Ectopic Photoreceptors and Cone Bipolar Cells in the Developing and Mature Retina

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The Journal of Neuroscience, February 15, 2003, 23(4):1383

Ectopic Photoreceptors and Cone Bipolar Cells in the Developing and Mature Retina
Emine Günhan¹, Deborah van der List¹, and Leo M. Chalupa¹^,²
¹ Section of Neurobiology, Physiology, and Behavior, Division of Biological Sciences, and ² Department of Ophthalmology, School of Medicine, University of California, Davis, California 95616

  ABSTRACT

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

An antibody against recoverin, the calcium-binding protein, labels photoreceptors, cone bipolar cells, and a subpopulationof cells in the ganglion cell layer. In the present study, wesought to establish the origin and identity of the cells expressingrecoverin in the ganglion cell layer of the rat retina. By doublelabeling with rhodopsin, we demonstrate that early in developmentsome of the recoverin-positive cells in the ganglion cell layerare photoreceptors. During the first postnatal week, these rhodopsin-positivecells are eliminated from the ganglion cell layer, but such neuronsremain in the inner nuclear layer well into the first postnatalmonth. Another contingent of recoverin-positive cells, with morphologicalfeatures equivalent to those of bipolar cells, is present in thepostnatal retina, and ~50% of these neurons survive to maturity.The incidence of such cells in the ganglion cell layer was notaffected by early transection of the optic nerve, a manipulationthat causes rapid loss of retinal ganglion cells. These recoverin-positivecells were not double-labeled by cell-specific markers expressedby photoreceptors, rod bipolar cells, or horizontal and amacrinecells. Based on their staining with recoverin and salient morphologicalfeatures, these ectopic profiles in the ganglion cell layer aremost likely cone bipolar cells. Collectively, the results provideevidence for photoreceptors in the ganglion cell and inner nuclearlayers of the developing retina, and a more permanent subpopulationof cone bipolar cells displaced to the ganglion celllayer.

Key words: ectopic cells; recoverin; bipolar cells; photoreceptors; retina; development

  Introduction

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

A striking feature of the vertebrate retina is its distinct laminar organization. Cells in the three cellular layers havebeen extensively characterized on the basis of their morphological,functional, and molecular properties, and sound estimates forthe total number of cell types present in the mammalian retinahave been provided recently (Masland and Raviola, 2000). To attaintheir layer-specific distribution patterns, newborn neurons mustmigrate from the proliferative zone of the inner retina to theirappropriate laminar destination. Unlike the temporal sequencethat has been delineated in the other layered structures of thebrain, the pattern of cell generation in the retina does not followa spatially dependent order. Thus, ganglion cells and photoreceptorsare generated during similar developmental periods (Morest, 1970;Barnstable et al., 1988; Treisman et al., 1988; Watanabe and Raff,1990; Reese and Colello, 1992). Moreover, compared with otherbrain structures, our understanding of the mechanisms underlyingcell migration in the developing retina is still rudimentary,but Müller cells as well as cell-to-cell interactions have beenimplicated in this process (Altshuler and Cepko, 1992; Reh, 1992;Wong and Godinho, 2003).

A cell marker that has proven particularly effective for studying the developing retina is recoverin, a 23 kDa calcium-bindingprotein originally purified from bovine rod outer segments (Dizhooret al., 1991; Lambrecht and Koch, 1992). The anti-recoverin antibodylabels cone and rod photoreceptors (Dizhoor et al., 1991; Korfet al., 1992; Milam et al., 1993; Wiechmann and Hammarback, 1993;Grunert et al., 1994; Johnson et al., 1999) as well as ON andOFF cone bipolar cells (Milam et al., 1993; Miller et al., 1999;Günhan-Agar et al., 2000; Günhan et al., 2002). Somas and processesare recognized by the anti-recoverin antibody at a relativelyearly stage of development, even before neurons have begun theirmigration. This has made it feasible to use recoverin as a markerto assess the development of photoreceptors (Johnson et al., 1999)as well as ON and OFF cone bipolar cells (Miller et al., 1999;Günhan-Agar et al., 2000).

Recoverin or its mRNA also has been localized in a small number of cells in the ganglion cell layer of several different species(Stepanik et al., 1993; Wiechmann and Hammarback, 1993; McGinniset al., 1999; Günhan-Agar et al., 2000), including the humanretina (Yan and Wiechmann, 1997). Neither the origin nor the identityof these recoverin-positive cells has been established, althoughit has been commonly assumed that these represent a subclass ofganglion cells and displaced amacrinecells.

In the present study, we provide evidence that the recoverin-positive cells in the ganglion cell layer are composed of twodistinct populations: photoreceptors and cone bipolar cells. Thephotoreceptors survive in the ganglion cell layer for only a shorttime, being eliminated by the first postnatal week. In contrast,a significant number of cone bipolar cells remain in the ganglioncell layer into maturity, although the majority of these cellsare also lost during postnatal development. Thus, in additionto ganglion cells and displaced amacrine cells, the ganglion celllayer of the mature retina contains displaced bipolarcells.

  Materials and Methods

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Animals and tissue preparation. Timed-pregnant and adult Long-Evans rats were obtained from Charles River Laboratories (NewYork, NY). The animals were housed and bred in accordance withUniversity of California guidelines for the use of laboratoryanimals. The animals were killed by a lethal injection of sodiumpentobarbital (0.6 mg/kg body weight, i.p.) at time points rangingfrom the day of birth [postnatal day 0 (P0)] to adult. The eyecupswere removed from the embryos, hemisected, and fixed in 4% paraformaldehyde(PFA) for 1 hr. Postnatal animals were perfused transcardiallywith PBS followed by 4% PFA. The eyecups were removed, hemisected,and postfixed with 4% PFA for 30 min. The tissue was then immersedin 25% sucrose solution and embedded in tissue freezing medium(Tissue Tek, Torrance, CA), and 10-12 µm sections were made usinga Leica (Bannockburn, IL) 1900 cryostat. The sections were mountedon poly-L-lysine-coated slides (Sigma, St Louis, MO) and keptfrozen.

For the whole-mount preparations, a suture was placed in the connective tissue to mark the temporal edge before enucleation.After the retina was removed, a radial cut was made at the siteof the suture and additional radial cuts were made to facilitateflattening.

To deplete retinal ganglion cells, a unilateral transection of the optic nerve was performed at P0 or P1. For this purpose,the pups were anesthetized by hypothermia and the frontal cortexand optic nerve were aspirated under visualcontrol.

Antibodies. Photoreceptors, two types of cone bipolar cells, and some cells in the ganglion cell layer were labeled with arabbit polyclonal antibody to recoverin (1:500-1:2500; a giftfrom Dr. Alexander Dizhoor Wayne State University, Detroit, MI).Rod photoreceptors were also labeled with a monoclonal antibodyto rhodopsin (10 µg/ml; Chemicon, Temecula, CA). The immunogenwas prepared using adult rat retina; this antibody reacts witha protein of 39 kDa identified as rhodopsin. Horizontal cellswere stained with a monoclonal antibody to calbindin (1:1000;Sigma). A subpopulation of cone bipolar cells was identified withanti-G_o antibody (10 µg/ml; Chemicon). Rod bipolar cells werestained with a monoclonal protein kinase C (PKC) antibody (1:10;Amersham Biosciences, Piscataway, NJ). AII amacrine cells wereidentified with a monoclonal antibody to parvalbumin (1:2000;Sigma). Dopaminergic amacrine cells were labeled using a polyclonalantibody to tyrosine hydroxylase (TH) (1:500, Chemicon), and cholinergiccells were labeled with antivesicular acetylcholine transporter(VAChT; 1:2500) or anti-choline acetyl transferase (ChAT; 1:50)antibodies (Chemicon). A monoclonal vimentin antibody was usedto identify Müller cells (1:500; Dako, Carpinteria,CA).

Immunohistochemistry. Retinal sections were incubated in blocking solution containing 10% normal serum, 2% bovine serum albumin,and 0.3% Triton X-100 in PBS for 1 hr at room temperature (RT).Primary antibodies were diluted in blocking solution, and thesections were incubated in the primary antibody solution overnightat 4°C. Primary antibody incubation was omitted for control slides.After several washes with PBS, the sections were incubated withfluorescent secondary antibodies (1:500; Jackson ImmunoResearch,West Grove, PA; 3 µg/ml, Molecular Probes, Eugene, OR) dilutedin PBS for 1 hr at RT, washed three times with PBS, and coverslippedwith Vectashield mounting media (Vector Laboratories, Burlingame,CA). Other sections were incubated with biotinylated secondaryantibodies (1:500; Jackson ImmunoResearch) for 1 hr at RT. Afterseveral washes with PBS, tissues were incubated for 1 hr in theVectastain Elite ABC Kit (Vector Laboratories), and peroxidasewas visualized with a 0.5 mg/ml diaminobenzidine (DAB) solutionin the presence of H₂O₂. After final washes, the slides were coverslippedwith Vectamount (Vector Laboratories). For double-labeling, sectionswere incubated in a mixture of two primary antibodies, rinsedwith PBS, and incubated in a mixture of two secondary-antibody-conjugatedfluorochromes that have different excitationranges.

For retinal whole-mount processing, the dissected retina was washed in PBS, placed in 25% sucrose solution, and alternatelyfrozen and thawed three times. The tissue was then placed on aglass slide, ganglion cell layer down, treated for endogenousperoxidase with 0.6% H₂O₂ for 30 min, and then washed thoroughlyin PBS. Anti-recoverin antibody was diluted 1:500 in blockingsolution. The tissue was incubated in the primary antibody at4°C for 5 d in younger animals and for up to 7 d in adults. Theretina was then washed in PBS, placed in biotinylated goat anti-rabbitsecondary antibody diluted 1:300, and incubated for 3 d at 4°C.After washing in PBS, the retina was incubated with ABC solution(Vector Laboratories) overnight at 4°C and then treated with a0.5 mg/ml DAB solution in the presence of H₂O₂ for 5-10 min. Theretina was then coverslipped with Vectashield mounting media (VectorLaboratories).

Imaging. Confocal images for immunofluorescence were acquired by an Olympus Optical (Tokyo, Japan) upright confocal microscopeequipped with an argon-krypton laser in the epifluorescence-confocalmode. A stack of images along the z-axis (0.2-2 µm steps) wascollected for each slide. Bright-field photomicrographs were takenby a digital camera (Optronics International, Chelmsford, MA)attached to a Nikon (Tokyo, Japan) eclipse E600 microscope andviewed by differential interference contrastoptics.

Statistical analysis. Recoverin-positive cells in the ganglion cell layer were counted using two different methods. In twopostnatal retinas (P6 and P8), immunopositive cells were countedin retinal whole mounts using methods described previously (Whiteand Chalupa, 1991; Hutsler and Chalupa, 1995). Briefly, a drawingtube mounted to an upright Nikon microscope was used to createa drawing of the flattened retina, and every immunopositive cellwas counted and its locus marked by a dot on the retinal whole-mountdrawing. The number of dots in each retina was then counted toobtain an estimate of the total number of recoverin-positive cells.It was problematic to obtain complete labeling of cells in whole-mountedadult retinas. To circumvent this problem, counts were made insections of the adult retina using the optical volume fractionatormethod (Gundersen et al., 1988a,b; Bolender et al., 1993). Briefly,12 µm vertical serial sections were obtained from whole hemisectedeyes, and every 11th and 12th section was taken and immunostainedwith recoverin antibody using peroxidase staining for bright-fieldmicroscopy. All of the recoverin-positive cells were counted inthe 11th section, and the cells that overlapped in the 11th and12th sections were subtracted from the total number to avoid double-counting.After these counts were completed, the average number of cellsin a single section was calculated and multiplied by the totalnumber of sections to obtain the "unbiased" total number of recoverin-positivecells.

Soma size was measured in P4, P6, P8, P10, and adult whole-mount retinas. Images were captured using a color digital camera(Optronics International) attached to an upright, binocular microscope(Nikon Eclipse E600) using Adobe Photoshop (Adobe Systems, SanJose, CA), and transferred to a Dell computer (Workstation PWS530;Dell Computer Company, Round Rock, TX), where Neurolucida 2000(MicroBrightField, Inc., Colchester, VT) was used to trace thecontours of each soma. NeuroExplorer (MicroBrightField, Inc.)was used to analyze the data, which were then transferred to Microsoft(Seattle, WA) Excel for additionalanalysis.

  Results

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

Recoverin labeling in the mature rat retina

In the mature retina, recoverin labels two major classes of cells: photoreceptors in the outer nuclear layer as well as ONand OFF cone bipolar cells in the inner nuclear layer (Milam etal., 1993; Euler and Wässle, 1995; Günhan-Agar et al., 2000).Recoverin-positive cells are also present in the ganglion celllayer [Günhan-Agar et al. (2000), their Figs. 2 and 3] (see Fig.5 and vimentin-recoverin labeling in Fig. 6 of the present study).In the present study counts, of these cells in the ganglion celllayer of two adult rats provided population estimates of 960 suchneurons in one retina and 823 in another. Although recoverin-positiveneurons have been noted previously in several species (Stepaniket al., 1993; Wiechmann and Hammarback, 1993; Yan and Wiechmann,1997; McGinnis et al., 1999; Günhan-Agar et al., 2000), theirorigin and cell class have not been established. In an effortto resolve this issue, we examined recoverin-labeled cells thatmigrated toward and into the presumptive ganglion cell layer inthe developing rat retina. We also sought to establish the identityof these recoverin-positive cells by immunocytochemical markersthat label selectively different classes of retinalneurons.

Recoverin labeling in the developing rat retina

Recoverin is expressed by developing cells in the ventricular zone of the rat retina as early as embryonic day 16 (E16) (datanot shown). Recoverin-labeled cells can be observed migratingtoward the inner part of the retina at E18, as shown in Figure1. On E20, ~2 d before birth, recoverin-positive cells are alreadypresent in the presumptive ganglion cell layer. By P4, such neuronsbecome more numerous, and by P10, the recoverin-labeled cellsin the ganglion cell layer appear to be well differentiated. Inmany cases, dendritic and/or axonal processes could be seen tooriginate from particular somas, indicated by arrows in Figure1.

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Figure 1. Confocal images of recoverin expression patterns in the rat retina during prenatal and postnatal development. Ages are indicated in each photomicrograph. Gestation in the rat is 21 d. Recoverin is expressed by developing cells in the neuroblast layer of the rat retina as early as E16. The number of cells that express recoverin increases markedly during the last days of gestation and the first week of postnatal life. Note that the migration of these cells into the ganglion cell layer (GCL, arrows) precedes normal migration into the inner nuclear layer (INL). In this and all of the other figures, the ganglion cell layer is oriented down. NBL, Neuroblast layer; ONL, outer nuclear layer; OPL, outer plexiform layer; IPL, inner plexiform layer. Scale bars, 20 µm.

To assess the overall distribution of the recoverin-positive cells in the ganglion cell layer, we attempted to label the entirepopulation of these neurons in P6 and P8 retinal whole mounts.Figure 2 (top) shows the location of every recoverin-positivecell in the ganglion cell layer in these two retinas. Note thatsuch cells are scattered throughout all retinal quadrants, andthat their density appears relatively uniform. A detailed countrevealed that there were 2038 cells at P8, whereas there were2222 in the P6 retina. This is more than twice the number estimatedto be present in the mature retina.

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Figure 2. Top, Distribution of recoverin-positive cells in the ganglion cell layer of P6 and P8 whole-mounted retinas. Shaded regions had incomplete staining. Scale bar, 1 mm. Note that the P8 retina is sized to be comparable with the P6 retina. N, Nasal; T, temporal. Bottom, Selected low- and high-power images from P6 (top row) and P8 (bottom row) whole-mounted retinas. Scale bars, 50 µm in low-power images and 20 µm in high-power images.

The extensive dendritic processes of the recoverin-positive neurons could be observed in their entirety in these retinal wholemounts, as shown in the photomicrographs depicted in Figure 2,bottom. In older retinas, recoverin-positive processes were lessextensive and the soma sizes were significantly smaller. At P4,P6, and P8, the average soma sizes were 58.20 ± 14.17, 58.24 ±10.94, and 59.27 ± 12.6 µm² (means ± SD), respectively. By P10, the soma sizes were smaller,48.67 ± 8.74 µm², comparable with the adult size of 46.08 ± 8.22 µm². The age-related differences were found to be statistically significant(p < 0.01; one-way ANOVA). Additional analysis showed that therewere no differences among ages P4, P6, and P8, nor was there adifference between P10 and adult retinas; however, there was astatistically significant difference between the P4-P6-P8 groupand the P10 to adult group (p < 0.01; Tukeytest).

Rhodopsin labeling of recoverin-positive cells

In the rat, photoreceptors are generated from approximately E16 to P5, with the majority of the rods developing after birth(Kuwabara and Weidman, 1974; Carter-Dawson and LaVail, 1979; Hindsand Hinds, 1979; Barnstable, 1981; Young, 1985). Rhodopsin expression,a visual pigment specific to differentiated rods, does not occuruntil P1-P2 (Treisman et al., 1988; Watanabe and Raff, 1990).Double-labeling developing retinas with antibodies against recoverinand rhodopsin revealed that some of the recoverin-positive cellsoutside the photoreceptor layer were rhodopsin-positive. Figure3 depicts such double-labeled neurons at P0, P1, P3, and P7. Atthe youngest ages (P0-P3), these cells were situated in the presumptiveganglion cell layer (i.e., in the innermost retinal layer). Severaldays later, virtually all of these neurons were eliminated fromthe ganglion cell layer, but a significant number of cells couldnow be visualized in the inner nuclear layer (Fig. 3, P7 panels).Opsin-like immunoreactive cells have been noted previously inthe inner nuclear layer of the developing rat retina (Barnstable,1982; Araki et al., 1988), but not in the ganglion cell layer.

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Figure 3. Confocal images of rhodopsin-labeled cells (left) and recoverin-labeled cells (middle) in the rat retina during postnatal development (P0-P7). As indicated by arrows in the right panels, some recoverin-positive cells are rods that have migrated beyond the photoreceptor layer. GCL, Ganglion cell layer; NBL, neuroblast layer; OPL, outer plexiform layer; IPL, inner plexiform layer; INL, inner nuclear layer. Scale bars, 20 µm.

The distribution of rhodopsin-positive cells within the inner nuclear layer at P20 is shown in Figure 4, top. In the matureretina, all rhodopsin labeling is confined to the photoreceptorlayer (Fig. 4, bottom). Because rhodopsin-positive cells are eliminatedfrom the ganglion cell layer a few days after birth, this meansthat such cells were not included in the distributions depictedin Figure 2.

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Figure 4. Bright-field images of rhodopsin labeling in the P20 and adult retinas. Note that in the adult retina there are no rhodopsin-positive cells in the inner retina. Inset, High-power image of P20. Scale bars, 10 µm in low-power images and 5 µm in high-power images.

Identity of recoverin-positive cells in ganglion cell layer of adult retina

To determine whether the cells expressing recoverin in the ganglion cell layer of the mature retina might be ganglion cells,the optic nerve was transected at either P0 or P1. This manipulationcauses a complete and rapid loss of retinal ganglion cells (Millerand Oberdorfer, 1981; Osborne and Perry, 1985; Beazley et al.,1987; Günhan-Agar et al., 2000). Examples of recoverin-positiveprofiles in the ganglion cell layer of the normal adult retinaand in an adult retina that sustained optic nerve transectionat P0 are shown in Figure 5. The morphological features and theincidence of such cells in normal retinas and those with earlyoptic nerve sections were virtually identical. These results indicatethat the recoverin-positive cells observed in the ganglion celllayer of the adult retina are not ganglion cells.

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Figure 5. Confocal images of recoverin-expressing cells (arrows) in the ganglion cell layer of adult retinas (Normal) and in retinas of comparable age in which all ganglion cells were depleted by an optic nerve transection (ONT) at P0 or P1. The presence of such recoverin-positive neurons after early ONT suggests that these were not ganglion cells with centrally projecting axons. In some cases, the axon of a recoverin-expressing cell was found to project upward toward the inner plexiform layer, as shown in the left middle panel. Scale bar, 20 µm.

In retinal cross sections, the recoverin-positive cells in the ganglion cell layer appeared to have morphological featuresidentical to those of bipolar cells. Note in the cells demarcatedby arrows in Figure 5 the dense dendritic arbors of the recoverin-positivecells situated in the ganglion cell layer extending into the innerplexiform layer and in some cases the single axon stemming fromthe opposite pole of the soma. Moreover, axonal processes of somecells could be seen to make a sharp turn upward to innervate theinner plexiform layer (Figs. 5, 6, vimentin-recoverin panel).

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Figure 6. Confocal images of Thy1.1-, vimentin-, parvalbumin-, and PKC-labeled cells (left) and recoverin-labeled cells (middle) in the rat retina. Overlapping images are shown at the left. Note that none of the recoverin-positive cells in the ganglion cell layer are double-labeled. Note also that the axonal process of recoverin-positive cells in the ganglion cell layer is directed toward the inner plexiform layer in the vimentin-recoverin panel. Scale bar, 20 µm.

In an additional effort to establish the identity of these neurons, we also double-labeled retinas with recoverin and a varietyof markers specific for different retinal cell types, includingChAT, VAChT, Thy1.1, vimentin, TH, calbindin, parvalbumin, G_o,and PKC. Figure 6 depicts the resulting labeling patterns forfour of these markers in conjunction with recoverin labeling.As can be seen, there was no evidence of cells double-labeledwith recoverin and Thy1.1, vimentin, parvalbumin, or PKC. Thiswas also the case for the five other cell-specific markers weused (data notshown).

  Discussion

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

In the present study, we provide evidence for the presence of two distinct subpopulations of ectopic neurons in the developingand mature rat retina that express the calcium-binding proteinrecoverin. In the adult retina, the anti-recoverin antibody labelsphotoreceptors and ON and OFF cone bipolar cells, as well as asmaller number of neurons in the ganglion cell layer. Here weshow that these atypical cells are photoreceptors and cone bipolarcells. By labeling retinas from E16 through the early postnatalperiod, separated at 1 d intervals, we were able to visualizerecoverin-positive profiles migrating from the outer to the innerretina. Such cells were observed to exit the germinative layerat E18, and by E20 they were found in the presumptive ganglioncell layer. Thus, most likely, the presence of these neurons outsidetheir normal retinal layers reflects migration errors during earlydevelopment.

To identify ectopic photoreceptors, we relied on double-labeling with antibodies against recoverin and rhodopsin. Recoverin/rhodopsin-positiveprofiles were apparent in the presumptive ganglion cell layeras early as P0, but 1 week after birth they were present onlyin the inner nuclear layer, and at maturity none were found outsidethe photoreceptor layer. A possible explanation for this sequenceof events is that this contingent of photoreceptors fails to recognizea signal to stop migrating when these cells arrive at the photoreceptorlayer. The early elimination of these photoreceptors from theganglion cell layer, and their later demise from the inner nuclearlayer probably reflects a failure of these cells to form functionalsynapses in the inappropriate retinallayers.

The other population of recoverin-positive cells in the ganglion cell layer survives to maturity. Several lines of evidenceindicate that these are cone bipolar cells. First, these neuronsare recoverin-positive, as is the case with ON and OFF cone bipolarcells. Second, their salient morphological features, consistingof a relatively small cell body with dendritic and axonal processesemanating from opposite poles of the soma, are identical to thoseof retinal bipolar cells. Third, these cells survived early transectionof the optic nerve, a manipulation that induces a rapid loss ofdeveloping ganglion cells but does not have an impact on the survivalof recoverin-expressing cone bipolar cells (Günhan-Agar et al.,2000). Fourth, these recoverin-positive cells were not double-labeledwith any of the 10 cell-specific markers we used, including Thy1.1for ganglion cells (Beale and Osborne, 1982; Barnstable and Drager,1984; Barres et al., 1988), rhodopsin for photoreceptors (Treismanet al., 1988; Watanabe and Raff, 1990), PKC for rod bipolar cells(Greferath et al., 1990), calbindin for horizontal cells (Pochetet al., 1991; Mitchell et al., 1995), vimentin for Müller cells(Okada et al., 1990), G_o for ON-cone bipolar cells (Vardi, 1998),parvalbumin for AII amacrine cells (Endo et al., 1986; Wässleet al., 1993), TH for dopaminergic amacrine cells (Oyster et al.,1985; Martin-Martinelli et al., 1989), and ChAT (Eckenstein andThoenen, 1982; Pourcho and Osman, 1986; Brandon, 1987; Wässleet al., 1987; Chun et al., 1988) and VAChT (Koulen, 1997) forcholinergic amacrinecells.

At ~1 week after birth, the number of recoverin-positive cells in the ganglion cell layer was found to be >2000. In the matureretina, this number drops by >50%, to <1000. The long-term survivalof such a sizable contingent of cone bipolar cells in the ganglioncell layer is intriguing, because it is generally assumed thatectopic cells must form functional connections to survive (Rakic,1975, 1988).

What could be the functional significance of the surviving ectopic bipolar cells in the mature retina? One possibility isthat they have formed synaptic connections appropriate for conebipolar cells. This seems unlikely when one considers the inputsto these neurons. We never observed the dendrites of the recoverin-positivecells to extend into the outer plexiform layer, nor did we noteexuberant photoreceptor processes projecting to the inner plexiformlayer, as has been documented in the developing ferret retina(Johnson et al., 1999). With respect to the axonal connectionsof the ectopic bipolar cells, in at least some cases, these couldhave made appropriate contacts with the dendrites of retinal ganglioncells. In cases in which ostensibly the full extent of the axonalprocess could be visualized, it appeared that the axon was directedinto the inner plexiform layer, in which contacts with the dendritesof retinal ganglion cells could have been established. Whethersuch functional contacts play a role in the processing of visualinformation remains to be established. Given the sizable contingentof displaced bipolar cells identified in the present study andthe presence of recoverin-positive cells in the human retina,this issue is certainly worthpursuing.

  FOOTNOTES

Received Aug. 26, 2002; revised Oct. 31, 2002; accepted Nov. 22, 2002.

This work was supported by National Eye Institute (NEI) Grant EY0339, an NEI Core Grant, and the Foundation to Prevent Blindness.We thank Dr. Alexander Dizhoor (Wayne State University, Detroit,MI) for the generous gift of the recoverin antibody and Dr. HandanCamdeviren (Mersin University, Mersin, Turkey) for statisticalconsultation.

Correspondence should be addressed to Dr. Leo M. Chalupa, Section of Neurobiology, Physiology, and Behavior, 1 Shields Avenue,University of California, Davis, CA 95616. E-mail: lmchalupa{at}ucdavis.edu.

E. Günhan's present address: Mersin University, School of Medicine, Yenisehir Campus, Yenisehir 33169, Mersin,Turkey.

  References

TOP
ABSTRACT
Introduction
Materials and Methods
Results
Discussion
REFERENCES

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