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The Journal of Neuroscience, July 30, 2003, 23(17):6904-6913
Previous Article | Next Article
AII Amacrine Cells Express L-Type Calcium Channels at Their Output Synapses
Christopher J. Habermann, Brendan J. O'Brien, Heinz Wässle, andDario A. Protti Department of Neuroanatomy, Max Planck Institute for Brain Research, D-60528 Frankfurt am Main, Germany
Abstract
Top
Abstract
Introduction
AII amacrine cells play a critical role in the high-fidelity signal transmission pathways involved with nighttime vision. The temporal properties of the light responses strongly depend on the transfer function at different synaptic stages and consequently on presynaptic calcium influx. AII light responses are complex waveforms generated by graded input, they comprise Na+-based spikes as well as a sustained component, and they are transferred to graded cone bipolar cells. It is, therefore, of interest to determine the properties of AII voltage-dependent calcium channels (VDCCs) to establish whether these cells express N-type and/or P/Q-type VDCCs, characteristic of spiking neurons, or whether they are more like graded neurons, which mostly use L-type VDCCs. We combined electrophysiological, molecular biological, and imaging techniques to characterize calcium currents and their sites of origin in mouse AII amacrine cells. Calcium currents activated at potentials more positive than -60 mV (maximally between -50 and -20 mV) and inactivated slowly. These currents were blocked by dihydropyridine (DHP) antagonists and were enhanced by the DHP agonist BayK 8644. Single-cell RT-PCR analysis of mRNA encoding for different calcium channelsubunits in AIIs revealed a consistent expression of the
Key words: amacrine; rod vision; scotopic pathways; tonic synapses; transmitter release;
Introduction
Narrow-field bistratified AII amacrine cells play a crucial role in signal processing in nighttime vision. In the conventional rod pathway, rod photoreceptors convert light into an electrical signal that is transferred via a sign-inverting synapse to rod bipolar (RB) cells, which in turn synapse onto AII amacrine cells. The AII cells then split the incoming signal into the ON and OFF channels of the visual system by making electrical synapses, via gap junctions, with ON-cone bipolar (CB) cells and glycinergic inhibitory synapses with OFF-CB cells. CB cells transmit the information further to their respective ON and OFF ganglion cells.In scotopic conditions, the light responses of various cell types appear to possess a robust sustained component. Light responses of rods show an early transient response, followed by a sustained phase (Baylor et al., 1984
; Schneeweis and Schnapf, 1995
In rods and RB cells, neurotransmitter release takes place in zones that are highly specialized for the transmission of sustained graded responses and large bandwidths of information (Rao-Mirotznik et al., 1995
Therefore, we set out to investigate the calcium channel types as well as their location in AII amacrine cells in mouse retinal slices using whole-cell recordings combined with single-cell RTPCR and intracellular calcium imaging. Our data show that AII cells possess slowly inactivating VDCCs of the
Materials and Methods
All procedures were in accordance with the guidelines for animal experiments issued by the Federal Republic of Germany (Tierschutzgesetz). Vertical slices were prepared from the retinas of C57Bl/6J mice, 5-7 weeks of age, as described previously (Boos et al., 1993-Conotoxin GVIA was purchased from Alamone Labs (Jerusalem, Israel), and
Electrophysiological recordings. Experiments were performed with the tight-seal whole-cell recording configuration of the patch-clamp technique. All experiments were performed at room temperature (20-22°C) using a fixed stage, upright microscope (Axioskop; Zeiss, Oberkochen, Germany) equipped with Nomarski differential interference contrast optics and a water immersion objective (63x; 0.9 NA). Recordings were obtained from the amacrine cells located in the innermost part of the inner nuclear layer (INL), using an EPC-9 amplifier (Heka Electronic, Landau, Germany). Borosilicate glass pipettes with 10 M
resistance were used. Experiments were performed with a cesium gluconate (CsGlu)-based intracellular solution containing (in mM): 106 CsGlu, 10 tetrabutylammonium chloride (TBA), 30 HEPES, 4.6 MgCl2, 0.4 Na-GTP, and 4 Na-ATP, pH 7.3. Neurobiotin (10 mg/ml) was included in the intracellular solution. Membrane potential values were corrected for junction potential (-15 mV). Leak and capacitive currents were subtracted (p/4 protocol). The tissue was perfused at a rate of 1-1.5 ml/min. Histological examination of neurobiotin-filled cells was performed after completion of electrophysiological recordings using standard staining procedures (Horikawa and Armstrong, 1988
Single-cell RT-PCR. Cytoplasm from AII amacrine cells (n = 9), ganglion cells (n = 1), and cerebellar Purkinje cells (n = 5) was harvested to determine the molecular composition of their VDCCs by RT-PCR. Whole-cell recordings were established with thick wall borosilicate glass pipettes that had been baked previously for >4 hr at 200°C to inactivate RNases. Pipettes (2-5M
cDNA was reverse transcribed from cellular mRNAs in the above-described PCR tubes overnight at 37°C. Simultaneous amplification of cDNAs present in the 10 µl reverse transcription reaction was performed using primers for
-actin and all neuronal calcium channel
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Table 1. PCR primer sequences
The first round of PCR was followed by a second round of PCR (35 cycles) using 2 µl of the first PCR with the same cycling parameters and reaction solution as above, but with only a single primer set. From each 100 µl PCR reaction, 10 µl were electrophoresed through 2% agarose gels, stained with ethidium bromide (0.5 µg/ml), and imaged under UV excitation (Eagle Eye; Stratagene, La Jolla, CA). This protocol was initially tested on 50 pg of whole-brain RNA extracted using Trizol (Invitrogen), and all transcripts were amplified to detectable levels (data not shown). The identity of PCR products was confirmed by sequence analysis after cloning (TOPO; Invitrogen).
Fluorometric calcium imaging. Changes in intracellular calcium concentrations ([Ca2+]i) were detected as changes in the fluorescence intensity of Oregon Green 488 BAPTA-5N (OG5; 200 µM), which was included in the patch pipette. Calcium Green 1 (CG1; 100 µM) and Oregon Green 488 BAPTA 2 (OG2; 100 µM) were also used as calcium indicators. Fluorescence images were obtained with a MERLIN imaging system (Life Science Resources, Cambridge, UK). The excitation pathway consisted of a high-intensity Xe light source focused in a high-speed SpectraMASTER monochromator system coupled to the microscope by a liquid light guide. Excitation wavelength centered at 488 nm was used to monitor intracellular calcium concentration with the aforementioned dyes. The dichroic mirror and high-pass emission filter had center wavelengths at 510 nm and 520 nm, respectively. Images were acquired with an eight-bit-intensified analog video camera operating at 768 x 576 pixels, in its integrating mode. MERLIN 1.88 was used as acquisition and analysis software.
The standard protocol to study [Ca2+]i transients consisted of acquiring a sequence of images at regular intervals for 15-20 sec. Control images were taken either for 2 or 5 sec before depolarization. Stimuli consisted of a sequence of depolarizing pulses from -75 mV. Images were integrated for times ranging from 100 to 450 msec, optimizing this time separately for acquisition from the lobular appendages and the arboreal dendrites regions, the two regions that were the focus of our study. Changes in [Ca2+]i in the soma were also observed but not investigated, because the dynamic range of the imaging system used (256 bits) would have required different image acquisition rates. Fluorescence changes were analyzed offline by measuring the average fluorescence in small regions of interest (ROI) and converting the value to a percentage change in fluorescence:
F/F0 = 100*(F - Fr)/(Fr - B), where F is the measured fluorescence signal at any given time, Fr is the average fluorescence from several consecutive images preceding the stimulus, and B is the average value of the background fluorescence from four regions located in the periphery of the visual field and of similar size to the cellular ROIs. Background values were stable during each experiment. The decay phase of calcium transients was fitted using a least-squares fitting routine to a single exponential function: F(t) = A exp(-t/
), in which t is time and A is the fitted amplitude of the transient. Data were analyzed with Igor Pro software (WaveMetrics, Lake Oswego, OR) using custom-made routines.
Results
Identification and morphology of AII amacrine cells
Recordings were obtained from AII amacrine cells in light-adapted retinal slices. They were identified under Nomarski optics by the following morphological characteristics: their somata, localized to the innermost part of the INL, bulge into the inner plexiform layer (IPL) giving rise to one or more sturdy primary dendrites (lobular dendrites), from which the lobular appendages branch in sublamina a while several thinner bushy dendrites (arboreal dendrites) ramify further down in the IPL in sublamina b. Cells were first morphologically identified on the basis of fluorescence images obtained after breaking into the cell with the patch pipette and dialyzing with intracellular solution containing both a calcium sensitive dye and neurobiotin. Commonly, the lobular appendages were rapidly loaded with dye, whereas the arboreal dendrites needed more time to be filled. After the recordings, slices were fixed and histochemically processed to reveal the morphology of neurobiotin-filled cells. In the initial experiments, neurobiotin staining was always performed to corroborate the cell identity as observed in the fluorescence image. Because we achieved a very high rate of success in selecting AII cells, cell type recognition in subsequent experiments was based mainly on fluorescence images. On loading with the Ca2+ probes, only individual cells were labeled, because Ca2+-sensitive dyes have a high molecular weight such that they do not permeate gap junctions. However, after neurobiotin staining, an extensive network of somata and dendrites could be observed occasionally, revealing gap junctional coupling (Fig. 1). Mosaics consisting of other AII cells as well as different types of ON-CB cells were observed around the injected cells, in agreement with previous reports (Vaney, 1991
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Figure 1. Micrograph of a retinal slice showing neurobiotin staining of a group of coupled AII (inner IPL) and ON-CB cells (outer IPL) after filling a single AII amacrine cell via the patch pipette. The strongly stained soma located in the innermost part of the INL is the patched cell. Robust dendrites that constitute the lobular appendages of AII cells are observed in sublamina a of the IPL, whereas the more bushy arboreal dendrites are observed in sublamina b. Scale bar, 10 µm.
General electrophysiological properties
Whole-cell recordings from AII cells in light-adapted conditions revealed a high level of spontaneous activity. Current fluctuations with kinetics characteristic of spontaneous IPSC activity as described previously for ganglion and amacrine cells (Protti et al., 1997In a large number of cells, spontaneous currents characterized by a very fast rise and decay time (
1 msec) and a frequency between 10 and 180 Hz persisted after abolishing IPSC activity. The presence of these currents was dependent on membrane voltage and they ran down during the recordings. Pharmacological dissection revealed that they originated from activation of voltage-dependent Na+ channels, as shown by their sensitivity to 0.5-1 µM TTX (Boos et al., 1993
Characterization of Ca2+ currents
Cells were whole-cell patch clamped and dialyzed with an intracellular solution containing CsGlu and TBA to block most of the voltage-activated K+ currents. This internal solution in combination with bath perfusion of TTX, strychnine, and picrotoxin allowed us to isolate voltage-activated calcium currents. AII amacrine cells have been shown to possess very robust voltage-activated K+ currents, with peak amplitudes up to 3.5 nA (Boos et al., 1993
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Figure 2. Characterization of voltage-dependent calcium currents in AII amacrine cells. A, Voltage-activated currents recorded from an AII amacrine cell dialyzed with CsGlu. Depolarizing pulses of 10 mV steps were applied from a holding potential of -75 mV. B, Three individual traces from the currents shown in A from holding potential to test potentials -55, -35, and -15 mV from top to bottom, respectively. C, Average current-voltage relation measured from 14 cells recorded under similar conditions from Vhold = -75 and -95 mV. Values represent peak amplitude, and bars indicate SE. D, Amplitude histogram of the peak amplitude values (57 cells). E, Superimposed recordings from Vhold = -75 mV to Vtest = -35 mV for three different durations (100, 250, and 500 msec) showed a linear relation between charge transfer and pulse duration (F).
Pharmacology of calcium currents
So far, we have observed that in AII cells, both the activation threshold of Ca2+ currents and their voltage of maximal activation are more negative than those reported for the majority of other HVA Ca2+ currents, resembling more the activation properties of an LVA Ca2+ current. In other retinal neurons, however, it has been reported that L-type Ca2+ channels display more negative activation threshold than classically described L-type calcium channels (Protti and Llano, 1998HVA Ca2+ currents are currently categorized into several subclasses on the basis of their distinctive biophysical and pharmacological properties, as well as by their molecular identity. At least four different HVA Ca2+ channel types have previously been identified, namely L, N, P/Q, and R types (Zhang et al., 1993
We studied the effect of the L-type calcium channel agonist BayK 8644 (10 µM) on depolarization-induced calcium influx. Application of BayK 8644 produced a large increase in current amplitude above control values (Fig. 3A). Interestingly, the overall calcium current was enhanced, resulting in an increased amplitude but again with very slow inactivation kinetics. It is also evident that the tail current amplitude at the end of the depolarizing pulse was increased and lengthened. On average, the effect of BayK 8644 on depolarization-induced transmembrane charge was doubled in the presence of BayK 8644, and this effect was reversible (Fig. 3B; n = 20).
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Figure 3. Effect of DHP agonists and antagonists on VDCCs of AII cells. A, Representative recordings showing calcium currents elicited by steps to -45 mV from a holding potential of -95 mV. After recording currents in control conditions (middle trace), 10 µM BayK 8644 was added to the bathing medium (bottom trace). BayK 8644 was washed out from the bathing medium, and the calcium current returned to its initial amplitude. Perfusion of the tissue with medium containing 10 µM nitrendipine significantly reduced the current (top trace). B, Ca2+ influx expressed as charge transfer on depolarization. The summary of the effect of DHP antagonists (14 cells) and BayK (20 cells) on depolarization-elicited transmembrane charge is carried by Ca2+ ions of AII cells.
Two different L-type calcium channel antagonists were tested on voltage-dependent calcium currents. Both nitrendipine and nifedipine (10 µM) greatly reduced calcium currents without substantially affecting the kinetics of the remaining current. Figure 3A shows an example of the blocking effect of 10 µM nitrendipine in the same AII amacrine cell previously treated with 10 µM BayK 8644. Nitrendipine clearly reduced both the early and delayed phase of the calcium current with equal potency. In a total of 14 AII cells, DHP antagonists reduced calcium currents by almost 80% (Fig. 3B). The reversibility of the blocking effect on calcium currents required long periods of washout and was only observed occasionally. We investigated the effect of N-type and P/Q-type calcium channel blockers, on the voltage-gated calcium currents of AII cells. After incubation for 10 min in medium containing 5 µM
90% of their control amplitude (two cells). A similar reduction is commonly observed in the absence of any drugs and reflects run down of the calcium currents. In two cells treated with 100 nM
Molecular characterization of the
To determine the molecular identity of the VDCCs underlying our recordings of AII amacrine cells, we undertook single-cell RT-PCR experiments. There are currently 10 known genes (CACNA1A-CACNA1I and CACNA1S) coding for each of the VDCCWe harvested cellular cytoplasm from nine AII amacrine cells. Four of these cells failed to give amplification of any product. All of the remaining five AII cells strongly and exclusively expressed a correctly sized PCR product for the CACNA1D gene (CaV1.3
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Figure 4. CaV gene expression in single cells. A, Expression of VDCC
As further confirmation of the efficiency of our technique, we amplified cDNA made from the cytoplasm of five cerebellar Purkinje cells. Calcium currents in mature Purkinje cells are dominated by P-type currents (CaV2.1
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Table 2.
These data strongly support the physiological and pharmacological evidence that AII amacrine cells exclusively express L-type VDCCs that contain the CaV1.3
Sites of origin of Ca2+ entry
Depolarization-induced calcium influx has been extensively investigated in several CNS neurons. All types of VDCCs have been localized to the dendrites of distinct classes of neurons, in which they have been found to play crucial roles in the modulation of dendritic action potentials, as well as being involved in a variety of forms of plasticity phenomena. In axonal terminals, N-type VDCCs as well as P/Q-type VDCCs seem to primarily mediate calcium influx responsible for transmitter release. Most amacrine cells represent an exceptional case among neurons, because transmitter release takes place at the active zones of their complex dendrites, since most of them do not possess an axon. The results presented previously revealed the presence of L-type calcium channels in AII amacrine cells, a channel type that does not normally play a major role in neuronal exocytosis. Thus, it is appealing to investigate their subcellular distribution in AII cells to see whether or not they are localized to the synaptic processes.The spatial distribution of depolarization-induced changes in intracellular calcium concentration ([Ca2+]i) was monitored by imaging the fluorescence emitted by low- and high-affinity Ca2+-sensitive dyes. We focused our attention mainly on the two different dendritic compartments, the lobular appendages, and the arboreal dendrites. The use of the low-affinity indicator OG5 (KD,
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Figure 5. Localization of depolarization-induced Ca2+ signals. A, Fluorescence image of an AII amacrine cell filled via the patch pipette with OG5. The circles denote ROI, namely the lobular appendages in the middle region and arboreal dendrites in the lower region, for the calculation of
Because Ca2+ transients in the arboreal dendrites were only detected occasionally and their magnitude was smaller than those observed in the lobular appendages, we also used intermediate affinity (OG2) and high-affinity (CG1) calcium dyes to investigate the nature of the calcium transients in more distal dendritic processes. The use of CG1 revealed again a large difference in the magnitude of the depolarization-induced change in fluorescence between the lobular appendages and the arboreal dendrites. The mean percentage of
To investigate whether L-type VDCCs mediate calcium influx in the lobular appendages, we studied the effect of DHPs on their calcium signals. BayK 8644 doubled the depolarization-induced increase in
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Figure 6. Pharmacological profile of depolarization-induced calcium signals. A, Effect of an L-type calcium channel agonist on depolarization-elicited fluorescence intensity changes of OG5 in the lobular appendages. Calcium transients in response to a 250 msec depolarization were recorded in control conditions, after perfusion with 10 µM BayK 8644 and after a washout. BayK 8644 almost doubled the change in fluorescence, and this effect was reversible. B, Effect of L-type calcium channel antagonists on depolarization-evoked calcium transients of the lobular appendages detected with OG5. Calcium rises induced by a 250 msec depolarizing pulse were largely blocked by 10 µM nitrendipine.
Discussion
In the present study, we have identified and localized the VDCCs present in AII amacrine cells. Our results indicate that AII amacrine cells possess a single type of VDCC mainly localized to the lobular appendages, in which chemical synaptic transmission takes place. The pharmacological profile of AII calcium currents, their slow inactivation kinetics, their localization to the lobular appendages, and the consistent expression of CaV1.3Classically described L-type calcium channels are activated from a holding potential of -60 mV, their activation threshold ranges between -40 and -30 mV, and their peak amplitude is reached around -10 mV (Nowycky et al., 1985
The pharmacological profile of AII calcium currents also supports the idea that these cells express L-type VDCCs. Calcium current amplitude in AII cells was doubled in the presence of the L-type calcium channel agonist BayK 8644 and reduced by 80% on application of DHP antagonists. The incomplete block of AII calcium currents by DHP antagonists also corroborates our observation that these cells contain mRNA encoding the
Depolarization-induced changes in the intracellular calcium concentration were observed mainly in the lobular appendages. It is noteworthy to remark that local application of glutamate to AII amacrine cells in the presence of calcium channel blockers elicits inward currents accompanied by calcium rises (Habermann et al., 2001
As mentioned earlier, L-type calcium channels seem to be commonly used by graded neurons, which possess synaptic ribbons, at early stages of sensory processing. Amacrine cells are a very diverse class of third order retinal interneuron. They differ in their morphology, function, light responses, and in the neurotransmitters that they release (for review, see Wässle and Boycott, 1991
Implications for signal processing
It is well established that retinal neurons involved in the rod pathway are capable of responding in a graded manner. Synaptic input to AII amacrine cells mostly originates from RB cells, which release neurotransmitter via L-type VDCCs (Protti and Llano, 1998Additionally, the close proximity of the activation threshold of AII calcium currents to their resting potential, together with their slow inactivation kinetics, suggests that Ca2+ influx through L-type calcium currents may contribute to the sustained component of the light-evoked responses. Interestingly, the threshold of voltage-dependent Na+ currents in AII amacrine cells is also shifted to more negative values (Boos et al., 1993
In summary, AII amacrine cells, capable of spiking, which contain no ribbons in their terminal structure, express a slowly inactivating L-type calcium channel. This VDCC type seems to be highly conserved at early stages of the scotopic pathway to be able to transmit sustained signals at relatively hyperpolarized membrane potentials.
Footnotes
Received Dec. 17, 2002; revised Apr. 15, 2003; accepted Apr. 15, 2003.We thank Dr. Krishna Ghosh for critical reading of this manuscript. We also thank Drs. Bertrand Lambolez and Bruno Cauli for generous assistance with the single-cell RT-PCR.
Correspondence should be addressed to Dr. Dario A. Protti, Department of Physiology, Anderson Stuart Building (F13), University of Sydney, New South Wales 2006, Australia. E-mail: dariop{at}physiol.usyd.edu.au.
C. J. Habermann's present address: Max Planck Institute for Medical Research, Jahnstrasse 29, D-69120 Heidelberg, Germany.
Copyright © 2003 Society for Neuroscience 0270-6474/03/236904-10$15.00/0
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