Three-week-old female Dark Agouti (DA) rats and embryonic day (E)18 pregnant Wistar rats were obtained from Shimizu Laboratory Supplies (Kyoto, Japan). In all experimental procedures, the animals were treated according to the regulations in the ARVO Statement for the Use of Animals in Ophthalmic and Vision Research and the Guidelines for Animal Experiments of Kyoto University. All animal experiments were conducted with the approval of the Animal Research Committee, Graduate School of Medicine, Kyoto University. 

Rat iris and ciliary tissues were prepared from 3- to 4-week-old female DA rats. The procedure for iris cell culture has been described. ¹⁶ Briefly, after the iris with the cornea was separated from the other eye tissue at sufficient distance by careful incision, the iris tissue, treated with 1000 IU/mL dispase and 0.05% EDTA, was plated on a laminin-coated chamber slide. To prepare ciliary-derived cells, the neural retina was first peeled from the retinal pigmented epithelium (RPE) after removal of the cornea, iris tissue, and lens, not including neural retinal cells. Next, the pigmented epithelium of the ciliary margin (including the RPE) was separated by careful incision and treated with the Papain dissociation system (Worthington Biochemical Corp., Lakewood, NJ). Briefly, the pigmented epithelium was treated with Earle’s balanced salt solution (EBSS) containing papain and DNase I (DNase) for 40 minutes at 37°C and then centrifuged at 1000 rpm for 5 minutes and dissociated into small pieces by gentle trituration with a micropipette in EBSS containing DNase and albumin inhibitor. Then, the cell suspension was layered on top of EBSS containing albumin-inhibitor in a centrifuge tube and centrifuged at 800 rpm for 6 minutes. The supernatant was discarded, and the pelleted cells were resuspended in culture medium. The cells were dissociated into single cells by gentle trituration with a micropipette, and the pieces of undissociated tissues were removed. The dissociated ciliary-derived cells were cultured in 100-mm culture dishes containing serum-free culture medium at a cell density of 5 to 10 × 10⁴/mL. Dissociated ciliary-derived cells were cultured for 5 days to 2 weeks, to generate ciliary-derived sphere colonies. The iris tissue- and ciliary-derived cells were maintained at 37°C in Dulbecco’s modified Eagle’s medium/Ham’s F12 (DMEM/F12; Invitrogen-Gibco, Grand Island, NY) with B27 supplement (Invitrogen-Gibco) and 40 ng/mL basic fibroblast growth factor (bFGF; Genzyme/Techne, Minneapolis, MN). As with ciliary-derived cells, bFGF was added without medium change, or half the culture medium was changed every 2 days. The ciliary-derived cell cultures were passaged every 6 to 8 days. The medium of iris-derived cell culture was changed every 2 days. For cell differentiation, 1 day after gene induction the cells were cultured for 14 days in DMEM/F12/B27 with 1% fetal bovine serum (FBS) and 10 ng/mL bFGF. 

For preparation of brain-derived neural stem cells, tissue blocks of E18.5 Wistar rat ventral mesencephalon were resected, collected in cold phosphate-buffered saline (PBS), and dissociated into single cells by gentle trituration with a fire-polished Pasteur pipette, as described previously. ^{17 18} The cells were then cultured at 37°C in DMEM/F12 with N2 supplement (Invitrogen-Gibco) and 20 ng/mL bFGF. After 3 to 5 days of culture, the mesencephalic cells formed floating neurospheres. bFGF was added, or half the culture medium was changed every 2 days. The cultures were passaged every 8 to 10 days. For cell differentiation in the case of gene induction, the cells were first plated on a laminin-coated chamber slide and then cultured for 14 days under the same culture conditions as the ciliary- and iris-derived cells. 

For construction of CLIG-Crx and CLIG-Otx2, cDNAs for these factors were cloned into the EcoRI site of pCLIG, which directs expression of the cloned genes, together with enhanced green fluorescent protein (GFP) from the upstream long terminal repeat (LTR) promoter with cytomegalovirus enhancer. ¹⁹ To intensify the efficiency of the infection, viral preparations were pseudotyped with a vesicular stomatitis virus (VSV-G) coat protein. Retroviral DNAs and pcDNA-VSV-G (kindly provided by Tal Kafri, University of North Carolina), which are env expression vectors, were transfected (Lipofectamine; Invitrogen, Paisley, UK) into 293GP (BD-Clontech, Palo Alto, CA), the producer cells expressing gag and pol. ^{20 21} The supernatant was collected as described previously. ¹⁹  

After fixation with 4% paraformaldehyde, the samples were preincubated 1 hour with a blocking solution (5% normal goat serum and 0.1% Triton X-100 in PBS) and then incubated 3 hours at room temperature or overnight at 4°C in 1% goat serum and 0.1% Triton X-100, with the following antibodies: rabbit anti-GFP (1:500; Molecular Probes, Eugene, OR), mouse anti-rod opsin RET-P1 (1:2500; Sigma-Aldrich, St. Louis, MO), mouse anti-βIII-tubulin (TuJ1, 1:500; Sigma-Aldrich), mouse anti-nestin (1:1000; BD-PharMingen, San Diego, CA), and rabbit anti-glial fibrillary acidic protein (GFAP; 1:500; Dako, Glostrup, Denmark). Cell nuclei were counterstained with 4′,6′-diamidino-2-phenylindole (DAPI, 1:1000; Molecular Probes) or Cytox blue (1:500 in distilled water; Molecular Probes). Fluorescence was visualized by microscope (Leica Microsystems, Bannockburn, IL). Cultured cells were quantified by calculating the number of marker-positive cells as a percentage of immunopositive cells per ocular grid area at ×40 magnification (four random areas per sample). 

After cultured iris-derived cells and neural retina were washed three times with cold PBS, they were solubilized in 100 to 300 μL lysis buffer (50 mM Tris [pH 7.5], 0.5 M NaCl, 1% NP-40, 1% sodium deoxycholate monohydrate, 2 mM EDTA, and 0.1% SDS). After centrifugation at 10,000 rpm for 10 minutes, protein extracts were diluted with sample buffer (126 mM Tris HCl [pH 6.8] containing 20% glycerol, and 4% SDS, 0.005% bromophenol blue, and 5% 2-mercaptoethanol) at a 1:1 ratio and boiled for 3 minutes. Protein extracts were then subjected to 4% to 20% Tris-glycine gel electrophoresis and transferred electrically to a polyvinylidene difluoride (PVDF) membrane (Amersham Pharmacia Biotech, Buckinghamshire, UK). The membrane was then soaked for 1 hour at room temperature in a blocking buffer (TBS containing 0.2% Tween-20 and 5% skim milk) and incubated overnight at 4°C with the primary antibody: rabbit anti-recoverin (donated by James F. McGinnis and Rajesh J. Elias, University of Oklahoma Health Sciences Center, Oklahoma City, OK), ²² at a dilution of 1:8000, or rabbit anti-G∂t1 (Santa Cruz Biotechnology, Santa Cruz, CA) at a dilution of 1:500. The antibody was followed by the addition of horseradish-peroxidase–conjugated anti-mouse or rabbit Ig antibodies (Amersham Pharmacia Biotech) for 1 hour at room temperature. The membranes were then washed with TBS containing 0.2% Tween-20, and the signals detected with a Western blot analysis system (ECL; Amersham Pharmacia Biotech). 

To determine the effects of gene induction, we first prepared a replication-incompetent retrovirus, CLIG, which controls the expression of GFP as a marker of the upstream LTR promoter. For CLIG-Crx and CLIG-Otx2, cDNAs for Crx and Otx2 were inserted upstream of the internal ribosomal entry site (IRES) so that these genes were expressed bicistronically with GFP (Fig. 1) . 

It has been reported, with the neurosphere culture method, that adult mammalian eyes contain retinal stem cells in the ciliary margin. ^{13 14} To examine the effects of induction of Crx and Otx2 on ciliary-derived cells, we prepared ciliary-derived spheres from adult rats. Most of these cells were divided into single cells, and then, after 5 days, some of them formed spherical structures containing pigmented and nonpigmented progeny (Fig. 2A) . These results are consistent with those previously reported. ¹³ The spheres continued to grow slowly in serum-free medium containing bFGF, and many cells migrated from the spheres after they had been plated on a laminin-coated chamber slide (Fig. 2B) . Most of these cells (85.7% ± 1.41%, 262/306) immunostained with nestin, a marker for neural stem cells, a day after being plated. Table 1 shows the cell counts in the different types of cells studied. 

We next examined whether the ciliary-derived cells would respond to the forced expression of Crx and Otx2. The retrovirus was applied to the ciliary-derived cells 3 days after they had been plated on a laminin-coated chamber slide in serum-free medium, and the cells were transferred into an environment that promotes retinal cell differentiation. ^{13 16} As a negative control, 1.50% ± 1.37% of the CLIG-infected cells expressed rod opsin, suggesting that these ciliary-derived cells had rod-photoreceptor–producing capability without gene transfer (Figs. 2C 2D 2E 3) . In contrast, 91.7% ± 3.06% of the CLIG-Crx–infected and 92.3% ± 3.14% of the CLIG-Otx2–infected ciliary-derived cells had rod opsin immunoreactivity, suggesting that Crx and Otx2 induces the differentiation of ciliary-derived cells into photoreceptor-specific phenotypes, whereas only part of the CLIG-infected cells were rod opsin positive (Figs. 2F 2G 2H 2I 2J 2K 3) . 

Iris-derived cells were prepared as described previously. ¹⁶ The virus was applied to the iris-derived cells 4 to 5 days after culturing in serum-free medium, and the culture conditions were changed to an environment that promotes retinal cell differentiation 1 day after transfection. ^{13 16} After culturing for 14 days, 97.9% ± 1.50% of the CLIG-Crx–infected, iris-derived cells expressed rod opsin, whereas the iris-derived cells without gene transfer showed no rod opsin immunoreactivity, as has been reported (Figs. 3 4D 4E 4F) . ¹⁶ To examine whether Otx2 induces iris-derived cells to differentiate into a photoreceptor-specific phenotype, we applied CLIG-Otx2 to the cells, transferred them into an retinal cell-differentiation–promoting environment 1 day after transfection, and cultured them for 14 days. Of the CLIG-Otx2–infected, iris-derived cells, 95.7% ± 2.17% were immunopositive for rod opsin, demonstrating that Otx2 induction may lead the iris-derived cells to express rod opsin, whereas no CLIG-infected, iris-derived cells displayed immunoreactivity to rod opsin (Figs. 3 4A 4B 4C 4G 4H 4I) . The rod opsin-expressing cells misexpressed by Crx or Otx2 had small, round shapes, characteristic of rod photoreceptors in monolayer culture. Otx2 thus has the capacity to produce photoreceptor-like cells from iris-derived cells in the same manner as Crx, although it has not been determined whether Otx2 and Crx operate at the same hierarchical level to establish the identity of photoreceptors. 

To determine whether rod opsin expression responding to Crx- and Otx2-inductions were relatively specific for iris and ciliary-derived cells, we prepared neurospheres derived from E18.5 rat ventral mesencephalon (Figs. 5A 5B) . The mesencephalon-derived neurospheres proliferated in serum-free medium containing bFGF, and most of these cells were positive for nestin (Figs. 5D 5E 5F) . After being transferred to differentiation-promoting conditions, neurons (βIII-tubulin-positive: 4.5% ± 0.41%, 106/2364) and glial cells (GFAP positive: 80.5% ± 0.40%, 1903/2364) were produced from the same neurospheres, indicating that these neurospheres have the characteristics of neural stem cells (Fig. 5C) . 

To examine the effects of Crx and Otx2 induction on these neural stem cells, we applied CLIG, CLIG-Crx, and CLIG-Otx2 to the neurospheres and cultured them under differentiation-promoting conditions 1 to 3 days after plating them on laminin-coated chamber slides. The pseudotyped retrovirus effectively infected the cells of the neurospheres. No mesencephalic neural stem cells infected with CLIG were rod-opsin immunopositive, and only 2.88% ± 3.61% of the CLIG-Crx–infected cells and 7.0% ± 4.76% of the CLIG-Otx2–infected cells expressed rod opsin, suggesting that few of them acquired rod-opsin immunoreactivity, although transfection of the Crx and Otx2 genes into the neural stem cells was successful (Figs. 3 5G 5H 5I 5J 5K 5L 5M 5N 5O) . Most of the rod-opsin–negative cells misexpressed by Crx or Otx2 did not assume small, round shapes. This suggests that the mesencephalic neural stem cells may be intrinsically restricted in their response to Crx or Otx2. 

Immunocytochemical analysis showed that the Crx- and Otx2-transfected rat iris-derived cells were labeled with a monoclonal antibody against rod opsin, RETP1, whereas the iris-derived cells without gene delivery did not express rod opsin (Figs. 3 4A 4B 4C 4D 4E 4F 4G 4H 4I) . To determine whether the iris-derived cells with Crx- or Otx2-gene transfer expresses any other phototransduction components, anti-recoverin and anti-α subunits of transducin (G∂t1) antibodies were tested by means of Western blot. Total protein extract from the rat retina (1.0 μg) was used as a positive control (Figs. 6A 6B ; lane 4). Recoverin is a calcium-binding protein that is involved in the inactivation of phototransduction, and G∂t1 is a photoreceptor-specific G-protein molecule that activates cGMP-specific phosphodiesterase (PDE). ²³ We recognized similar patterns in the extracts (40 μg/lane) of the Crx- and Otx2-transfected, iris-derived cells that expressed recoverin and G∂t1, although we did not detect bands of the same size in equal amounts of proteins prepared from the iris-derived cells infected with CLIG as we did in the corresponding retinal extracts (Figs. 6A 6B ; lanes 1–3). These results indicated that the Crx- and Otx2-transfected rat iris-derived cells express at least two additional key components of the phototransduction cascade: recoverin and G∂t1. 

In this study, both Otx2 and Crx inductions effectively led ciliary- and iris-derived cells to differentiate into a photoreceptor-specific phenotype. These photoreceptor-like cells induced by Otx2 and Crx misexpressions displayed photoreceptor-specific morphology in vitro. A recently conducted extensive experiment, using an Otx2 conditional knockout mouse line in which the Otx2 genes were inactivated under control of the Crx promoter, proved that Otx2 is a key regulatory gene for photoreceptor development. ¹² In our study, Otx2 induction effectively led ciliary- and iris-derived cells to differentiate into a photoreceptor-specific phenotype. However, the mechanism of the photoreceptor generation remains obscure, in that Otx2 expression is not restricted to the photoreceptor cells, but covers most of the forebrain and midbrain, including the eye domain in the developmental stage. ²⁴ Furthermore, Otx2 expression in the eye has been demonstrated in several cell types, including bipolar cells, ganglion cells, photoreceptor cells, and retinal pigment epithelial cells. ^{12 25 26} In addition, Otx2 has been shown to be a direct upstream regulator of Crx, so that Crx is also thought to be misexpressed in Otx2-induced cells. ¹² Crx appears to be capable of inducing photoreceptor-specific phenotypes in ciliary- and iris-derived cells, although further studies are needed to examine the differences between Crx- and Otx2-induced cells in terms of other photoreceptor-specific characteristics, including photoresponsiveness, which may provide the key to producing genuine functional photoreceptors. 

The pigmented cells of the adult mouse ciliary marginal zone contain a population of retinal stem cells. ^{13 14} We cultured pigmented cells of the ciliary margin and successfully obtained neurospheres; however, without gene induction the level of expression of rod opsin by the differentiated cells in our experiment was very small compared with the a previously report. ¹³ This low rod photoreceptor-generating capability is possibly due to different culture conditions, including dissociation and culture media. Another possible cause is the difference in species—that is, mouse and rat. ¹³ Although the culture conditions for ciliary-derived cells need improvement, Crx or Otx2 induction helped increase the differentiation efficiency of photoreceptor cells dramatically. 

It has been reported that cultured human ciliary epithelial cells have the potential to express components of phototransduction, ²⁷ whereas iris tissue also reportedly to has the potential to respond to light in vitro and in vivo by following a non-neural pathway. ^{28 29 30 31 32} The iris-derived cells in our study, however, did not differentiate into cells expressing rod opsin, recoverin, and G∂t1 without appropriate gene induction, which means that rat iris tissue does not normally express components of phototransduction. The possible explanation for this is that iris-derived cells normally have the potential to express these components, including rhodopsin, but that their expression levels are too low to be detectable by immunocytochemistry. 

We have reported that Crx does not induce rhodopsin immunoreactivity in hippocampus-derived neural stem cells. ¹⁶ In the current study, some cell populations responded to Crx or Otx2 induction in neurospheres derived from the embryonic mesencephalon, although only very few did so. This lack of uniformity may be explained in terms of the different characteristics between the long-cultured neural stem cells and the freshly obtained neural progenitor cells. Further studies are needed to find an explanation for the inhibitory effects of other gene products, which may result in gaining information as to how to produce photoreceptor cells from other tissues. 

In conclusion, forced expression of the Otx2 gene, in the same manner as the Crx gene, effectively induced the cells derived from the adult iris and ciliary margin to become photoreceptor-like cells, whereas most of the mesencephalon-derived neural stem cells did not respond to Otx2. Furthermore, the Crx- and Otx2-transfected rat iris-derived cells expressed at least two additional key components of the phototransduction cascade. Thus, the Otx2 gene is one of the key regulators of both normal photoreceptor development and, by means of gene delivery, photoreceptor production. 

 

The authors thank Constance L. Cepko (Harvard Medical School, Boston, MA) and Takahisa Furukawa (Osaka Bioscience Institute, Osaka, Japan) for their generous gift of Crx cDNA.