand ON-cone bipolar cells would be closed by increasing levelsof light, mediated by an increase in the intracellular concentrationof cGMP. In our experiments, no attempt was made to directly manipulatethe concentration of cGMP or any other potential intracellularsecond messenger. Furthermore, the open probability of the gapjunction channels is unknown and cannot be determined from themeasured electrical junction conductance without knowing the numberof channels and the single-channel conductance. It will be importantto determine whether the electrical junction conductance betweenAII amacrine cells and ON-cone bipolar cells is under modulatorycontrol and how this might be controlled by the state of lightadaptation.

The electrical synapses displayed the functional characteristics of a low-pass filter with similar transmission characteristicsfor both directions of coupling. For steady-state signals, wefound coupling coefficients up to ~75% for coupling from AII amacrinecells to ON-cone bipolar cells. For higher-frequency signals likeaction potentials, coupling coefficients were lower (2-49%), butthey evoked distinct electrical PSPs in the ON-cone bipolar cells.In experiments with prerecorded action potentials as voltage-clamptemplates, the evoked electrical PSPs in ON-cone bipolar cellswere very similar to those evoked by spontaneous action potentials,suggesting that propagation of action potentials (Martina et al.,2000) toward the site of coupling does not constitute a mechanismfor amplifying the coupling strength between AII amacrine cellsand ON-cone bipolar cells. Because of cable filtering along theON-cone bipolar axon, the temporal characteristics of the electricalPSPs will most likely be even more transient at the axon terminalsthan at the soma where we recorded them. This is likely to beof considerable functional importance for the release characteristicsof the chemical synapses made by the ON-cone bipolar cells onprocesses of amacrine cells and ganglion cells in the inner plexiformlayer (Strettoi et al., 1994).

Our study demonstrates temporally precise synchronization of subthreshold membrane potential fluctuations between AII amacrinecells and ON-cone bipolar cells. Under our experimental conditions,the AII amacrine cell generally leads and the ON-cone bipolarcell follows. This relationship was blocked by TTX, suggestingthat it could be mediated by the regenerative properties of thevoltage-dependent I_Na in the AII amacrine cells. An importantissue for future research will be to determine how the membranepotential of an AII amacrine cell can influence transmitter releasefrom the axon terminal of an ON-cone bipolar cell to which itis electricallycoupled.

We are unaware of any evidence suggesting the presence of chemical synapses between AII amacrine cells and ON-cone bipolarcells. Thus, the direct interaction between these cell types mustbe limited to electrical synapses, but there might be indirectpathways of interaction. Chemical synaptic output from ON-conebipolar cells to amacrine cells (Strettoi et al., 1994) couldmediate negative feedback to the AII amacrine cells. Chemicalsynaptic output from AII amacrine cells to OFF-cone bipolar cells(Strettoi et al., 1992) could suppress excitatory input to amacrinecells with inhibitory connections to ON-cone bipolar cells. Undernatural conditions, it is likely that such network interactions,as well as common chemical synaptic input from rod bipolar cellsto electrically coupled AII amacrine cells (Strettoi et al., 1992),will interact with the electrical synapses between AII amacrinecells and between AII amacrine cells and ON-cone bipolar cells.An important next step will be to investigate directly the dynamicinteractions within these heterogeneousnetworks.

  FOOTNOTES

Received June 27, 2002; revised Sept. 24, 2002; accepted Sept. 26, 2002.

This work was supported by the Norwegian Research Council (NFR 123487/310, 129566/310, 123485/310, 141392/310) and the Meltzerfund (University ofBergen).

Correspondence should be addressed to Espen Hartveit, University of Bergen, Department of Anatomy and Cell Biology, Årstadveien19, N-5009 Bergen, Norway. E-mail: espen.hartveit{at}iac.uib.no.

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RESULTS
DISCUSSION
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