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The Journal of Neuroscience, January 1, 2000, 20(1):306-314
Segregation of On and Off Bipolar Cell Axonal Arbors in the Absence of Retinal Ganglion Cells
Emine Günhan-Agar, Dianna Kahn, and Leo M. Chalupa Section of Neurobiology, Physiology, and Behavior, Department of Psychology and Center for Neuroscience, University of California, Davis, California 95616
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Retinal cells that respond selectively to light onset or offset are segregated into On and Off pathways. Here, we describe the development of cone bipolar cells whose axonal arbors at maturity synapse onto ganglion cell dendrites confined to On and Off strata of the inner plexiform layer (IPL). In particular, we sought to determine whether the formation of this segregated pattern is dependent on the presence of ganglion cells. Developing bipolar cells were visualized using an antibody against recoverin, the calcium binding protein that labels On and Off cone bipolar cells in the adult rat retina. Recoverin-positive cells were apparent in the ventricular zone on the day of birth [postnatal day 0 (P0)], before bipolar cells begin to migrate to the inner nuclear layer. Two distinct strata were first apparent in the IPL at P8, with the Off pathway maturing earlier than the On pathway. There was no indication of exuberant bipolar cell projections. Throughout development, there were also a small number of recoverin-positive cells of unknown origin in the ganglion cell layer.
To assess whether the formation of On and Off cone bipolar cell projections is dependent on the presence of ganglion cells, these target neurons were eliminated by unilateral section of the optic nerve. This was done on the day of birth, resulting in a total loss of ganglion cells 5-6 d before bipolar cell axons innervate the IPL. In retinas with optic nerve sections, On and Off cone bipolar cells were present, albeit at a lower than normal density, and the axonal arbors of these interneurons were organized into two distinct strata. This indicates that ganglion cells are not essential for the formation of segregated On and Off bipolar cell inputs. These results lend support to the hypothesis that specific ingrowth patterns of bipolar cell terminal arbors could regulate the formation of stratified retinal ganglion cell dendrites.
Key words: On and Off pathways; bipolar cells; ganglion cells; retina; recoverin; development
INTRODUCTION
A fundamental feature of the vertebrate retina is the separation of On and Off channels into functionally and structurally distinct pathways (Famiglietti and Kolb, 1976
; Nelson et al., 1978
In contrast to this separation of On and Off pathways in the adult retina, early in development the dendrites of retinal ganglion cells ramify throughout the IPL. The restriction of these processes into On and Off sublaminae occurs during the period when bipolar cells form synapses with ganglion cells (Maslim and Stone, 1986
To explain how bipolar cell activity could regulate the stratification of ganglion cells, a model has been proposed that assumes On and Off bipolar cells selectively innervate either the proximal or the distal aspect of initially multistratified dendrites (Bodnarenko et al., 1995
Our main objective was to determine whether retinal ganglion cells, the main targets of bipolar cells, are required for the segregation of bipolar cell axons into On and Off sublaminae of the IPL. Ganglion cells were depleted by sectioning an optic nerve in newborn rats, before the time when bipolar cells begin to innervate the IPL. This revealed that bipolar cells can form segregated On and Off projections in the absence of retinal ganglion cells, although this manipulation causes a significant decrease in the incidence of such interneurons. Thus, whereas the stratification of retinal ganglion cell dendrites into On and Off sublaminae is regulated by bipolar cell activity (Bodnarenko and Chalupa, 1993
MATERIALS AND METHODS
All procedures were performed in strict compliance with the protocol approved by the Animal Care and Use Committee of the University of California at Davis.
Surgical procedures. Time pregnant Long-Evans rats were obtained from Simonsen Laboratories (Gilroy, CA). Unilateral optic nerve sections were performed on the day of birth, defined as postnatal day 0 (P0). The pups were anesthetized by hypothermia, and the frontal portion of the brain was exposed by an incision in the skin and skull. The frontal cortex and the optic nerve were aspirated under visual guidance using a blunt needle attached to a vacuum pump. Animals were returned to their mother after recovery until they were killed at 3-4 weeks of age.
Tissue preparation. Normal postnatal pups (between P0 and P16) and 3- to 4-week-old experimental animals (that had one optic nerve sectioned at P0) were killed by an intraperitoneal injection of sodium pentobarbital. The animals were then perfused transcardially with 4% paraformaldehyde solution, followed by 0.9% saline solution. The eyecups were removed, hemisected, and post-fixed with 4% paraformaldehyde.
Primary antibodies. A polyclonal antibody against 23 kDa calcium-binding protein, recoverin (gift from Dr. A. Dizhoor, Wayne State University, Detroit, MI), was used at dilutions of 1:10000-1:20000 to label the bipolar cells.
A monoclonal antibody against the Thy1.1 surface glycoprotein (clone OX-7; Chemicon, Temecula, CA) was used at dilutions of 1:10000-1:20000 to label retinal ganglion cells.
A monoclonal antibody against the rat rhodopsin antigen (clone RET-P1; Biodesign International, Kennebunk, ME) was used at dilutions of 1:50-1:100 to label rod photoreceptors.
Secondary antibodies. All of the secondary antibodies were purchased from Jackson ImmunoResearch (West Grove, PA). Cy-3-conjugated goat anti-rabbit IgG (1:200 dilution) or biotnylated goat anti-rabbit IgG (1:500 dilution) for recoverin and biotnylated goat anti-mouse IgG (1:500 dilution) for Thy1.1 was used as secondary antibodies. For double labeling with recoverin and rhodopsin antibodies, rhodamine redX-conjugated goat anti-rabbit IgG (1:200 dilution) and biotnylated goat anti-mouse IgG (1:500 dilution) were used. Both antibodies were prepared for double-labeling experiments to prevent cross-reaction with opposite species. Streptavidin-conjugated Alexa-408 fluorescent probe (Molecular Probes, Eugene, OR) was used to visualize rhodopsin immunolabeling.
Immunohistochemistry. After post-fixation for 2-4 hr, hemisected eyes were immersed in gradually increasing concentrations of sucrose solution (5, 15, and 30%) to cryoprotect the tissue. Vertical sections were taken at a thickness of 10-15 µm on a cryostat and mounted on subbed slides. All incubations were performed at room temperature. Sections were preincubated in blocking solution [10% normal goat serum, 0.3% Triton X-100, and 1% bovine serum albumin in PBS] for 1 hr. The primary antibodies were diluted in blocking solution. The sections were incubated in the primary antibody solution for 1-2 hr. After several washes with PBS, the sections were incubated in the secondary antibody diluted in blocking solution for 1-2 hr. Primary antibody incubation was omitted for control slides in each procedure.
To minimize the high background problem caused by Thy1.1 primary antibody in rat retina, we used the indirect tyramide signal amplification method (NEN Life Science, Boston, MA) for Thy1.1 immunostaining. After incubation with primary and biotnylated secondary antibodies, sections were incubated with streptavidin-HRP (diluted 1:100 in blocking buffer) for 30 min, followed by incubation with the amplification agent for 10 min. Streptavidin-HRP incubation was repeated, and peroxidase was visualized with 0.001% DAB and 0.003% H2O2 in PBS.
The indirect immunofluroscence technique was used to visualize recoverin immunolabeling for quantitative analysis. After incubation with primary and biotnylated secondary antibodies, sections were incubated for 1 hr in the Vectastain Elite ABC kit (Vector Laboratories, Burlingame, CA), and peroxidase was visualized with 0.001% DAB and 0.003% H2O2 in PBS.
For double-labeling studies, sections were incubated in a mixture of two primary antibodies, rinsed with PBS, and incubated in a mixture of two secondary antibodies.
After final washes, slides for epifluroscence and confocal microscopy were coverslipped with Citifluor (Ted Pella, Redding, CA), and slides for bright-field microscopy were coverslipped with Vectamount (Vector Laboratories).
Nissl staining. Vertical sections at a thickness of 20-25 µm were obtained on a cryostat for both experimental and control eyes. Sections were stained with 0.1% thionin in sodium acetate buffer for 2 hr at room temperature. Slides were washed, dehydrated, and coverslipped with Vectamount.
1,1'-Dioctadecyl-3,3,3'3'-tetrametylindocarbocyanine perchlorate labeling. Six adult rats with unilateral optic nerve sections at P0 were perfused with 0.9% isotonic saline, followed by 4% paraformaldehyde. Both experimental and control eyes were removed and hemisected, and whole retinas were taken out. The retinas were embedded in 5% agar, and vertical sections were obtained with a vibratome at a 200 µm thickness. Crystals of 1,1'-dioctadecyl-3,3,3'3'-tetrametylindocarbocyanine perchlorate (DiI) (Molecular Probes, Eugene, OR) were put into the IPL or outer plexiform layer (OPL). Sections were kept in an oven (37°C) for 12-24 hr to allow dye diffusion.
Imaging. Bright-field photomicrographs were taken by a digital camera (Optronics International, Chelmsford, MA) attached to a Nikon (Tokyo, Japan) eclipse E600 microscope and viewed by differential interference contrast optics. Confocal images for immunofluorescence and DiI labelings were acquired by either Bio-Rad (Hercules, CA) MRC 1024 ES or Leica (Nussloch, Germany) TCS-SP confocal microscope equipped with argon-krypton laser in epifluorescence-confocal mode. Three lines (488, 568, and 647) in argon-krypton laser, Nomarski filters, and prisms, plus transmitted light detector, were used to create Nomarski images. A stack of images along the z-axis (0.5-2.0 µm steps) was collected for each slide. For illustrative purposes, selected images of DiI-labeled cells were printed and traced on a light box with drawing pens.
Cell counts. Recoverin-positive bipolar cells were counted in immunostained sections from six animals that had an unilateral optic nerve section at P0. Ten separate regions in each section (including peripheral, paracentral, and central retina) were counted, and four to six sections from each eye (six control and six experimental) were analyzed. Stereological techniques were used to determine the number of recoverin-labeled cells in the inner nuclear layer (INL) (Sterio, 1984
where NV Recoverin/INL is the number of recoverin-positive cells per volume of INL, NRecoverin is the number of recoverin-positive cells counted in 10-15 µm sections, excluding those that intersected the top of the section and two sides of the counting frame, AINL is the area of INL in the counting frame, HINL is the height of the optical dissector (usually 15 µm), and a/p is the area per point for the objective used (100×, 1.30 oil; Olympus Optical, Tokyo, Japan).
INL, IPL, and cell body measurements. The thickness of the INL and IPL and the soma size of the recoverin-labeled bipolar cells were measured in both the control and experimental animals using NIH Image software. Bright-field images viewed by Nomarski optics were captured on the computer screen using the digital camera attached to the microscope. Twelve measurements per section were taken (four each from the peripheral, paracentral, and central retina), and four to six sections were analyzed from each of the five animals that sustained optic nerve sections.
Statistical analysis. The data were analyzed by ANOVA using the general linear model procedure (SAS Institute, Cary, NC), followed by Duncan's multiple range test with a significance level of p < 0.05.
RESULTS
Figure 1 illustrates the recoverin labeling pattern in the adult rat. As can be seen in the low-power photomicrographs obtained from the central (Fig. 1A) and peripheral (Fig. 1B) regions of the retina, recoverin labels the somas of bipolar cells in the INL, as well as the processes of these interneurons that terminate in two distinct sublaminae of the IPL. Note that the separation between the On and Off strata in the IPL is greater in the central than the peripheral retina, reflecting central-to-peripheral differences in overall retinal thickness attributable to differential growth of the retina during development (Mastronarde et al., 1984
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Figure 1. Confocal images of recoverin-labeled cells in the central (A) and peripheral (B) sections of the adult rat retina. In this and all other figures, the photoreceptor layer is up, and the ganglion cell layer is down. Recoverin labels photoreceptors in the outer nuclear layer and two types of cone bipolar cells in the inner nuclear layer whose axon terminals form two strata in the inner plexiform layer. C, A higher power image illustrating two recoverin-labeled bipolar cells. Note that, in both cases, the axonal processes (indicated by arrows) could be visualized from the soma to the terminal in sublamina a (cell on the right) or in sublamina b (cell on the left). Scale bars, 50 µm.
Cells expressing recoverin were evident in the ventricular zone at P0 (data not shown). Figure 2 illustrates the developmental changes in recoverin labeling patterns between P1 and P12. As may be seen at P1, recoverin-positive cells are migrating from the ventricular zone toward the inner retina. At older ages (P3-P7), there is a progressive increase in the intensity of staining within the outer retina. At P6, recoverin-positive cells were noted within the INL (data not shown), and at P7, labeled terminal arbors were evident within the IPL (Fig. 2, arrow). In some cases, these could be observed to originate from presumed bipolar cells within the INL. By P8, a clear band of labeled processes was evident in the IPL (indicated by arrows), corresponding to sublamina a in which the axons of Off cone cells form synaptic contacts with the dendrites of Off ganglion cells. In comparison, there was only a hint of a laminar organization in the prospective sublamina b, corresponding to the On pathway (Fig. 2, inset). At P12, both the On and Off strata were clearly apparent, but note that at this age the On pathway is still less dense than in the adult animal (compare Fig. 2, P12, with Fig. 1A,B). By P16, recoverin labeling in both sublaminae appeared indistinguishable from that observed in the adult animal (data not shown).
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Figure 2. Superimposed confocal and Nomarski images of recoverin labeling patterns for P1-P12 rat retinas. Recoverin labels putative bipolar cells (as well as rod photoreceptors) in the ventricular zone and cells that are migrating toward the inner nuclear layer (P1-P5). At P7, some recoverin-labeled bipolar cells are present in the inner nuclear layer, and the axon terminals of these cells can be identified in the IPL (arrow). At P8, two strata of axon terminals in the IPL can be seen (arrows). At this age, the Off layer is well defined, whereas the On layer is just beginning to be formed. The inset shows a higher power image of the square indicated on the photomicrograph. By P12, both the On and Off strata are well defined. Note at all ages the presence of some recoverin-positive profiles in the ganglion cell layer. Scale bars, 20 µm.
Also clearly apparent in Figure 2 are recoverin-labeled cells within the developing ganglion cell layer. Such labeled profiles, first observed at P1, were present at all postnatal ages, as well as in the adult retina. In the adult retina (Fig. 3), these were variable in shape and size, and in many cases dendritic and/or axonal processes could be seen to originate from particular somas. The properties of such cells will be considered in detail elsewhere (Günhan-Agar and Chalupa, 1999
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Figure 3. Confocal images of recoverin-labeled cells in the ganglion cell layer of the adult rat retina. A, Low-power image showing all retinal layers. B, Higher magnification of the recoverin-labeled cells in the ganglion cell layer. Scale bars, 20 µm.
Because recoverin is expressed by photoreceptors that are born during an overlapping time period with bipolar cells (Morest, 1970
In many developing systems, target neurons are known to play a crucial role in the establishment or the refinement of projection patterns, as well as in the survival of afferent neurons (Murphy and Kalil, 1979
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Figure 4. Bright-field-Nomarski images of Nissl (A, B) and Thy1.1 (C, D) stainings in normal (A, C) and optic nerve-transected rat retinas (B, D). Black lines indicate the limits of the ganglion cell layer in all four pictures. Note that the large Nissl-stained cells and Thy1.1-labeled cells are missing in the ganglion cell layer of optic nerve-transected retinas (B, D). Scale bar, 50 µm.
We next assessed whether or not retinal ganglion cells are required for the formation of segregated On and Off bipolar cell strata within the IPL. This was done by labeling cells with recoverin or with DiI after deposits of this tracer into the IPL or OPL in fixed sections.
Examination of the recoverin labeling in the INL of animals that sustained optic nerve sections revealed that bipolar cell axon terminals were stratified into two distinct layers within the IPL (Fig. 5). This was the case in all six animals in which this manipulation was performed. The retinas of the experimental animals were also substantially thinner than normal. To a large degree, this reflected the shrunken ganglion cell layer (Fig. 4), but measures of the other retinal layers revealed that the IPL was also significantly thinner so that the overall separation between the On and Off strata was less than normal. Counts of recoverin-positive profiles showed that the incidence of such neurons was also significantly lower in the retinas with optic nerve section, but soma size did not differ from normal. These measurements are summarized in Table 1.
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Figure 5. Bright-field images of recoverin labeling in the normal (A) and optic nerve-transected (B) retinas. Note that the labeling patterns are the same in both cases, although the density of labeled cells in the inner nuclear layer and the distance separating the two strata in the inner plexiform layer are less in B than in A. Scale bar, 50 µm.
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Table 1. Quantitative analysis of recoverin-immunostained retinas The DiI labeling confirmed the segregation of bipolar cell terminals and provided additional information about the morphological properties of these neurons. As may be seen in Figure 6, the axons of individual neurons in both the normal and experimental animals terminated in a confined region of the IPL. An examination of 100 bipolar cells labeled with DiI in the experimental retinas and 130 such neurons in control retinas revealed no cells with bifurcating axonal processes. Moreover, the terminal arbors of all neurons, although showing considerable heterogeneity in size and shape, appeared confined to a given strata of the IPL. It should be noted that our deposits of DiI most likely labeled all classes of bipolar cells, not just those expressing recoverin (cf. Euler and Wassle, 1995
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Figure 6. Drawings of DiI-labeled bipolar cells. A-D are bipolar cells from normal retinas, and E-H are bipolar cells from optic nerve-transected retinas. Note that, in all cases, the axons terminate in a confined region of the inner plexiform layer. Scale bar, 10 µm.
DISCUSSION
We have shown that the antibody against the calcium binding protein, recoverin, which labels On and Off cone bipolar cells in the mature retina (Milam et al., 1993
The formation of stratified On and Off cone bipolar cell projections does not appear to involve an intermingling of the processes of these interneurons. Indeed, we are struck by the remarkable degree of specificity exhibited by On and Off bipolar cell axons. At P8, a clearly defined strata corresponding to terminals of Off cone bipolar cells is present, but at this age, the On strata is just beginning to appear. The earlier formation of the Off sublamina of the IPL observed here with recoverin immunocytochemistry corresponds to the temporal sequence of synapse formation between bipolar cells and ganglion cells noted in the developing monkey retina (Okada et al., 1994
Stratification of bipolar cells after ganglion cell loss
Previous studies have shown that optic nerve section in the neonatal rat results in rapid and complete loss of ganglion cells, with most cells dying within 48 hr of this procedure (Perry et al., 1983
This raises the question of why certain recoverin-immunoreactive bipolar cells would be eliminated while others (the majority) would survive after section of the optic nerve. One possibility is that the bipolar cells that were lost failed to make synaptic contacts with ganglion cells or with interneurons eliminated by the optic nerve section. The lack of such targets would presumably deprive these afferents of essential trophic factors, leading to their elimination. Along the same line, the bipolar cells that survived optic nerve section may be neurons that make synaptic contacts primarily with amacrine cells that were unaffected by ganglion cell loss. This explanation assumes that cone bipolar cells in the rat comprise different subtypes based on their synaptic contacts, as has been demonstrated in the cat retina (Cohen and Sterling, 1990
Despite these changes in the inner nuclear and synaptic layers, a large contingent of recoverin-positive cells remained in the INL of the eye that sustained section of the optic nerve. Perhaps the most remarkable observation was that the terminal processes of these cone bipolar cells were clearly segregated into two distinct strata, corresponding to the On and Off sublaminae present in the normal retina. It should be emphasized that retinal ganglion cells were depleted by optic nerve section ~5-6 d before bipolar cells innervate the IPL. This indicates that the segregation of On and Off cone bipolar cells into two segregated On and Off pathways is not dependent on retinal ganglion cells, the major target of these interneurons.
What might regulate the segregated On and Off cone bipolar cell axons? One possibility is that the formation of two distinct strata in the IPL by the terminal arbors of these neurons reflects an intrinsic program. Although this cannot be ruled out, we think it unlikely given the extensive literature on the role of cell-cell interactions in the formation of specific innervation patterns (Tessier-Lavigne and Goodman, 1996
Functional implications
The pattern of bipolar cell ingrowth observed here is in line with the model proposed for explaining how bipolar cell afferent activity could regulate the stratification of retinal ganglion cell dendrites (Bodnarenko et al., 1995
FOOTNOTES Received Aug. 24, 1999; revised Oct. 6, 1999; accepted Oct. 14, 1999.
This work was supported by National Science Foundation Grant IBN12593 and National Institutes of Health Grant EYO3391. We thank Dr. Alexander M. Dizhoor for his generosity in supplying us with the anti-recoverin antibody and Dr. Lamberto Maffei for assistance in optic nerve sections.
Correspondence should be addressed to Leo M. Chalupa, Neurobiology, Physiology, and Behavior, University of California, Davis, CA 95616. E-mail: lmchalupa{at}ucdavis.edu.
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