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The Journal of Neuroscience, January 15, 2003, 23(2):518-529
Vesicular Neurotransmitter Transporter Expression in Developing Postnatal Rodent Retina: GABA and Glycine Precede Glutamate
Juliette Johnson1, 2, Ning Tian5, Matthew S. Caywood2, Richard J. Reimer4, Robert H. Edwards2, 3, and David R. Copenhagen1, 2 Departments of 1 Ophthalmology, 2 Physiology, and 3 Neurology, University of California School of Medicine, San Francisco, California 94143, 4 Department of Neurology and Neurological Sciences, Stanford University School of Medicine, Stanford, California 94305-5489, and 5 Department of Ophthalmology and Visual Science, Yale University School of Medicine, New Haven, Connecticut 06520
ABSTRACT
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ABSTRACT
Introduction
Vesicular transporters regulate the amount and type of neurotransmitter sequestered into synaptic vesicles and, hence, the kind of signal transmitted to postsynaptic neurons. Glutamate is the prominent excitatory neurotransmitter in retina; GABA and glycine are the main inhibitory neurotransmitters. Little is known about the ontogeny of vesicular neurotransmission in retina. We investigated expression of glutamatergic [vesicular glutamate transporter 1 (VGLUT1)] and GABA/glycinergic [vesicular GABA/glycine transporter (VGAT)] vesicular transporters in postnatal retina. VGLUT1 labels glutamatergic synapses. VGLUT1 and synaptic vesicle 2 colocalized to photoreceptor terminals. VGLUT1 colocalized with PKC to rod bipolar terminals and to ON bipolar terminals in metabotropic glutamate receptor 6+/
mice. Developmentally, VGAT expression precedes VGLUT1. In rat and mouse retina, VGAT occurred in the inner retina by postnatal day 1 (P1). In rat retina, VGLUT1 was in the outer retina by P5-P7 and the inner retina by P7. In the mouse retina, VGLUT1 expression was in the outer retina by P3 and the inner retina by P5. Both rat and mouse retina had an adult pattern of VGLUT1 expression by P14. VGLUT1 expression precedes ribbon synapses, which are first observed in the inner retina at P11 (Fisher, 1979
) in mouse and P13 (Horsburgh and Sefton, 1987
Key words: GABA; glycine; glutamate; retina; VGLUT1; VGAT
Introduction
Synaptic transmission depends on the controlled release of synaptic vesicles containing a neurotransmitter. Vesicular transporters regulate the uptake and type of neurotransmitter sequestered into synaptic vesicles and, therefore, the amount and type of neurotransmitter released (Pothos et al., 2000
VGLUT1 transports glutamate with the same kinetics as that reported for vesicular glutamate transport (Bellocchio et al., 2000
VGAT transports GABA with characteristics similar to those reported for vesicular GABAergic transport (McIntire et al., 1997
The expression of specific vesicular transporters directly determines phenotype. GABAergic neurons transfected with VGLUT1 are transformed into glutamatergic neurons (Takamori et al., 2000a
VGAT expression has been investigated in several mammalian retinas, including rat, mouse, rabbit, and monkey. VGAT localized to the outer plexiform layer (OPL) and inner plexiform layer (IPL), with weak immunostaining of cell bodies in the inner nuclear layer (INL) and ganglion cell layer (GCL; Haverkamp et al., 2000
Despite detailed morphological studies of retinal synaptic architecture in developing retina, little is known about the ontogeny of vesicular glutamatergic and GABA/glycinergic synaptic neurotransmission. Recent identification of the vesicular transporters for glutamate and GABA and glycine confers a novel way to determine the onset of vesicular transmission in postnatal retina. We investigated expression of vesicular transporters for glutamate and GABA and glycine in mouse and rat retina. We also studied spontaneous excitatory and inhibitory synaptic inputs to retinal ganglion cells in young mouse retina. Spontaneous EPSCs (sEPSCs) in ganglion cells are present as early as postnatal day 7 (P7). VGLUT1 expression is present before observation of ribbons in the inner retina of mouse (Fisher, 1979
Materials and Methods
Animals and tissue preparation for immunohistochemical experiments. Long-Evans rats (Simonsen, Gilroy, CA) at P1-P40 and adult were used. C57BL/6 mice at P1-P20 and adult (B and K Universal, Fremont, CA) were used. In addition, metabotropic glutamate receptor 6 (mGluR6)+/
20°C until immunostaining.
Antibodies. A rabbit polyclonal antibody for VGLUT1 (also known as brain-specific Na+-dependent inorganic phosphate transporter) was used. This antibody was directed against the last 68 amino acids of a rat VGLUT1 fusion protein (Ni et al., 1994
Monoclonal antibodies against the following proteins were used:
-galactosidase (Chemicon International, Temecula, CA), glutamic acid decarboxylase 6 (GAD6) (obtained from the Developmental Studies Hybridoma Bank, Department of Biological Sciences, University of Iowa, Iowa City, IA), protein kinase C (
,
isoforms, clone MC5; Santa Cruz Biotechnology, Santa Cruz, CA); RIBEYE (a kind gift from Dr. Thomas C. Südhof, University of Texas Southwestern Medical Center, Dallas, TX), and synaptic vesicle 2 (SV2; developed by Kathleen Buckley and obtained from the Developmental Studies Hybridoma Bank). Primary antibodies were detected using affinity-purified goat anti-rabbit Alexa 488, goat anti-rabbit Alexa 594, goat anti-mouse Alexa 488, goat anti-mouse Alexa 594, or goat anti-mouse Alexa 633 (Molecular Probes, Eugene, OR).
Immunohistochemical procedures. Cryostat sections were washed in 0.1 M PB, incubated 12-36 hr in primary antibody with 0.3 or 0.5% Triton X-100 and 10% normal goat serum at 4°C, and then washed in 0.1 M PB. Sections were incubated at a 1:1000 dilution in secondary antibody with 0.3 or 0.5% Triton X-100 and 10% normal goat serum for 1.5-2 hr at room temperature. Sections were coverslipped with Vectashield (Vector Laboratories, Burlingame, CA) to retard fading.
Detection and image processing. Confocal laser-scanning immunofluorescent images were collected using 40× air and 63× oil objectives on a Bio-Rad (Hercules, CA) MRC 1034 confocal microscope. Confocal laser-scanning Nomarski and immunofluorescent images were also obtained using 40× oil, 40× water, 63× water, and 63× oil objectives on a Zeiss (Thornwood, NY) Pascal confocal microscope. For double-labeling studies, sequential confocal scans were collected to prevent bleed-through (Vu et al., 2000
Adobe Photoshop 5.5 (Adobe Systems, Inc., Mountain View, CA) was used to adjust the levels and curves of the confocal images and to make pseudocolor-overlay images. Zeiss confocal Pascal software was used to perform simple intensity profiles of the immunostaining in retinal sections.
Retinal slice preparation. Spontaneous excitatory and inhibitory synaptic inputs to mouse retinal ganglion cells were studied as reported previously (Tian et al., 1998
), which generally took 20-30 min. Membrane currents were recorded with an Axopatch 1D amplifier (Axon Instruments, Foster City, CA), and data were collected using either a Macintosh- or personal computer-based interface (ITC-16 Mac computer interface; Instrutech Corp., Great Neck, NY) run by HEKA software (Pulse + PulseFit; HEKA Elektronik). The signals were filtered at 1 kHz.
sEPSCs were separated from spontaneous IPSCs (sIPSCs) by quantification of rise time, peak amplitude, and monoexponential decay times of spontaneous events. Our previous studies have found that histograms of decay times are separated into a group of faster-decaying events and a group of slower-decaying events. The faster events are glutamatergic AMPA-mediated sEPSCs, whereas the slower events are GABA- and glycine-mediated sIPSCs (Tian et al., 1998
Results
One principal goal of this study was to test whether VGLUT1 is localized to glutamatergic neurons in the retina. Having established this expression pattern, subsequent goals addressed the developmental expression of VGLUT1 in postnatal retina. We were particularly interested in the relative time of expression of VGLUT1 compared with VGAT and whether vesicular excitatory neurotransmission depended on the establishment of ribbons in bipolar synapses.
VGLUT1 is expressed exclusively in the inner and outer plexiform layers of retina
VGLUT1, a vesicular glutamate transporter, is expressed in adult rat and mouse retina. VGLUT1 expression is confined to theouter and inner plexiform layers where vesicular glutamate transmission occurs (Copenhagen and Jahr, 1989
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Figure 1. VGLUT1 immunoreactivity localizes to the synaptic layers of retina. Photomicrographs of vertical sections through rat retina are shown. A, Confocal fluorescence micrograph of VGLUT1 immunolabeling. VGLUT1 expression is confined to the outer and inner plexiform layers where vesicular glutamate transmission occurs. In the OPL, there is intense VGLUT1 immunolabeling. Labeling is absent from the ONL. Discrete and punctate immunostaining was observed across the full extent of the IPL, with larger puncta observed in the inner portion of the IPL near the GCL. B, There was no immunostaining observed when primary antibody was preabsorbed with VGLUT1 fusion protein. Scale bar, 15 µm.
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Figure 2. VGLUT1 colocalizes with the presynaptic protein SV2. Confocal fluorescence micrographs of a vertical section of rat retina are shown. A, D, VGLUT1; B, E, SV2; C, F, overlay of VGLUT1 and SV2. Yellow indicates colocalization. Nearly complete colocalization occurs in the OPL, indicating expression of VGLUT1 in photoreceptor terminals. In the IPL, SV2 immunoreactivity is more widespread than VGLUT1, suggesting that VGLUT1 is expressed in a subset of synapses in the IPL. Scale bars: A-C, 15 µm; D-F, 20 µm.
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Figure 3. VGLUT1 is expressed in both rod and cone ON bipolars. Confocal fluorescent micrographs of a vertical section of rat retina are shown. A, VGLUT1; B, PKC; C, overlay of VGLUT1 and PKC. Yellow indicates colocalization. VGLUT1 and PKC immunoreactivities overlap in punctate structures located at the inner region of the IPL, consistent with expression of VGLUT1 in rod bipolar cell terminals. Staining was performed in retina from mGluR6+/
VGLUT1 is expressed in photoreceptor synaptic terminals
Double-labeling experiments confirmed the exclusive presynaptic localization of VGLUT1 to photoreceptor terminals in the OPL. Figure 2 shows a vertical section of rat retina that was double-labeled with antibodies against VGLUT1 (Fig. 2A,D) and SV2 (Fig. 2B,E). SV2 is a specific marker of synaptic vesicle membrane proteins (Buckley and Kelly, 1985
VGLUT1 is expressed selectively in bipolar cell terminals in the inner plexiform layer
Punctate immunostaining for VGLUT1 was observed throughout the entire extent of the IPL (Figs. 1A, 2A, 3A,D). Small punctate profiles were observed in both the ON and OFF sublamina of the IPL (Wässle et al., 1991
Colocalization of SV2 and VGLUT1 expression in the IPL supports the hypothesis that VGLUT is confined to synaptic terminals (Fig. 2). In the IPL, SV2 labels both conventional and ribbon synapses belonging to amacrine and bipolar cells, respectively (Von Kriegstein et al., 1999
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Figure 4. VGLUT1 is not expressed in GABAergic neurons. Confocal fluorescence micrographs of vertical sections of rat retina are shown. A, In the OPL, VGAT (green) does not colocalize with SV2 (red), a maker of photoreceptor terminals, which express VGLUT1. B, In the inner retina, VGLUT1 (green) and GAD6 (red), a marker of GABAergic synapses, do not colocalize. VGAT and SV2 colocalize to a subset of synapses in the IPL. Vertical sections of rat retina are shown. C, VGAT immunolabeling in the IPL; D, SV2 colocalizing (E) to a subset of GABAergic synapses in the IPL. Yellow indicates colocalization. Scale bars: A, B, 15 µm; C-E, 20 µm.
Confirmation of VGLUT1 expression in rod bipolar cell terminals was determined by double-labeling experiments with the selective rod bipolar cell marker PKC (Greferath et al., 1990
VGLUT1 is the principal vesicular glutamate transporter used by photoreceptors and bipolar cells
VGLUT2, a vesicular glutamate transporter that is closely related to VGLUT1, has recently been localized to glutamatergic synapses (Fremeau et al., 2001
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Figure 5. VGLUT2 does not colocalize with the synaptic marker SV2. Vertical sections of adult rat retina are shown. A, VGLUT2 immunostaining was observed in putative Müller cell processes in the inner portion of the retina, and there was also sometimes faint and diffuse immunostaining of cells bodies in the ganglion cell layer. B, SV2 immunostaining was observed exclusively in the outer and inner plexiform layers. C, Double labeling for VGLUT2 and SV2 shows that these markers do not colocalize. Scale bar, 20 µm.
In summary, our findings show that intense VGLUT1 expression is found in the OPL and is colocalized with SV2 to photoreceptor terminals. VGLUT1 immunolabels punctate profiles throughout the distal and proximal IPL. Colocalization of VGLUT1 with PKC and with LacZ in mGluR6+/
VGAT expression precedes VGLUT1 in developing postnatal rat and mouse retina
We determined the ontogeny of vesicular GABA and glycine and vesicular glutamate transporters by examining the time course of expression of VGAT and VGLUT1. We used SV2 expression as an internal reference, because previous experiments have extensively investigated SV2 expression in the developing rodent retina (Rich et al., 1997
VGAT
As reported previously, prominent VGAT immunolabeling in adult retina was observed in the OPL and in the IPL, whereas weak immunostaining was observed in cell bodies in the INL and GCL (Figs. 4A,C-E, 6, 7) (Haverkamp et al., 2000
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Figure 6. Vertical sections showing the postnatal development of VGAT in the rat retina. VGAT was present in the inner retina by P1. Retinal layers are shown with Nomarski optics adjacent to the micrographs. Intensity profiles are also included for each fluorescent image. VGAT immunolabeling was examined at the following ages: A, P1; B, P3; C, P5; D, P7; E, P10; F, P14. Scale bar, 20 µm.
Figure 6 shows VGAT immunostaining in developing postnatal rat retina. Vertical retinal sections were examined at ages P1, P3, P5, P7, P10, and P14. Adjacent to the immunolabeling are Nomarski images and intensity profiles. VGAT expression was first observed by P1 in the inner retina (Fig. 6A), and faint immunostaining was detected in the outer retina by P5-P7 (Fig. 6C,D). VGAT immunostaining had an adult pattern of expression by P10. A developmental series of VGAT immunostaining in the mouse retina was investigated at ages P1, P3, P5, P7, P10, and P14 (Fig. 7). VGAT expression was observed by P1 in the inner retina, and faint immunolabeling was detected by P3 in the outer retina (Fig. 7A). VGAT immunolabeling had an adult pattern of expression by P7. Taken together, these findings indicate that VGAT expression is present in the inner retina by P1, and that vesicular GABA/glycinergic transmission is possible at an early age.
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Figure 7. Vertical sections showing the postnatal development of VGAT in the mouse retina. VGAT immunostaining was observed in the inner retina by P1. Retinal layers are shown with Nomarski optics adjacent to the micrographs. Intensity profiles are also included for each fluorescent image. VGAT immunolabeling was examined at the following ages: A, P1; B, P3; C, P5; D, P7; E, P10; F, P14. Scale bar, 20 µm.
VGLUT1
Our developmental studies in rat and mouse retina show that VGLUT1 has a delayed temporal onset of expression compared with VGAT and SV2; VGLUT1 expression is first observed in the outer retina followed by the inner retina. Figure 8 shows VGLUT1 immunostaining at ages P1, P3, P5, P7, P10, and P14 in the rat retina. Nomarski images and intensity profiles are adjacent to the VGLUT1 immunostaining. VGLUT1 immunostaining was first observed by P5-P7 in the outer retina (Fig. 8C,D), and by P7 in the inner retina (Fig. 8D). VGLUT1 immunostaining acquires an adult-like pattern by P14 (Fig. 9F). At ages P7 and P10, VGLUT1 has a selective distribution to presumptive ON and OFF strata of bipolar terminals in the IPL (Figs. 8A-F, 9). Figure 9 shows a P7 rat retina immunostained for VGLUT1 (Fig. 9A), and SV2 (Fig. 9B). The VGLUT1 stratification pattern in the IPL was not present in the SV2 immunostaining, which labeled the entire IPL (Fig. 9B). VGLUT1 expression was also examined in developing postnatal mouse retina at ages P1, P3, P5, P7, P10, and P14 (Fig. 10). VGLUT1 immunostaining was detected in the outer retina by P3 (Fig. 10B,C) and in the inner retina by P5 (Fig. 10C,D). An adult pattern of expression was found by P14. Our findings indicate that VGLUT1 expression is delayed in comparison with VGAT, and that vesicular glutamatergic transmission is possible by P7 in the inner retina of mouse and rat retina.
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Figure 8. Vertical sections of postnatal developing rat retina immunostained for VGLUT1. VGLUT1 had delayed expression compared with VGAT. VGLUT1 was observed in the outer retina by P5-P7 and in the inner retina by P7. Retinal layers are shown with Nomarski optics adjacent to the micrographs. Intensity profiles are also included for each fluorescent image. VGLUT1 immunolabeling was examined at the following ages: A, P1; B, P3; C, P5; D, P7; E, P10; F, P14. Scale bar, 20 µm.
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Figure 9. VGLUT1 has a selective distribution to presumptive ON and OFF strata of bipolar terminals in the IPL of P7 rat retina. Vertical sections of P7 rat retina are shown. Nomarski optics are shown adjacent to the immunofluorescence micrographs. A, VGLUT1 immunostaining is present in two strata in the IPL. B, This distinct stratification pattern is not present in SV2 immunolabeling. Scale bar, 20 µm.
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Figure 10. Vertical sections immunostained for VGLUT1 in the postnatal developing mouse retina. VGLUT1 expression was delayed compared with VGAT. VGLUT1 was first observed in the outer retina by P3 and the inner retina by P5. Retinal layers are shown with Nomarski optics adjacent to the micrographs. Intensity profiles are also included for each fluorescent image. VGLUT1 immunolabeling was examined at the following ages: A, P1; B, P3; C, P5; D, P7; E, P10; F, P14. Scale bar, 20 µm.
SV2
We examined SV2 expression in postnatal rat and mouse retina. We used this as an internal reference, because SV2 expression in developing rodent retina has been thoroughly investigated (Rich et al., 1997
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Figure 11. Vertical sections showing the postnatal development of SV2 in the rat retina. SV2 immunolabeling was present in the inner retina by P1. Retinal layers are shown with Nomarski optics adjacent to the micrographs. Intensity profiles are also included for each fluorescent image. SV2 immunolabeling was examined at the following ages: A, P1; B, P3; C, P5; D, P7; E, P10; F, P14. Scale bar, 20 µm.
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Figure 12. Vertical sections showing the postnatal development of SV2 in the mouse retina. SV2 had an early onset of expression and was first observed in the inner retina by P1. Retinal layers are shown with Nomarski optics adjacent to the micrographs. Intensity profiles are also included for each fluorescent image. SV2 immunolabeling was examined at the following ages: A, P1; B, P3; C, P5; D, P7; E, P10; F, P14. Scale bar, 20 µm.
RIBEYE
We examined expression of an antibody against RIBEYE in developing rat retina. Previous studies have found that RIBEYE is a component of the ribbon synapse (Schmitz et al., 2000
In summary, these findings show that vesicular GABA/glycinergic transmission is possible in the inner retina by P1, whereas vesicular glutamatergic transmission has a delayed onset. VGLUT1 expression is observed at a time before ribbon structures are observed in bipolar cell terminals, suggesting that vesicular glutamatergic transmission occurs before the formation of ribbon synapses in bipolar cells.
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Figure 13. RIBEYE is not present in the inner rat retina by P7, an age at which there is strong immunostaining for VGLUT1. Vertical sections of postnatal rat retina immunostained for RIBEYE are shown. RIBEYE immunoreactivity is not present in the outer or inner retina of P5 or P7 rat. Some nonspecific immunostaining of cell bodies was present in the INL and GCL at all ages examined. RIBEYE immunoreactivity is observed in the OPL of P10 rat retina, along with barely detectable immunostaining in the IPL. Robust immunostaining for RIBEYE was present in the OPL and IPL of P14 retina. RIBEYE localized to the OPL and IPL in P15 and P21 retina. Retinal layers are shown with Nomarski optics adjacent to the micrographs. Intensity profiles are also included for each fluorescent image. RIBEYE immunolabeling was examined at the following ages: A, P5; B, P7; C, P10; D, P14; E, P15; F, P21. Scale bar, 20 µm.
Spontaneous excitatory and inhibitory synaptic events are observed in mouse retinal ganglion cells as early as P7
We sought to determine whether sEPSCs to mouse retinal ganglion cells occur at an age when VGLUT1 expression is present but precedes the establishment of ribbon synapses in the inner retina. We examined spontaneous events to mouse retinal ganglion cells at ages P7-P9, P10-P12, and P13-P15. Previous work by our laboratory has investigated spontaneous excitatory and inhibitory synaptic inputs to retinal ganglion cells in mouse retina. These studies have found that histograms of the decay times of the spontaneous events allow for the separation of the events into two groups, a faster-decaying event group and a slower-decaying event group. The faster event group consists of AMPA-mediated glutamatergic sEPSCs, whereas the slower event group consists of GABA- and glycine-mediated sIPSCs (Tian et al., 1998
Figure 14A shows a representative 5 min recording from a retinal ganglion cell of P7 mouse retina. The inset shows a single sEPSC and sIPSC on an expanded time scale. The rise time, peak amplitude, and monoexponential decay times of sEPSCs and sIPSCs were calculated from three groups of animals aged P7-P9, P10-P12, and P13-P16 (Fig. 14B). The average frequency (events per minute) of sEPSCs and sIPSCs increased with age. For example, at P7-P9, the average frequencies of sEPSCs and sIPSCs were 6.89 ± 2.84 and 8.18 ± 2.81 events/min, respectively. At P10-P12, the average frequencies of sEPSCs and sIPSCs increased to 23.1 ± 7.01 and 18.59 ± 5.43 events/min, and by P13-P16, they were 32.79 ± 8.19 and 20.08 ± 4.91 events/min, respectively.
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Figure 14. A, Representative 5 min recording of retinal ganglion cell membrane currents from a P7 mouse retina. Individual spontaneous events in the records were first detected and then quantified by the rise time, peak amplitude, and monoexponential decay times. In our previous studies, histograms of decay times showed a clear demarcation between a group of faster-decaying events and a group of slower-decaying events. The faster events were AMPA-mediated glutamatergic sEPSCs, and the slower ones were GABA- and glycine-mediated sIPSCs (Tian et al., 1998 , monoexponential decay time constant of the averaged waveforms ± SE; n, number of events for the calculation of each averaged waveform. ANOVA tests showed that the differences among the amplitudes of sEPSCs from the three age groups were not statistically significant (p = 0.2817). However, differences of the decay time constants between P7-P9 and P10-P12 and between P10-P12 and P13-P15 were significant (p = 0.0289; p < 0.0001, respectively). ANOVA tests also showed that the difference of the sIPSC amplitudes between P10-P12 and P13-P15 mice was statistically significant (p = 0.0005). The differences of decay time constants between P7-P9 and P10-P12 and between P7-P9 and P13-P15 were significant (p < 0.0001). C, Average frequency (events per minute) of retinal ganglion cell sEPSCs as a function of postnatal age. The difference of the average sEPSC frequency between P7-P9 and P13-P16 mice was statistically significant (**p = 0.042; ANOVA). D, Average frequency (events per minute) of retinal ganglion cell sIPSCs as a function of postnatal age. The difference of the average sIPSC frequency among these three groups of mice was not statistically significant (p = 0.371; ANOVA).
ANOVA tests were performed to determine statistically significant results. There was a significant difference in the average sEPSCs frequency between P7-P9 and P13-P16 aged mice (Fig. 14C) (p = 0.042; ANOVA). The average frequency of sIPSCs among the three groups of mice was not statistically significant. sEPSCs and sIPSCs were observed as early as P7. Our findings indicate the presence of vesicular glutamatergic and vesicular GABA and glycine neurotransmission as early as P7 in the inner retina of the mouse.
Discussion
We show here that VGLUT1 immunoreactivity in adult rat and mouse retina is found exclusively in the terminals of photoreceptor and bipolar cells, which are the principal glutamatergic neurons in the retina. VGLUT1 immunoreactivity colocalized with the synaptic vesicle marker SV2 to photoreceptor terminals in the OPL. VGLUT1 immunolabeling was found in a subset of SV2 synapses in the IPL, and VGLUT1 colocalized with PKC to rod bipolar terminals in the IPL. VGLUT1 also colocalized with LacZ to ON rod and cone bipolar terminals in mGlur6+/
We found that VGAT expression precedes VGLUT1 expression in postnatal mouse and rat retina. VGAT expression was present in the inner retina by P1 in mouse and rat retina, suggesting that vesicular GABA/glycinergic transmission is possible at an early age. We found sIPSCs in retinal ganglion cells as early as P7 in mouse retina. Furthermore, our studies demonstrate that VGLUT1 expression is present before the establishment of ribbon synapses in the inner retina of mouse (Fisher, 1979
Localization of VGLUT1 in adult retina
VGLUT1 was localized exclusively to photoreceptor and bipolar terminals. These cells have a specialized synapse called a ribbon synapse. Photoreceptors in the OPL and bipolar cells in the IPL release glutamate in a tonic manner, which is regulated by small graded changes in the presynaptic potential (von Gersdorff et al., 1996
Developmental expression of VGAT and VGLUT1 in the retina
VGAT and VGLUT1 expression was investigated in developing postnatal rat and mouse retina. In the rat and mouse retina, VGAT expression was observed at P1 in the inner retina. In the rat retina, VGLUT1 was found at P5-P7 in the outer retina and by P7 in the inner retina. In the mouse retina, VGLUT1 was observed at P3 in the outer retina and at P5 in the inner retina.
VGAT expression precedes VGLUT1 expression
Our observation of VGAT expression in P1 inner retina indicates that vesicular GABA/glycinergic transmission is possible at this young age. In the mouse retina, conventional synapses in the inner retina are first detected at P3 (Fisher, 1979
GABA is thought to have a neurotrophic role in the developing retina. For example, addition of GABAA receptor antagonists to rabbit explant cultures disrupts cone photoreceptor synaptogenesis (Huang et al., 2000
VGLUT1 expression may precede formation of ribbon synapses in the inner retina
VGLUT1 expression was present in the inner retina at an age when ribbon synapses are not yet observed. For example, VGLUT1 expression was present in P7 inner retina in the mouse and rat retina. In the mouse retina, electron microscopic studies have found that ribbon synapses are first detected at P11 (Fisher, 1979
In agreement with our hypothesis that vesicular glutamate release precedes ribbon synapse formation in the inner retina, we found that sEPSCs in mouse retinal ganglion cells are present as early as P7 (Fig. 14). Interestingly, there was an increase with age in the average frequency of sEPSCs from mice aged P7-P9, P10-P12, and P13-P16. There was a significant difference between the average frequency of sEPSCs of P7-P9 and P13-P16 mice. This increase in the average frequency of sEPSCs in the different age groups may correspond to the establishment of functional ribbon synapses, which may bolster the efficiency of vesicular glutamatergic transmission and result in an increased frequency of release. In agreement with our results, other studies have found glutamatergic inputs in young retina. For example, at P5 in rat retina, glutamatergic sEPSCs were observed in retinal ganglion cells (Rorig and Grantyn, 1993
FOOTNOTES Received Sept. 12, 2002; revised Oct. 24, 2002; accepted Oct. 25, 2002.
This work was supported primarily by National Institutes of Health grants (D.R.C. and R.H.E). Additional support was provided by a National Eye Institute core grant, That Man May See (D.R.C), and Research to Prevent Blindness (D.R.C). We thank Dr. René Renteria and Dr. David Krizaj for valuable discussions during the course of this study, Dr. Thomas C. Südhof for the RIBEYE antibody, and Edwin Dumlao for technical assistance.
Correspondence should be addressed to Dr. Juliette Johnson, Department of Ophthalmology, University of California, San Francisco, School of Medicine, 10 Kirkham Street, Room K-140, San Francisco, CA 94143-0730. E-mail: cjj{at}itsa.ucsf.edu.
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