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1 Departments of Physiology and Biophysics and Ophthalmology, University of Arkansas for Medical Sciences, Little Rock, AR 72205, USA
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(Received 14 April 2004;
accepted after revision 6 August 2004;
first published online 12 August 2004)
Corresponding author Z. J. Zhou: Department of Physiology and Biophysics, University of Arkansas for Medical Sciences, 4301 W. Markham Street, Mail Slot 505, Little Rock, AR 72205-7199, USA. Email: zhoujimmy{at}uams.edu
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Introduction |
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To understand the potentially diverse functions of retinal waves at various stages of development, it is important to determine the sequence of wave development itself. Although retinal waves have been studied extensively in a variety of species (Feller, 1999; Wong, 1999), little is known about the entire developmental course of retinal waves. It has remained unclear how the waves initiate, progress and disappear during development, and what mechanisms regulate the wave dynamics at various developmental stages. Spontaneous waves in the inner mammalian retina were previously known to develop through two pharmacological stages: an early stage wave mediated mainly by nicotinic interactions, and a late stage wave driven by glutamatergic (Feller et al. 1996; Zhou, 1998; Bansal et al. 2000; Wong et al. 2000; Zhou & Zhao, 2000) and muscarinic (Zhou & Zhao, 2000) systems. More recently, an even earlier stage was reported in embryonic mice, during which some, but not all, waves are resistant to nicotinic antagonists (Bansal et al. 2000). However, it is unknown what mediates this early, nicotinic receptor-independent activity.
As development proceeds, changes in retinal wave dynamics have been found in a number of species (Wong & Oakley, 1996; Bansal et al. 2000; Demas et al. 2003; Sernagor et al. 2003b), consistent with the idea that the changing wave pattern may encode changing cues for visual development. The wave dynamics have also been shown to be modulated by cAMP in the ferret (Stellwagen et al. 1999; Bansal et al. 2000) and mouse (Bansal et al. 2000), by GABAA interaction in the turtle (Sernagor et al. 2003b), and by GABAB activation in the chick (Catsicas & Mobbs, 2001). However, it is unclear how the wave pattern in any one species changes systematically over the entire course of wave development, and whether the regulatory mechanisms shape wave dynamics differently at different stages of development.
This study systematically investigated the dynamics, regulation and distribution of spontaneous waves in the rabbit retina, starting from the first appearance of the wave prior to synaptogenesis, to the last stage of the wave shortly before eye opening. The results provided a comprehensive view of the developmental process of spontaneous waves in the mammalian retina. Preliminary results of this study have been reported in abstract form (Zhao et al. 1999; Zhou et al. 2002).
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Methods |
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Retinal flatmounts were prepared from New Zealand White and New Zealand Red rabbits aged between embryonic day 20 (E20, gestation period = 31 days) and postnatal day 14 (P14) as previously described (Zhou, 1998; Zhou & Zhao, 2000). Embryonic rabbits were delivered by Caesarian section from pregnant rabbits (4–5 kg in weight), which were deeply anaesthetized with 1–2 ml of pre-mixed (at a ratio of 100: 8) ketamine (100 mg ml–1) and xylazine (100 mg ml–1) (I.V) during the surgery. After Caesarian section, the doe was killed immediately with an overdose of sodium pentobarbital (250 mg, I.V.). All procedures involving the use of animals were in accordance with the National Institutes of Health guidelines as implemented by the institutional animal care and use committee. Immediately after an animal was killed by an overdose of sodium pentobarbital, retinas were dissected in cold (
10°C) Hepes-buffered Ames medium, which was modified from Ames medium (Ames & Nesbett, 1981) by replacing NaHCO3 with 20 mM Hepes. Isolated retinas were cut into 3 x 5 mm pieces and mounted on black filter paper (HABP, Millipore, Bedford, MA, USA) with either the vitreal or ventriclar surface facing the paper, depending on the experimental requirement.
To load the calcium indicator dye Fura-2AM (Molecular Probes, Eugene, OR, USA), retinal flatmounts were incubated in Hepes-buffered Ames medium containing 10 µM Fura-2AM and 0.001% pluronic acid for 1–6 h at 30°C. The extracellular matrix and immature Müller cell endfeet that covered ganglion cells were partially removed with forceps, so that ganglion and displaced amacrine cells could be loaded with the dye nearly uniformly in local areas (> 4 mm2) of the retina up to age P7–8. Loading of Fura-2AM in the distal (ventricular) surface of the retina was also nearly uniform at all ages tested (E20–P8). During Ca2+ imaging, the recording chamber was continuously superfused (3–4 ml min–1) with Ames medium at 35–37°C. Cells in the ganglion cell layer were imaged with an intensified, cooled CCD camera (I-Pantamax, Roper Scientific Instruments, Princeton, NJ, USA) mounted on a fixed-stage, upright microscope (Olympus BX50WI, Olympus USA, New York).
Whole-cell patch-clamp recordings were made from ganglion cells in the flatmount retina (without filter paper) as previously described (Zhou, 1998). Simultaneous patch-clamp and Ca2+ imaging was made from Fura-2AM-loaded retina under a 40x water immersion objective lens (NA = 0.8) (Zhou, 2001). The voltage and current traces were digitized at 10 kHz and stored on computer hard drive via Power Laboratory (AD Instruments, Colorado Spring, CO, USA) and subsequently filtered (Gaussian digital) and redigitized at lower rates depending on the resolution required. The images were acquired at a rate of one frame per second, with an exposure (integration) time of 0.6 s. The presence of a dye-free patch pipette in the field of view did not interfere with fluorescence imaging of retinal waves. The pipette resistance was 5–7 M
measured in Ames medium and a standard pipette solution containing (mM) 95 K-gluconate, 15 KCl, 5 NaOH, 0.5 CaCl2, 2 MgCl2, 5 EGTA, 2 ATP, 0.5 GTP, 2 ascorbic acid and 10 Hepes. Drugs were applied to the retina by bath perfusion (dead volume: 2 ml). Ames and Hepes-buffered Ames media were saturated with carbogen (95% O2, 5% CO2) and oxygen, respectively. All pharmacological agents used in this study were purchased from Sigma Chemicals (St Louis, MO, USA) except CGP55845and baclofen, which were purchased from Tocris Cookson (Bristol, UK).
Data acquisition and analysis
Fluorescence images of the retina were collected and analysed with the software Axon Imaging Workbench (AIW, Axon Instruments, Union City, CA, USA) and MetaImaging (MetaFluor and MetaMorph, Universal Imaging Inc., Downing, PA, USA) software. To monitor the excitability of the retina, oval zones were drawn in various regions of the image field. The average fluorescence intensity in each zone was plotted as a function of time F(t). The relative change in the emission fluorescence intensity (
F/F) was defined as [F(t) – Fo(t)]/Fo(t), where Fo(t) was the baseline intensity, which was obtained by drawing a curve that connected the fluorescence intensity values in the absence of waves. For simplicity, F/F from a single zone, selected randomly from the field of view, was shown in most figures, but similar results were also found from most of the remaining zones in the field. Thus, the measured F/F from a single zone not only reflected the Ca2+ activities in the zone, but also indicated the presence of a wave that passed through the zone. This was also verified by measuring F(t) in a selected zone with the software, while playing back the images in a movie series, so that the appearance of the waves could be observed simultaneously with the occurrence of F(t) measured from the zone. The propagation of retinal waves was imaged with a 10 x objective lens (NA = 0.3) at an acquisition rate of one frame per 0.9 s (with an exposure time of 0.6 s). Differential images (F) of the wave were obtained by subtracting a control image (averaged from four frames recorded immediately before a wave) from images recorded during the wave. To measure the speed (v) of the wave, the rate of displacement of the wavefront in the direction of wave propagation was measured using MetaMorph. Data were expressed as mean ± S.D. Student's t test was used to determine the significance of the data.
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Results |
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To understand the developmental sequence of spontaneous waves in the mammalian retina, we began by examining the wave property when the waves first appeared in the rabbit retina. Ca2+ imaging was made from Fura-2AM-loaded retinas isolated from rabbits starting at age E20, when ganglion cells were differentiated but had not yet undergone chemical synaptogenesis (Greiner & Weidman, 1982). At this age, ganglion cells were quite passive in their membrane electric properties, showing only small voltage-gated currents and very small regenerative potentials (data not shown). No propagating wave of spontaneous activity was found from the ganglion cell layer (GCL) at E20 (6 rabbits) and E21 (5 rabbits). The earliest age at which spontaneous waves were detected was E22, when ganglion cells began to generate large action potentials. E22 was also the age when ganglion cell axons first reached their central visual targets (Crabtree, 1990), suggesting that the earliest electric signals from the retina to the central visual targets were in the form of propagating waves. Figure 1 shows an example of patch-clamp recording from a ganglion cell and simultaneous Ca2+ imaging from the area surrounding the patch-clamped cell in a Fura-2AM-loaded E22 retina. The rhythmic bursts of spikes in the ganglion cell were found to correlate with the Ca2+ rises measured from the surrounding area (Fig. 1, n = 3). Importantly, at E22 neither the bursts of spikes in individual ganglion cells, nor the propagating Ca2+ waves in the GCL were sensitive to most neurotransmitter receptor antagonists, including blockers of acetylcholine (both nicotinic and muscarinic) receptors, ionotropic glutamate and GABA receptors and glycine receptors (Figs 1 and 2A, n = 6), suggesting that the earliest spontaneous waves were distinctly different from the waves previously reported in older mammalian retinas.
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We next examined whether adenosine played a role in spontaneous wave formation at E22. Application of the broad-band adenosine receptor antagonist aminophylline (100–500 µM) completely and reversibly blocked the earliest wave (Fig. 2B, n = 4). Because adenosine has been reported to up-modulate retinal waves via the cyclic AMP pathway in older (postnatal) ferrets and mice (Stellwagen et al. 1999; Bansal et al. 2000), we also tested the effect of the adenylate cyclase activator, forskolin. Application of forskolin (10 µM, n = 3) increased the wave frequency tremendously (Fig. 2C). In the presence of forskolin, the waves rapidly propagated across the field of view one immediately after another, and the Ca2+ concentration in ganglion cells underwent continuous oscillation (Fig. 2C). Thus, the dynamics of the earliest retinal wave in rabbits were regulated strongly by the cyclic AMP pathway. In contrast, depleting intracellular Ca2+ stores with thapsigargin (2 µM, n = 2) did not block the wave (Fig. 2D), even though thapsigargin caused a large, transient increase in the baseline Ca2+ level, presumably due to the blockade of Ca2+ uptake into intracellular stores, suggesting that the earliest retinal wave was not generated by Ca2+ release from thapsigargin-sensitive intracellular Ca2+ stores.
In addition to adenosine receptor antagonists, the common purinergic receptor antagonist reactive blue-2 (30–100 µM) also effectively blocked the waves in E22 rabbits (Fig. 2E) (n = 3), raising the possibility of an involvement of purinergic receptor activation in the waves. Suramin, a different purinergic antagonist, also blocked the wave, but only at a high concentration (500 µM, n = 2). However, another common purinergic antagonist, pyridoxal-5'-phosphate-6-phenylazo-2',4'-disulphonate (PPADS, 100–800 µM), did not have a consistent effect (n = 4), even though PPADS could block ATP-activated currents in ganglion cells (data not shown). The different effects of these antagonists on the wave might be attributable to the fact that different subclasses of P2X and P2Y receptors have very different sensitivities to various purinergic antagonists (Burnstock & Williams, 2000; Norenberg & Illes, 2000; von Kugelgen & Wetter, 2000). On the other hand, we could not rule out the possibility that the blockade of the wave by reactive blue-2 and suramin could be a result of a non-specific effect of the drugs, because attempts to exhaust endogenous ATP with hexokinase (3–10 u/ml) failed to block the wave (n = 3). The possibility of a purinergic involvement in retinal wave generation or regulation remains to be further investigated.
Spontaneous retinal waves in rabbit developed through three distinct stages
The unique pharmacological profile of the spontaneous wave in E22 rabbits suggested that the waves prior to synaptogenesis were generated by a distinct mechanism. Based on this finding and on the pharmacological properties of retinal waves previously described in older rabbits (Zhou & Zhao, 2000), we classified spontaneous waves in the inner rabbit retina into three stages. Stage I waves appeared between E22 and E23. They were not mediated by the common fast neurotransmitter receptors, including acetylcholine, glutamate, GABA and glycine receptors; however, they were abolished by the blockers of gap junctions, adenosine receptors, and possibly, purinergic receptors. Stage II waves occurred between E24 and P1, when the nicotinic system was the primary driving force for the waves (Zhou & Zhao, 2000). Stage III waves emerged at P4, after a transitional period (P2–P3) during which the excitatory drive for the wave switched from a nicotinic system to a system involving both glutamate and muscarinic receptors (Zhou & Zhao, 2000). Stage III waves were found between P4 and P8, the oldest age studied with Ca2+ imaging. Movies showing examples of stage I–III waves are provided in the Supplementary Materials.
Stage I waves.
Stage I waves appeared in the inner retina prior to synaptogenesis. These waves were very strong, sweeping across the entire field of view (1.15 x 1.15 mm) (Fig. 3A, upper) at an average speed of 451 ± 92 µm s–1 (n = 20), much faster than the waves at stages II and III (Fig. 5B). Stage I waves also appeared frequently, with an average interwave interval of 36 ± 18 s (n = 68) (Fig. 5B). The distribution of the interwave interval (Fig. 4C) showed a minimum interval of 
5 s, indicating a lack of prolonged postwave refractory period. Consequently, stage I waves did not form a clear boundary between neighbouring waves. When two waves collided, they superimposed (Fig. 3A, lower), instead of annihilating each other. Figure 4A shows, in the same retinal area, two successive waves that were separated by only 8 s. The Ca2+ increases during these two waves (measured as F/F from the small circles shown in Fig. 4A, upper) were additive (Fig. 4B, arrows), indicating a superposition of the two waves. This propagation pattern sharply contrasted the wave patterns in the other two stages (see below).
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35 s (Fig. 4C), indicative of the presence of a long-lasting postwave refractory process (Feller et al. 1997). It was at stage II that spatial boundaries became evident between neighbouring waves. When two waves collided, they annihilated each other (Fig. 3B, lower), instead of superimposing on one another as in stage I (Fig. 3A, lower). Figure 4A (lower) shows two consecutive stage II waves separated by as long as 82 s. Yet, the two waves still formed a clear border between them, such that the second wave stopped right at the boundary of the preceding wave. Interestingly, in an E22 retina, we observed the coexistence of two mechanisms that supported stage I and stage II waves, respectively. As shown in Fig. 4D, this piece of retina initially generated typical stage II waves, which occurred at an interwave interval of 2–3 min and could be completely blocked by 150 µM hexamethonium, suggesting the transition from stage I to stage II waves had already completed. Remarkably, soon after blocking these stage II waves with hexamethonium, the same region of the retina began to generate typical stage I waves, which appeared at an interwave interval of less than 20 s and were no longer sensitive to hexamethonium (150 µM). Thus, blocking stage II waves could induce the reappearance of stage I waves during the transitional period. This result is consistent with our finding that the transition between stages I and II waves occurred abruptly (between E22 and E23), perhaps by a switch between two different mechanisms of wave generation.
Stage III waves.
The emergence of stage III waves in the rabbit began as retinal development progressed beyond the early stage of conventional synaptogenesis, when vesicular glutamate transporters began to appear in the mammalian IPL (Johnson et al. 2003) and early ribbon synaptogenesis in IPL was just about to occur (McArdle et al. 1977). During this period (P4–P8), the waves were insensitive to nicotinic antagonists, but were dependent on glutamatergic and muscarinic drives (Zhou & Zhao, 2000). The transition from stage II to stage III took 2–3 days (P2–P3), during which the emergence of glutamate and muscarinic drives was quite rapid (between P1 and P2), whereas the disappearance of the nicotinic drive took place from P1 to P3/P4. Compared to stage I and stage II waves, spontaneous waves at stage III appeared at a much lower frequency. The average interwave interval reached 228 ± 77 s (n = 10) at stage III, up from 36 ± 18 s and 113 ± 25 s (n = 39) at stages I and II, respectively (Fig. 5B). Many (45%, Fig. 5) stage III waves did not propagate or propagated only a very short distance before dying out (Fig. 5B); they appeared as localized, non-propagating bursts. The amplitude of the Ca2+ rise during a wave (F/F) also became progressively smaller after P4, often making it difficult to detect spontaneous stage III waves. Because of the small amplitude and limited lateral propagation of stage III waves, a quantitative measurement of the wave speed was difficult. The average wave speed of a selection of 12 strong and propagating stage III waves was 159 ± 29 µm s–1.
Notably, we found the progressive weakening of the spontaneous stage III wave with age was associated with the maturation of the GABAergic and glycinergic systems, because picrotoxin and strychnine were very effective in enhancing stage III waves, dramatically increasing the wave frequency and transforming localized bursts of Ca2+ into large propagating Ca2+ waves (Fig. 5). This result suggests a possible role of the inhibitory GABAergic and glycinergic systems in the progressive weakening and final disappearance of stage III spontaneous retinal waves around the time of eye opening (P11) (see below).
Stage-dependent GABAergic regulation of wave dynamics
GABAA/C. To determine whether, in addition to adenosine, acetylcholine and glutamate, other neurotransmitters also contributed to the changing dynamics of retinal waves, we investigated the possible involvement of GABA in modulating the spatiotemporal properties of the waves in rabbit. We first examined the effects of ionotropic GABA receptor antagonists on wave dynamics at various developmental stages (Fig. 5). When SR95531 (100 µM) or picrotoxin (100 µM) was applied to the retina to block GABAA or GABAA/C receptors, respectively, changes in wave dynamics were observed in a stage-dependent manner. At stage I, picrotoxin had no significant effect on any of the wave parameters examined (Fig. 5), including the percentage of waves that were propagating (control: 100%, n = 40; picrotoxin/SR95531: 100%, n = 40), the wavefront speed (control: 449 ± 92 µm s–1, n = 25; picrotoxin/SR95531: 463 ± 80 µm s–1, n = 25) and the interwave interval (control: 37 ± 21 s, n = 60; picrotoxin/SR95531: 37 ± 18 s, n = 20) (Fig. 5).
At stage II, ionotropic GABA currents constituted a significant component of the neurotransmitter input to ganglion and starburst amacrine cells during spontaneous waves (S. Lee and Z. J. Zhou, unpublished observation from patch-clamp recordings). However, blocking this component with picrotoxin or SR95531 had no significant effect on the dynamics of stage II waves. As shown in Fig. 5B, all (100%) stage II waves were propagating, regardless of whether they were in control conditions (n = 40) or in the presence of picrotoxin or SR95531 (n = 40). The wavefront speed was 187 ± 27 µm s–1 (n = 13) in control and 216 ± 55 µm s–1 (n = 16) with picrotoxin/SR95531. The interwave interval was also not significantly different: 106 ± 36 s (n = 18) in control and 126 ± 46 s (n = 16) with picrotoxin/SR95531 (Fig. 5B).
In contrast, as the spontaneous waves became weaker, less frequent and more localized during stage III, picrotoxin or SR95531 became increasingly effective in changing the wave dynamics. In the presence of picrotoxin (100 µM), all of the small and non-propagating spontaneous waves, which accounted for about 45% of the rhythmic bursts seen under the control conditions (n = 10 retinas), were converted to large and propagating waves (Fig. 5A). The average wavefront speed, which became easily measurable in the presence of picrotoxin, was 361 ± 75 µm s–1 (n = 15), much higher than the average speed of the strongest stage III waves in control conditions (159 ± 29, n = 12). The interwave interval was reduced from 228 ± 77 s (n = 20) in controls to 110 ± 31 s (n = 20) in the presence of picrotoxin or SR95331 (Fig. 5B). These results demonstrated that endogenous activation of ionotropic GABA receptors modulated the wave dynamics in an age-dependent manner (Fig. 6B, E, G and H), exerting a strong inhibitory effect only during stage III. The developmental profile of this ionotropic GABAergic inhibition matched the developmental expression pattern of the K+–Cl– cotransporter, KCC2, in the inner mammalian retina (Vu et al. 2000), suggesting a progressive inhibition produced by the shifting of the Cl– equilibrium potential toward a more hyperpolarized potential.
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Transition from a GABAB- to a GABAA-mediated regulation of wave dynamics
The above results showed that the GABAergic system in the developing rabbit retina played an important and stage-dependent role in modulating the spontaneous wave dynamics. The overall effect of GABA modulation was to reduce the level of spontaneous activity, through selective activation of two different families of GABA receptors (Fig. 7). During early development (stage I), when the GABAA system was not yet inhibitory presumably due to a lack of KCC2 expression, the downmodulation of spontaneous retinal waves was mediated by the GABAB system. At stage II, neither GABAA nor GABAB system had a significant effect on the wave dynamics. As the waves progressed to stage III, the GABAA/C system became strongly inhibitory and took over the role of downregulating the waves, while the GABAB system no longer participated in the endogenous modulation of the waves. These results revealed a coordinated, stage-dependent GABAergic modulation of retinal waves mediated by a transition from a metabotropic to an ionotropic GABAergic action.
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Unlike the changing contributions of various neurotransmitter systems to the spontaneous retinal waves, a contribution of gap junctions to wave generation was implicated at all stages of wave development. The gap junction blocker (18ß-GA, 75 µM) was effective in completely blocking spontaneous retinal waves at stages I (Fig. 2A, n = 3), II (Fig. 8B, n = 6) and III (n = 4). When applied at a low concentration (15 µM), 18ß-GA reduced the amplitude and restricted the lateral propagation of stage II waves (Fig. 8B), suggesting a dependence of stage II wave propagation on gap junction communication. The inhibitory effects of 18ß-GA could also be mimicked by octanol-1 (100 µM, Fig. 8A). However, another common gap junction blocker, carbenoxolone (100–200 µM), did not block the waves. The stereoisomer of 18ß-GA, 18
-GA, also did not have a significant effect on the waves up to the highest dissolvable concentration of 75 µM (n = 4), possibly due to a lack of effective concentration or a lack of sensitivity of the gap junctions involved to this drug. Because of the potential side-effects of gap junction blockers in general, the possibility of a non-specific effect of 18ß-GA and octanol-1 on retinal waves cannot be completely ruled out. On the other hand, the very lack of an effect of 18-GA may serve as a control, arguing against a non-specific effect of 18ß-GA on the waves.
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We previously reported spontaneous waves in the VZ of E24–P0 rabbit retinas (Syed et al. 2004). The waves in the VZ and the inner retina (IR) shared a similar speed and frequency and were closely correlated in both space and time. Drugs that blocked IR waves, including hexamethonium and 18ß-GA, also blocked VZ waves; however, atropine blocked only VZ, but not IR waves between E24 and P0 (stage II). We concluded that VZ waves were initiated in the IR and backpropagated to the VZ (Syed et al. 2004).
In this study we investigated whether VZ waves also existed at more than one developmental stage and, if so, how they progressed through various stages. We discovered that, if the retina was mounted loosely on a damp filter paper instead of a dry one, the VZ waves could be better preserved and became detectable in the same age window (E22–P8) as were IR waves, although the probability of finding VZ waves decreased considerably after P2. VZ waves could also be categorized into three stages on the basis of pharmacology. Like IR waves, stage I (E22) VZ waves were insensitive to hexamthonium (300 µM) (Fig. 9A, n = 3), but could be blocked by aminophylline (150 µM, n = 3) (Fig. 9B) and 18ß-GA (75 µM, n = 2) (data not shown). However, in contrast to stage I IR waves which were insensitive to muscarinic antagonists (Fig. 2A), E22 VZ waves could be completely blocked by atropine (1 µM, n = 2) (Fig. 9C), suggesting that VZ waves required additional muscarinic communication. At stage II (P24–P1), VZ waves were inhibited by nicotinic (hexamethonium, 100 µM), muscarinic (pirenzepine, 2 µM, Fig. 9D-E) and gap junction (18ß-GA, 75 µM, data not shown) blockers, but not by CNQX (40 µM) (Fig. 9F) or CNQX (40 µM) + AP7 (100 µM), as we previously found (Syed et al. 2004). At stage III (>P2), the VZ waves were blocked by CNQX (25–40 µM) + AP7 (100 µM) (n = 3) and the muscarinic antagonist pirenzepine (2 µM, n = 2) (Fig. 9G). We also found a transitional period between stages II and III (P2–P4), during which both hexamethonium (150 µM) and CNQX could block the VZ wave (Fig. 9G, n = 2). The nicotinic antagonist ceased to block VZ waves after P5 (Fig. 9H) (n = 2). Taken together, these data suggested that VZ and IR waves progressed through three similar developmental stages and had similar transitional periods. The main pharmacological difference between VZ and IR waves at stages I and II was that atropine blocked only VZ but not IR waves, consistent with our previous finding that stage II VZ waves are dependent on IR waves, but not vice versa, suggesting the waves spread from the inner to the outer retina (Syed et al. 2004). However, in this study, we did not investigate whether stages I and III VZ waves were correlated with IR waves in spatial and temporal domains.
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Discussion |
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TopAbstractIntroductionMethodsResultsDiscussionSupplementary materialReferences |
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The above results provide a systematic characterization of the developmental process of spontaneous waves in both the inner and outer rabbit retina, starting from the initial wave appearance prior to synaptogenesis to the final stage of spontaneous waves before eye opening. As summarized in Fig. 12, our study established three distinct developmental stages of spontaneous waves in the rabbit retina prior to eye opening. These stages coincided with three specific periods of retinal development: pre-synaptogenesis, early conventional synaptogenesis and early ribbon synaptogenesis in the IPL (McArdle et al. 1977; Greiner & Weidman, 1982; Robinson, 1991; Johnson et al. 2003). They are also consistent with the three stages of waves previously reported in the mouse retina (Bansal et al. 2000). More importantly, we found that each stage of wave had a distinct dynamic pattern and pharmacological profile. Stage I waves in the inner rabbit retina were novel in many aspects: they were dependent on gap junction communication but independent of nicotinic interactions; they were fast propagating and lacked the prolonged refractory period typically found at other developmental stages; and, as a result, they appeared at a high frequency and did not observe any boundaries between neighbouring waves. The insensitivity of stage I waves to nicotinic antagonists seems to resemble the pharmacology of the localized activity previously reported in the embryonic mouse retina, where two types of spontaneous activities have been observed: non-propagating, curare-insensitive Ca2+ transients in small clusters of ganglion cells, and large propagating waves that were blocked by nicotinic antagonists (Bansal et al. 2000). It should be distinguished, however, that stage I waves in rabbit were always propagating and uniformly insensitive to nicotinic blockers. Thus, they were different from all previously reported retinal waves.
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3 nAChR (nicotinic acetylcholine receptor) subunit have no stage II retinal waves but exhibit an embryonic form of patterned activity (Bansal et al. 2000). A similar phenomenon has also been reported in the developing spinal cord, where a blockade of one neurotransmitter system (ACh at E4, or glutamate at E11) causes a different system (GABA) to emerge as the new driving force for the spontaneous activity (Chub & O'Donovan, 1998; Milner & Landmesser, 1999). It has been proposed that the early spinal cord network maintains its homeostatic regulation of network firing properties by having multiple mechanisms that are capable of compensating one another when the excitability of one mechanism is reduced (O'Donovan, 1999). Our results suggest that a similar mechanism may also exist in the developing mammalian retina. However, because the waves (stage I) that reappeared 10–15 min after the blockade of the nicotinic system were dramatically different from the original (stage II) waves (Fig. 4D), our results also demonstrated that the coexisting mechanisms, though capable of mutual compensation, are not functionally equivalent. It should also be pointed out that the reversion of stage II waves to stage I after nicotinic blockade was rarely seen. Blocking stage II waves in E29 rabbits, for example, never resulted in an induction of stage I waves. It is thus likely that these compensatory mechanisms only coexisted during the transitional period between two different stages.
Stage III waves in the rabbit are critically dependent on glutamatergic and muscarinic inputs, but not on nicotinic excitation (Zhou & Zhao, 2000). As the retina continued to mature, stage III waves became weaker, less frequent, and spatially more restricted. They were rarely detected after P6–7. The steady decline of stage III waves with age indicated that spontaneous waves would disappear shortly after P8, probably around eye opening (P11). P8 is also the age when rabbit ganglion cells first show light responses (Masland, 1977). However, it should be noted that patch-clamp recordings occasionally found rhythmic activities from starburst and ganglion cells even after eye opening (S. Lee and J. Z. Zhou, unpublished observation). These events occurred in semiperiodic bursts at a frequency (0.2 Hz) much higher than that of stage III waves (0.004 Hz), but they were not observed consistently and could sometimes be disrupted by light stimulation. As the retina further matured, these events were replaced by even more frequent (nearly continuous) bursts of synaptic events (S. Lee and J. Z. Zhou, unpublished observation), suggesting that they might represent an early form of the spontaneous synaptic activity found in the mature retina, although one cannot rule out the possibility that these bursts might be considered yet another stage (stage IV) of spontaneous retinal waves, that appear around eye opening and disappear quickly thereafter. Multielectrode recordings from the GCL of the mouse retina found rhythmic activities around eye opening that were temporally correlated (Demas et al. 2003).
Stage-dependent GABAergic modulation of retinal waves
Our results demonstrated an important role of GABA in regulating the dynamics of mammalian retinal waves, consistent with previous reports in lower vertebrates that GABAB activation modulates retinal waves in the early chick (Catsicas & Mobbs, 2001) and GABAA activation modulates retinal waves in the turtle (Sernagor et al. 2003b). Importantly, we showed that the GABAergic regulation of retinal wave dynamics was stage dependent, involving an interesting transition from a GABAB to a GABAA/C system as development proceeded from stage I to stage III. By using two different families of receptors for the same transmitter, the GABAergic system was able to achieve different levels of regulation at different stages. This is reminiscent of the stage-dependent involvement of the nicotinic (at stage II) and muscarinic (at stage III) systems in the generation of the IR waves in rabbit (Zhou & Zhao, 2000).
Because the early-developing neural network is highly excitable due to the early excitatory actions of GABA and glycine receptor channels (Ben-Ari, 2002), the regulation of spontaneous bursts of excitation in many early-developing networks is thought to be mediated by homeostasis (O'Donovan, 1999). Our finding of the GABAergic inhibition of retinal waves now suggests that neurotransmitter-mediated inhibition also plays an important role in regulating the pattern of early spontaneous retinal waves. This inhibition may be particularly important for stage I waves, since these waves did not have a prolonged postwave refractory period. Although the cellular mechanism of the GABAB modulation of stage I waves in the rabbit remains to be uncovered, it seems that the cyclic AMP pathway is likely to be involved (Catsicas & Mobbs, 2001), since activating adenylate cyclase with forskolin enhanced the wave tremendously (Fig. 2). Thus, the adenosine (probably via A2 receptors) and GABAB systems may act in opposition to regulate the wave dynamics at this early stage of development.
Our result that GABAA/C antagonists dramatically increased the amplitude, frequency, speed and lateral propagation of stage III waves and induced propagating waves in older (>P6) retinas that did not show spontaneous waves suggests an important role of the GABAA/C-mediated inhibition in the decline and eventual disappearance of stage III retinal waves. This conclusion is also consistent with a similar finding in the turtle retina (Sernagor et al. 2003b). While our results clearly demonstrated a role of the GABAergic system in shaping the wave dynamics at stage I and stage III, it is currently unclear and puzzling why blocking endogenous GABA transmission (both GABAA/C and GABAB) apparently did not affect the wave dynamics at stage II (Fig. 3B), even though patch-clamp recordings from rabbit starburst amacrine and ganglion cells showed robust GABAA inputs to these cells during the wave (S. Lee and Z. J. Zhou, unpublished observation). Application of picrotoxin to the ferret retina at a similar stage also did not result in a detectable change in wave dynamics (Stellwagen et al. 1999). Interestingly, a recent report in the turtle (Sernagor et al. 2003a) suggests that GABA input during spontaneous waves may be important for the expression of the K+–Cl– cotransporter, KCC2. Thus, it is possible that the GABA input during stage II waves may be critical for the development of GABAA/C inhibition at stage III, even though GABA does not affect the wave dynamics at stage II.
Spontaneous waves existed over an extensive developmental period and appeared in more than one retinal layer
It has been previously reported that spontaneous retinal activity plays a critical role in the refinement of retinogeniculate and retinocollicular connectivity (Penn et al. 1998; Stellwagen & Shatz, 2002; Grubb et al. 2003; McLaughlin et al. 2003), although the exact function of the waves in retinogenicular development remains controversial (Huberman et al. 2003). Our observation of both VZ and IR waves at all three stages of wave development suggests that rhythmic spontaneous retinal activity is a general developmental phenomenon that is not limited to a single critical period or a single developmental event. The first appearance of the waves at E22 closely correlates in time with the initial arrival of ganglion cell axon terminals at the central visual targets (Crabtree, 1989, 1990; Gayer et al. 1989). Our results show that spontaneous retinal waves are present and may play a role during the entire developmental period of retinogenicular and retinocollicular projections prior to eye opening. Thus, in the case of the developmental sequence of retinogenculate projections, stage I waves correspond to the initial innervation of optic nerve at the dLGN; stage II waves occurred during both the initial establishment of overlapping contra- and ipsilateral retinogeneculate connectivity and the subsequent refinement into eye-specific segregation in the alpha sector of the dLGN, which becomes nearly adult-like at E29–P3 (Gayer et al. 1989; Crabtree, 1990); and stage III waves may correspond to a period of more advanced connectivity refinement in the dLGN, such as ON/OFF segregation (Wong, 1999).
The presence of waves in both the inner and outer retina indicates that the waves are a property of both differentiated and undifferentiated/differentiating cells. Thus the developmental function of retinal waves is likely to be diverse, involving not only the establishment of precise retinofugal projections, but also the development of the retina itself, such as retinal cell cycle (Pearson et al. 2002) and receptive field formation (Sernagor & Grzywacz, 1996). As retinal waves progress from one stage to another (Fig. 12), their functional role will also evolve. Since the spatiotemporal pattern of spontaneous activity is thought to be important in encoding certain developmental cues (Spitzer & Gu, 1997), it seems natural that the wave dynamics are regulated differently at each stage for specific functions. We showed that different neurotransmitter systems shape the wave dynamics at different stages. Conversely, one may speculate that the normal development of these transmitter systems may in turn rely on the cues provided by the wave in a stage-specific manner. A full appreciation of the developmental functions of retinal waves would require the understanding of the complex developmental process and regulation of the waves.
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DOI: 10.1113/jphysiol.2004.066597
http://jp.physoc.org/cgi/content/full/jphysiol.2004.066597/DC1
and contains supplementary material consisting of movies (AVI format) of spontaneous stage I, II and III waves in the ganglion cell layer of Fura-2AM-loaded retinas from E22, E29 and P5 rabbits, respectively. The images in the movies were subtracted by a control image acquired prior to a spontaneous wave and represent difference fluorescence images (F). Darker regions in the images correspond to increases in calcium concentration. The movies are played at 9x the real speed. Frame size: 1.14 mm x 1.14 mm. Representative frames from these movies are also shown in parts of Fig. 3 in this paper.
This material can also be found at:
http://www.blackwellpublishing.com/products/journals/suppmat/tjp/tjp496/tjp496sm.htm
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F) were taken from Fura-2AM-loaded GCL at three developmental stages. The dark areas indicate regions of elevated intracellular Ca2+ associated with the wave. Each row shows two image frames of the same wave(s) together with a cartoon (right) depicting the propagation pattern of the wave(s). A, a stage I (E22) wave with a large wavefront and fast lateral propagation (upper row). When two stage I (E22) waves collided, they superimposed and passed through each other (lower row). B, a stage II (E29) wave propagating as a two-dimensional plane wave (upper row). When two stage II (E29) waves collided, they annihilated each other (lower row). C, stage III waves (P5) were weaker (smaller 
