Abstract
The divergence of retinal ganglion cell (RGC) axons into ipsilateral and contralateral projections at the optic chiasm and the subsequent segregation of retinal inputs into eye-specific domains in their target, the dorsal lateral geniculate nucleus (dLGN), are crucial for binocular vision. In albinism, affected individuals exhibit a lack or reduction of pigmentation in the eye and skin, a concomitant reduced ipsilateral projection, and diverse visual defects. Here we investigate how such altered decussation affects eye-specific retinogeniculate targeting in albino mice using the C57BL/6 Tyr c-2J/c-2J strain, in which tyrosinase, necessary for melanogenesis, is mutated. In albino mice, fewer RGCs from the ventrotemporal (VT) retina project ipsilaterally, reflected in a decrease in cells expressing ipsilateral markers. In addition, a population of RGCs from the VT retina projects contralaterally and, within the dLGN, their axons cluster into a patch separated from the contralateral termination area. Furthermore, eye-specific segregation is not complete in the albino dLGN and, upon perturbing postnatal retinal activity with epibatidine, the ipsilateral projection fragments and the aberrant contralateral patch disappears. These results suggest that the defects in afferent targeting and activity-dependent refinement in the albino dLGN arise from RGC misspecification together with potential perturbations of early activity patterns in the albino retina.
Introduction
The partial decussation of retinal ganglion cell (RGC) axons at the optic chiasm midline ensures that targets on each side of the brain receive inputs from both eyes. In their primary target, the dorsal lateral geniculate nucleus (dLGN), RGC afferents from each eye segregate into distinct territories. This precise organization of eye-specific inputs is crucial for binocular vision, and during development is dependent on both molecular factors and neural activity (Huberman et al., 2008).
Molecular determinants of chiasmatic decussation have been identified (Petros et al., 2008). The transcription factor Zic2 and the guidance receptor EphB1 expressed in RGCs from ventrotemporal (VT) retina direct the ipsilateral projection (Herrera et al., 2003; Williams et al., 2003). Contralateral markers such as the transcription factor Islet2 (Pak et al., 2004) and the adhesion molecule NrCAM (Williams et al., 2006) are expressed in a pattern complementary to Zic2 and EphB1 and are important for late-born VT RGCs to cross the midline.
Previously, we addressed how impaired decussation affects retinogeniculate targeting: in EphB1−/− mice, fewer RGCs project ipsilaterally but innervate the appropriate targeting zone (Rebsam et al., 2009). We next turned to analyzing eye-specific targeting in the albino mouse, another model with altered decussation. Albinism is a hypopigmentation disorder due to lack of melanin in the eye only (ocular albinism), or in the eyes, skin, and hair (oculocutaneous albinism) (Oetting, 1999). A universal phenotype of albinism is a decreased ipsilateral projection resulting in perturbed binocular vision (Creel et al., 1990; Apkarian, 1996). We used Tyr c-2J/c-2J mice, in which tyrosinase, crucial for melanin synthesis, is mutated (Le Fur et al., 1996). All albino mouse strains have a reduced ipsilateral projection to the dLGN (Guillery et al., 1973; LaVail et al., 1978; Dräger and Olsen, 1980; Rice et al., 1995), but no other dLGN targeting defects have been described (Guillery et al., 1973; Cronin et al., 2003). Moreover, in Tyr c-2J/c-2J mice, fewer RGCs express Zic2 in the VT retina (Herrera et al., 2003), mirroring the reduced ipsilateral projection.
Here, we show that the reduced ipsilateral projection in albino mice is not characterized by a simple misrouting of retinal axons to the contralateral dLGN with retention of their proper targeting pattern, as in EphB1−/− mice (Rebsam et al., 2009). Instead, some VT RGCs from the contralateral eye terminate near the target zone of VT RGCs that normally project contralaterally in pigmented mice, but as a cluster separated from the principle contralateral projection. The reduction of ipsilateral fibers in the albino correlates with fewer RGCs expressing Zic2 and EphB1, but not with an increase in RGCs expressing contralateral markers. Moreover, as in EphB1 mutants, eye-specific segregation in albino mice is impaired under normal conditions, and the formation of the aberrant patch of RGC axons from VT retina is dependent on normal retinal activity. Finally, perturbation of retinal activity with epibatidine in albino animals produces changes nearly opposite to those seen in pigmented animals, suggesting possible abnormalities in early patterns of neural activity in the albino retina.
Materials and Methods
Animals.
Wild-type C57BL/6J mice and albino mice lacking tyrosinase (C57BL/6J Tyr c-2J/c-2J from Jackson Laboratory) were maintained in a timed-pregnancy breeding colony at Columbia University. Pigmented and albino mice were generated from crosses between Tyr+/Tyrc-2J and Tyrc-2J/Tyrc-2J mice. We use the terms pigmented and albino to refer to animals of the genotypes Tyr+/Tyr+ or Tyr+/Tyrc-2J and Tyrc-2J/Tyrc-2J, respectively (LaVail et al., 1978). E0 was defined as midnight before a plug was found and P0 is the day of birth, and both sexes were studied. All animal procedures followed the regulatory guidelines of the Columbia University Institutional Animal Care and Use Committee.
Anterograde labeling of retinogeniculate projections.
P13 and P29 mice were anesthetized intraperitoneally with ketamine–xylazine (100 and 10 mg/kg, respectively, in 0.9% saline). For whole-eye injection, the eye was extruded by using two fingers and 2–4 μl of 0.2% cholera-toxin subunit B (CTB) conjugated to AlexaFluor 594, 488 (Invitrogen) diluted in 1% DMSO was injected into the eye intravitreally with a glass micropipette. To make focal injections, 300–400 nl of 4% liquid DiI in 10% sucrose (the liquid DiI solution consists of 10% DiI in dimethylformamide) or CTB-AlexaFluor 594 (0.1% in 0.5% DMSO, 10% sucrose solution) was injected beneath the scleral margin into the VT retina through a glass micropipette linked to a Picospritzer II (General Valve Corporation). The ventrotemporal position was determined using the eyelid junction and head position. After 2 d, mice were anesthetized and perfused transcardially with 4% paraformaldehyde (PFA) in 0.1 m phosphate buffer before dissection of brain and retinas. Brains were postfixed overnight, embedded in 3% agarose, and sectioned coronally with a vibratome (100 μm). Sections were mounted in Gelmount (Biomeda).
Epibatidine injection.
Postnatal mice were anesthetized on ice. The skin was cut open at the eyelid junction to access the eye. Every 24 h from P3 to P6, 0.5–1 μl of 1 mm epibatidine in 0.9% saline was injected intravitreally into both eyes through the same injection site. Pups were returned to their mother after recovery from anesthesia.
In situ hybridization and immunostaining.
Heads from E15.5 and E17.5 embryos were fixed overnight or 2 h for Islet2 immunostaining in 4% PFA, cryoprotected in 10% sucrose in PBS overnight, and subsequently frozen in TissueTek OCT compound using cold isopentane (−55°C). Coronal sections (20 μm) were cut with a cryostat, mounted on Superfrost slides, and processed for in situ hybridization as described by Schaeren-Wiemers and Gerfin-Moser (1993). Probes for EphB1 (Williams et al., 2003) and NrCAM (Williams et al., 2006) were synthesized using Digoxygenin RNA labeling mix (Roche). The sections were then processed for immunohistochemistry. Ten percent normal goat serum (NGS) in 0.2% Triton was used as blocking solution. A rabbit anti-Zic2 antibody (1/10,000; a gift from Dr. Steve Brown, University of Vermont, Burlington, VT) and a rabbit anti-Islet2 antibody (1/1000; a gift from Dr. Thomas Jessell, Columbia University, New York, NY) were used as primary antibodies, and a goat anti-rabbit Cy3 (1/500; Jackson Immunoresearch) was used as a secondary antibody in 1% NGS, 0.2% Triton in PBS. Sections were mounted in Gelmount.
Microscopy.
Imaging of embryonic retinas and brain sections was done with Axiovision software through Axiophot camera and a Zeiss Axioplan 2 microscope.
Analysis of the number, distribution, and segregation of ipsilateral fibers.
Quantification of eye-specific terminations in Figures 1 and 4 were performed using MetaMorph software on 10× images and statistical analysis using Student's t test were performed as previously described (Rebsam et al., 2009).
Results
The number, distribution, and segregation of ipsilateral fibers are altered in the albino mouse dLGN
Using whole-eye labeling with fluorescent CTB to trace retinogeniculate axons (Fig. 1e) and computer-assisted quantification, we found that at P31, the ipsilateral RGC projection in albino mice (n = 6) targets the dLGN core as in wild-type (pigmented) dLGN (Fig. 1a,c) but is reduced, as expected, by 48% compared with pigmented mice (n = 11) (pigmented, 17.2%, and albino, 9.7% of dLGN territory is occupied by ipsilateral terminal arbors; p = 9.3 × 10−5). The reduced ipsilateral projection in the albino dLGN is confined to a smaller zone along the ML axis and has a more elongated shape (Fig. 1c) compared with pigmented mice (Fig. 1a). This pattern is supported by quantification of RGC terminations, indicating a reduced extension of the ipsilateral projection along the ML axis but not the DV axis (Fig. 1k). Moreover, eye-specific segregation in the albino dLGN is incomplete, reflected in a significantly greater overlap between ipsilateral and contralateral terminal arbors at P31 compared with pigmented mice (Fig. 1l).
RGCs from VT retina in albinos project within the contralateral input-recipient zone as a distinct patch
The most striking feature of the albino retinogeniculate projection is a patch of axon terminations from the contralateral eye that forms within the contralateral RGC-recipient zone but is separated from the normal contralateral projections from non-VT and VT retina (Fig. 1d). The patch of axons is situated in the caudal dLGN, adjacent to the optic tract and ventrolateral to the afferent zone of VT RGCs that are late-born and that project contralaterally in pigmented and albino mice (Fig. 1b,d). This phenotype is fully penetrant, as we observed this patch in every individual albino brain.
In pigmented mice, DiI injections made at P15 and restricted to the VT retina (Fig. 1j) labeled a projection to the core of the dLGN on the ipsilateral side (data not shown) and the dorsal tip of the dLGN on the contralateral side (Fig. 1f,f',h,h'), where the late-born contingent of VT RGCs terminates (Dräger, 1985; Pfeiffenberger et al., 2006). In albino mice, such VT injections revealed that the aberrant patch is composed of fibers from the contralateral VT retina (Fig. 1i,i',g,g'). This pattern of projection suggests that in the albino, VT RGC axons project to a site near the topographically correct terminal zone in the dLGN of contralateral VT RGC axons. However, because these RGCs form a cluster of terminals separated from the other contralateral projections, these RGCs may be differentially specified, expressing a combination of markers different from those in the normal contralaterally projecting VT and non-VT RGCs (Fig. 1j).
Changes in ipsilateral but not contralateral marker expression in the albino VT retina
We then assessed whether the expression pattern of markers of RGC specification and guidance fate are altered in the albino, especially in VT retina (Fig. 2). As previously described, the number of VT RGCs expressing the ipsilateral determinant Zic2 is reduced in albino mice (Fig. 2a2,b2) (Herrera et al., 2003). We found that the number of RGCs expressing the EphB1 receptor (Fig. 2a1,b1) is also reduced in the albino retina at E15.5, mirroring the reduction of Zic2-expressing cells (Fig. 2a,b). For contralateral markers, however, NrCAM expression at E15.5 (Fig. 2c,d) and E17.5 (Fig. 2e,f) and Islet2 expression at E17.5 (Fig. 2g,h) are similar in pigmented and albino mice. This result suggests that the reduction in the number of RGCs with an ipsilateral identity is not accompanied by an increase in RGCs expressing known contralateral markers.
Perturbation of retinal waves has an unusual effect on RGC fiber refinement in albino mice
Spontaneous waves of activity in the retina are important for eye-specific segregation (Huberman et al., 2008; Xu et al., 2011). As retinal waves rely on cholinergic transmission through the first postnatal week, ocular injections of the nicotinic acetylcholine receptor agonist epibatidine perturbs retinal waves through receptor desensitization (Feller et al., 1996), increasing firing in some RGCs and silencing others (Cang et al., 2005; Sun et al., 2008). We have previously shown that disrupting retinal activity during the first postnatal week has lasting effects on the distribution and segregation of ipsilateral terminals (Rebsam et al., 2009). After epibatidine treatment in wild-type mice (Fig. 3b), ipsilateral fibers are distributed over a larger territory along the DV and ML axis compared with saline-treated wild-type mice (Figs. 3a,b; 4b) and are less segregated from contralateral fibers (Figs. 3a',b'; 4c,d). However, the proportion of dLGN occupied by ipsilateral fibers is not significantly increased (Fig. 4a).
In albino mice treated with epibatidine (n = 7), ipsilateral projections fragment into distinct patches (often three) along the DV axis of the dLGN (Fig. 3d) and are distributed along a wider extent of the DV axis compared with saline-treated albino mice (n = 5; Figs. 3c,d; 4b). No significant differences were observed between saline- and epibatidine-treated albino mice in the percentage of the dLGN area occupied by ipsilateral fibers, in extent along the ML axis, nor in eye-specific segregation (Figs. 3c',d'; 4), even though segregation is incomplete in the albino under normal spontaneous activity compared with pigmented mice (Fig. 3a',c'). Importantly, binocular epibatidine treatment in albino mice prevents the formation of the aberrant patch formed by contralateral fibers (Fig. 3e,f). Thus, epibatidine treatment has an almost opposite effect on distribution and segregation of RGC afferents in albino mice compared with wild-type mice. Furthermore, these data indicate that retinal activity is required for the clustering of the aberrant contralateral fibers arising from VT RGCs in albino mice.
Discussion
We have examined how altered RGC decussation at the optic chiasm in albino mice affects targeting in the dLGN. In albino mice, fewer VT RGC axons project to the ipsilateral side and some contralaterally projecting VT RGCs form an aberrant patch that is separated from the normal contralateral and ipsilateral cohorts in an activity-dependent manner. In addition, in albino mice, retinal activity disruption by epibatidine induces the fragmentation of the ipsilateral projection into patches without further perturbing eye-specific segregation.
Albino and EphB1−/− mice have a reduced ipsilateral projection (Dräger and Olsen, 1980; Williams et al., 2003). In both mutants, a small cohort of VT RGCs projects contralaterally and forms a patch of terminations separated from the surrounding projections. However, whereas the aberrant patch in EphB1−/− mice is located adjacent to the normal ipsilateral projection, the aberrant patch in the albino terminates in a contralateral-recipient territory, adjacent to the zone where late-born contralateral RGCs from VT retina project. These results suggest that abnormal RGC specification may be responsible for the aberrant retinogeniculate projection pattern in the albino. Indeed, the albino retina contains fewer Zic2 (Herrera et al., 2003) and EphB1-positive RGCs, consistent with the regulation of EphB1 by Zic2 (García-Frigola et al., 2008; Lee et al., 2008). Because our previous results showed that albino VT RGCs display crossed RGC behaviors in vitro (Marcus et al., 1996), we expected to see an increase in crossed markers, but did not. Further, we could not determine whether the VT RGCS that form the patch are RGCs that are normally specified to project ipsilaterally and have changed fate or whether they are RGCs that were already fated to project contralaterally. In both cases, these RGCs might lack or aberrantly express a combination of transcription factors and guidance molecules differently from that in wild-type contralateral VT RGCs and thus project and terminate as a separate patch in the albino. The expression of transcription factors or surface molecules could in turn be regulated by activity (Itoh et al., 1995; Hanson and Landmesser, 2004), explaining why the patch disappears after blockade of correlated retinal activity.
VT RGCs in albino retina may have such an altered transcriptional profile due to defects in the pace of proliferation (Ilia and Jeffery, 1996; Rachel et al., 2002), supported by the finding that tyrosinase is required only during the generation of ipsilateral RGCs for the development of a normal projection (Cronin et al., 2003). If the aberrant population of VT RGCs are born too early or too late, they would be specified to express molecular determinants that would render the RGCs unrecognizable to the other VT axons and would consequently form their own termination zone. Understanding differences in the molecular code of the different populations of VT RGCs will be necessary to further dissect the molecular mechanisms of the targeting defect described in this study.
In albino mice, retinogeniculate axons incompletely segregate into eye-specific territories, even in normal activity conditions. Furthermore, epibatidine treatment induces fragmentation of the ipsilateral projection, a phenotype that is not observed in wild-type or EphB1−/− mice. The albino retina may exhibit altered physiological responses due to defects in proliferation and specification. This hypothesis is supported by an increased number of amacrine cells (which initiate the retinal waves during the first postnatal week) in albino rats (Mitrofanis and Stone, 1988). Future studies on neuronal activity in the albino retina should shed light on this intriguing phenotype.
The defects in RGC neurogenesis, molecular specification, axon guidance and targeting in the albino mouse could serve as reference points for rescue experiments and give insight into how melanin and the retinal pigment epithelium affect normal retinal development.
Footnotes
This work was supported by NIH Grants EY012736 and EY015290, the Gatsby Initiative in Brain Circuitry (C.A.M.), and the Fondation pour la Recherche Medicale and the Human Frontier Science Program (A.R.). We thank Takeshi Sakurai, Ray Guillery, Patricia Gaspar, Wes Grueber, and members of the Mason Lab for helpful discussions and critical review of the manuscript.
- Correspondence should be addressed to either Carol A. Mason, Department of Pathology and Cell Biology, College of Physicians and Surgeons, Columbia University, 630 W 168th Street, New York, NY 10032. cam4{at}columbia.edu or alexandra.rebsam{at}inserm.fr