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Toll-like receptor 4 restricts retinal progenitor cell proliferation
Correspondence to Michal Schwartz: michal.schwartz{at}weizmann.ac.il
Retinal neurogenesis ceases by the early postnatal period, although retinal progenitor cells (RPCs) persist throughout life. In this study, we show that in the mammalian eye, the function of Toll-like receptor 4 (TLR4) extends beyond regulation of the innate immune response; it restricts RPC proliferation. In TLR4-deficient mice, enhanced proliferation of cells reminiscent of RPCs is evident during the early postnatal period. In vitro experiments demonstrate that TLR4 acts as an intrinsic regulator of RPC fate decision. Increased TLR4 expression in the eye correlates with the postnatal cessation of cell proliferation. However, deficient TLR4 expression is not sufficient to extend the proliferative period but rather contributes to resumption of proliferation in combination with growth factors. Proliferation in vivo is inhibited by both MyD88-dependent and -independent pathways, similar to the mechanisms activated by TLR4 in immune cells. Thus, our study attributes a novel role to TLR4 as a negative regulator of RPC proliferation.
Abbreviations used in this paper: ANOVA, analysis of variance; βIIIT, βIII-tubulin; CE, ciliary epithelium; CNS, central nervous system; DCX, doublecortin; GF, growth factor; PN, postnatal day; RPC, retinal progenitor cell; TLR, Toll-like receptor; TLR4D, TLR4 deficient; upLPS, ultrapurified lipopolysaccharide; WT, wild type.
© 2008 Shechter et al. This article is distributed under the terms of an Attribution–Noncommercial–Share Alike–No Mirror Sites license for the first six months after the publication date (see http://www.jcb.org/misc/terms.shtml). After six months it is available under a Creative Commons License (Attribution–Noncommercial–Share Alike 3.0 Unported license, as described at http://creativecommons.org/licenses/by-nc-sa/3.0/).
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Introduction |
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 TopAbstract Introduction Results and discussionMaterials and methodsReferences |
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The expression of Toll-like receptor 4 (TLR4) has been recently documented in the ciliary body of the mammalian eye (Brito et al., 2004). TLR4 is primarily identified as an innate immune receptor (Takeda and Akira, 2005); therefore, its function in the eye has been commonly attributed to the immune response (Kumar et al., 2004; Chang et al., 2006). However, because TLRs recognize patterns rather than specific molecules, along with their ability to recognize physiological compounds (Ohashi et al., 2000; Okamura et al., 2001; Johnson et al., 2003), they are endowed with the innate ability to mediate a rapid response to a wide range of signals in the microenvironment and not merely to pathogens.
Nonimmune functions of the TLR family have been reported in Drosophila melanogaster in establishing the dorsal–ventral axis polarity, in synaptogenesis, and in axon pathfinding during embryogenesis (Anderson et al., 1985; Halfon et al., 1995; Rose et al., 1997). Such nonimmune functions of this receptor family have only recently emerged in mammals. We have recently shown that in the adult mammalian central nervous system (CNS), TLRs, including TLR4, regulate adult hippocampal neurogenesis (Rolls et al., 2007). In mammalian brain development, other members of the TLR family, TLR3 and TLR8, were identified as negative regulators of axonal/neurite outgrowth (Ma et al., 2006; Cameron et al., 2007). Conversely, TLR4 was found to be absent in neurons during the developmental stages of CNS formation (Lehnardt et al., 2003); however, with age, its expression levels increase (Wadachi and Hargreaves, 2006).
Collectively, the functions that have been recently attributed to TLRs in the mammalian CNS, the changes in TLR expression pattern with development, and the evidence of TLR4 expression in the retinal ciliary body, a location known to harbor RPCs, raised the possibility that TLR4 may play a role in the mammalian retina in RPC fate determination.
In this study, we identified TLR4 as a negative regulator of RPC proliferation. During the early postnatal period, TLR4-deficient (TLR4D) mice exhibited enhanced proliferation of cells expressing molecular markers commonly attributed to RPCs. In vitro experiments demonstrated that TLR4 directly modulates RPC fate decision. The increase in TLR4 levels, which coincided with the cessation of proliferation in the ciliary body, was found to be one of the factors that contributed to the decrease in proliferation. Thus, we suggest that although TLR4 is not the primary factor that regulates RPC proliferative capacity throughout life, it does determine the sensitivity of these cells to the microenvironment.
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Results and discussion |
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TopAbstractIntroductionResults and discussionMaterials and methodsReferences |
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Quantitative analysis 7 d after injection revealed an increased number of BrdU+ cells expressing the neuronal marker βIII-tubulin (βIIIT) in the TLR4D mice (16,590 ± 1,872 vs. 8,480 ± 2,687, TLR4D vs. WT, respectively; Student's t test, *, P = 0.05). This increase was not solely a result of enhanced proliferation but also an outcome of increased differentiation into neuronal cells (Fig. 2, A–C).
Because rod photoreceptors and bipolar cells are the major retinal neuronal cells formed during late histogenesis, we also quantified the percentage (out of total BrdU+ cells) of the bipolar-specific marker PKC-
and the photoreceptor-specific marker recoverin. Increased differentiation into the tested retinal neuronal cell types was evident in TLR4D mice (Fig. 2, A and B). Notably, these differences did not result from differential survival, as no effect on apoptosis (measured by cleaved caspase 3) was observed (Fig. 2 B). Collectively, these results suggest that in the PN6 retina, deficiency in TLR4 leads to both enhanced proliferation and neuronal differentiation of cells expressing markers characteristic of retinal progenitors.
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B, which acts as a master switch, regulating the transcription of many genes. TLR signaling, which relies on cytoplasmic adaptor molecules that can associate with the intracellular region of the TLR molecule, exerts its effect via two main signaling pathways, MyD88 (myeloid differentiation primary response protein 88)-dependent and -independent cascades. The former involves the activation of the intracellular adaptor MyD88, and the latter entails the participation of another adaptor, TICAM1 (TIR domain–containing adaptor protein inducing INF-β; Akira and Takeda, 2004; Krishnan et al., 2007).
Previous studies indicated that in developing neurons, TLR activation does not activate NFB (Ma et al., 2006; Cameron et al., 2007), demonstrating that a different signaling pathway is induced in these cells. In contrast, TLR4 activation in adult neural progenitor cells results in the activation of both MyD88-dependent and -independent pathways (Rolls et al., 2007), similar to the pathways activated in the immune system. As the proliferation of RPCs can be considered a recapitulation of both neurogenesis and developmental processes, we wished to identify the signaling pathways used in this process. Therefore, we tested whether MyD88 and TICAM1 participate in the regulation of cell proliferation in the eye. We found increased numbers of BrdU+ cells in the peripheral retina and the CE of both MyD88- and TICAM1-deficient mice relative to WT PN6 mice (Fig. 4, A–C).
We further confirmed that the proliferating cells expressed markers characteristic of RPCs, including nestin, Pax6, and Chx10 (Fig. 4 D). Our results therefore suggest that cell proliferation in the early postnatal eye is inhibited by both MyD88-dependent and -independent pathways, similar to the mechanism activated by TLRs in immune cells.
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The absence of proliferating RPCs in the adult eye can be either attributed to the lack of proliferation-promoting factors or to the presence of inhibitory molecules. The former was recently demonstrated, as GF administration results in in vivo proliferation of cells expressing markers characteristic of RPCs (Fischer and Reh, 2003; Zhao et al., 2005). Therefore, we tested whether TLR4 participates in restricting proliferation when GFs are provided (Fischer and Reh, 2003; Zhao et al., 2005). We intravitreally injected FGF-2 and insulin as previously described (Zhao et al., 2005) to WT and TLR4D mice at PN15 (Fig. 5 F). Incorporation of BrdU, which was injected together with the GF, revealed, as expected, an extension of the proliferation period. As in the early postnatal stage, providing the eye with GF resulted in significantly higher proliferation in the TLR4D mice compared with the WT animals (Fig. 5, G–I), indicating that TLR4 had a negative impact on proliferation when conditions permissive for RPC proliferation were restored. To confirm these results and to demonstrate the effect of GFs on cell proliferation, we analyzed retinas for the expression of Ki67. A higher number of proliferating cells was seen in the GF-treated retinas relative to controls in both strains (Fig. 5 J); however, the effect was far more pronounced in the TLR4D mice (fourfold increase) than in their matched controls (2.5-fold increase; Fig. 5 J). We further confirmed that the observed increased proliferation involved cells expressing markers distinguishing RPCs, such as Pax6 and Chx10 (Fig. 5, K and L). These results suggest that under permissive conditions, TLR4 down-regulates proliferation. Importantly, deficiency in TLR4 had a more pronounced effect on proliferation in the PN15 eyes supplied with GF relative to PN6 eyes (Fig. 5 M). This pronounced effect is supported by the enhanced expression of TLR4 at PN15 relative to PN6 (Fig. 5, A–C). Thus, our findings suggest that even though it cannot be considered the primary limiting factor of RPC proliferation in adulthood, enhanced TLR4 expression in the eye contributes to the restriction of RPC proliferation.
In this study, we identified TLR4 as a novel player in the regulation of RPC proliferation in the mammalian eye. We found that TLR4 inhibits proliferation of retinal cells expressing progenitor markers in the early postnatal period and contributes to their lack of proliferation in the subsequent time period. In vitro experiments confirmed that TLR4 is expressed on the RPCs and directly affects their cell fate decision. Notably, TLR4 does not belong to any of the previously known classes of cell–cell signaling pathways used to determine the fate of RPCs (Yang, 2004). Interestingly, the major classes of known cell–cell signaling pathways share a common property with the TLR orthologue, as they all participate in dorsal–ventral patterning in Drosophila (Biemar et al., 2006). Moreover, because similar effects of TLR4 on neural progenitor cell proliferation are also evident in the adult hippocampus (Rolls et al., 2007), our results further emphasize the importance of this receptor family in neurogenic processes in general.
TLR4 is a member of a larger receptor family. Thus, our results suggest that additional members of this family may participate in retinogenesis and RPC fate regulation. Revealing the specific function of these family members necessitates further investigation. The unique features of the TLR family, including pattern recognition rather than identification of a single ligand and their ability to recognize stress-related compounds (Johnson et al., 2003) or pathogens, provide RPCs with the capacity to respond to various deviations from homeostasis, such as injury. Our finding that TLR4 restricts RPC proliferation might provide, at least in part, an explanation for the limited neurogenesis in response to injury (Nickerson et al., 2007), a condition that releases a variety of ligands that can ultimately be recognized by the TLR family (Vabulas et al., 2002). Revealing the mechanisms that constrain RPC proliferation has promising therapeutic potential for inducing neurogenesis in the adult eye under pathological conditions.
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Materials and methods |
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TopAbstractIntroductionResults and discussionMaterials and methodsReferences |
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Administration of BrdU
Animals were given intraperitoneal injections of 0.125 mg/gram of body weight of BrdU (Sigma-Aldrich). For proliferation assays, mice were killed 6 h after injection, and their eyes were removed and prepared for histology as described in the Immunohistochemistry section. For differentiation assays, injected mice were maintained for 7 d and then killed.
GF administration
TLR4D and C57BL/10 PN15 mice were anesthetized, and GFs (20 ng/µl FGF-2 and 1 µg/µl insulin) together with 1 µg/µl BrdU were delivered into left eyes by intravitreal injection using a glass micropipette attached to a 10-µl Hamilton syringe (total volume of 1 µl/eye). Mice were injected on four consecutive days and killed 24 h after the last injection. Eyes were removed and prepared for histology as described in the next section.
Immunohistochemistry
Mice eyes were placed in 2.5% paraformaldehyde for 48 h and moved to 70% ethyl alcohol. The tissues were prepared for histology and stained as previously described (Shechter et al., 2007). The antibodies used are listed in Table I.
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Image acquisition and quantification
Cyanine dye (Cy2 [A492nm and E510nm], Cy3 [A550nm and E570nm], or Cy5 [A650nm and E670nm])–conjugated antibodies (Jackson ImmunoResearch Laboratories) were used to visualize antibody-bound molecules. For nuclear staining, we used Hoechst 33342 fluorochrome (Invitrogen). The stained sections were mounted with glycerol vinyl alcohol mounting solution (Invitrogen). For microscopic analysis, a fluorescence microscope (E800; Nikon) or laser-scanning confocal microscope (Carl Zeiss, Inc.) was used. The fluorescence microscope was equipped with a digital camera (DXM 1200F; Nikon) and with either a 20x NA 0.50 or 40x NA 0.75 objective lens (Plan Fluor; Nikon). The confocal microscope was equipped with LSM 510 laser scanning (three lasers: Ar 488, HeNe 543, and HeNe 633) and with a 40x oil-immersion NA 1.3 Plan Neofluor objective lens. Recordings were made on postfixed tissues at 24°C using acquisition software (ACT-1 [Nikon]; or LSM [Carl Zeiss, Inc.]). Images were cropped and optimized in Photoshop 9.0 (Adobe Systems, Inc.) by making minor adjustments to contrast and arranged using Canvas X (Deneba Software). The number of cells in the peripheral retina and immunoreactivity in the CE was determined automatically with Image-Pro Plus 4.5 software (Media Cybernetics, Inc.). All measurements were performed by an observer blinded as to the identity of the examined tissues.
Statistical analysis
The results were analyzed by Student's t test or factorial analysis of variance (ANOVA) followed by Fisher's exact test and are expressed as means ± SEM.
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Acknowledgments |
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This study was supported, in part, by a grant from the Siegal Foundation and the Glaucoma Foundation, New York. M. Schwartz holds the Maurice and Ilse Katz Professorial Chair in Neuroimmunology. R. Shechter, A. Ronen, and A. Rolls designed and performed the experiments, analyzed the data, and took part in writing the manuscript. A. London contributed to the experimental work. S. Bakalash isolated the RPCs.
Submitted: 1 April 2008
Accepted: 30 September 2008
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References |
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Ahmad, I., L. Tang, and H. Pham. 2000. Identification of neural progenitors in the adult mammalian eye. Biochem. Biophys. Res. Commun. 270:517–521.[CrossRef][Medline]
Akira, S., and K. Takeda. 2004. Toll-like receptor signalling. Nat. Rev. Immunol. 4:499–511.[CrossRef][Medline]
Anderson, K.V., L. Bokla, and C. Nusslein-Volhard. 1985. Establishment of dorsal-ventral polarity in the Drosophila embryo: the induction of polarity by the Toll gene product. Cell. 42:791–798.[CrossRef][Medline]
Biemar, F., D.A. Nix, J. Piel, B. Peterson, M. Ronshaugen, V. Sementchenko, I. Bell, J.R. Manak, and M.S. Levine. 2006. Comprehensive identification of Drosophila dorsal-ventral patterning genes using a whole-genome tiling array. Proc. Natl. Acad. Sci. USA. 103:12763–12768.
Blanks, J.C., and D. Bok. 1977. An autoradiographic analysis of postnatal cell proliferation in the normal and degenerative mouse retina. J. Comp. Neurol. 174:317–327.[CrossRef][Medline]
Brito, B.E., D.O. Zamora, R.A. Bonnah, Y. Pan, S.R. Planck, and J.T. Rosenbaum. 2004. Toll-like receptor 4 and CD14 expression in human ciliary body and TLR-4 in human iris endothelial cells. Exp. Eye Res. 79:203–208.[CrossRef][Medline]
Butovsky, O., Y. Ziv, A. Schwartz, G. Landa, A.E. Talpalar, S. Pluchino, G. Martino, and M. Schwartz. 2006. Microglia activated by IL-4 or IFN-gamma differentially induce neurogenesis and oligodendrogenesis from adult stem/progenitor cells. Mol. Cell. Neurosci. 31:149–160.[CrossRef][Medline]
Cameron, J.S., L. Alexopoulou, J.A. Sloane, A.B. DiBernardo, Y. Ma, B. Kosaras, R. Flavell, S.M. Strittmatter, J. Volpe, R. Sidman, and T. Vartanian. 2007. Toll-like receptor 3 is a potent negative regulator of axonal growth in mammals. J. Neurosci. 27:13033–13041.
Chang, J.H., P.J. McCluskey, and D. Wakefield. 2006. Toll-like receptors in ocular immunity and the immunopathogenesis of inflammatory eye disease. Br. J. Ophthalmol. 90:103–108.
Fischer, A.J., and T.A. Reh. 2003. Growth factors induce neurogenesis in the ciliary body. Dev. Biol. 259:225–240.[CrossRef][Medline]
Halfon, M.S., C. Hashimoto, and H. Keshishian. 1995. The Drosophila toll gene functions zygotically and is necessary for proper motoneuron and muscle development. Dev. Biol. 169:151–167.[CrossRef][Medline]
Johnson, G.B., G.J. Brunn, and J.L. Platt. 2003. Activation of mammalian Toll-like receptors by endogenous agonists. Crit. Rev. Immunol. 23:15–44.[CrossRef][Medline]
Krishnan, J., K. Selvarajoo, M. Tsuchiya, G. Lee, and S. Choi. 2007. Toll-like receptor signal transduction. Exp. Mol. Med. 39:421–438.[Medline]
Kumar, M.V., C.N. Nagineni, M.S. Chin, J.J. Hooks, and B. Detrick. 2004. Innate immunity in the retina: Toll-like receptor (TLR) signaling in human retinal pigment epithelial cells. J. Neuroimmunol. 153:7–15.[CrossRef][Medline]
Lehnardt, S., L. Massillon, P. Follett, F.E. Jensen, R. Ratan, P.A. Rosenberg, J.J. Volpe, and T. Vartanian. 2003. Activation of innate immunity in the CNS triggers neurodegeneration through a Toll-like receptor 4-dependent pathway. Proc. Natl. Acad. Sci. USA. 100:8514–8519.
Ma, Y., J. Li, I. Chiu, Y. Wang, J.A. Sloane, J. Lu, B. Kosaras, R.L. Sidman, J.J. Volpe, and T. Vartanian. 2006. Toll-like receptor 8 functions as a negative regulator of neurite outgrowth and inducer of neuronal apoptosis. J. Cell Biol. 175:209–215.
MacLaren, R.E., R.A. Pearson, A. MacNeil, R.H. Douglas, T.E. Salt, M. Akimoto, A. Swaroop, J.C. Sowden, and R.R. Ali. 2006. Retinal repair by transplantation of photoreceptor precursors. Nature. 444:203–207.[CrossRef][Medline]
Neeley, W.L., S. Redenti, H. Klassen, S. Tao, T. Desai, M.J. Young, and R. Langer. 2008. A microfabricated scaffold for retinal progenitor cell grafting. Biomaterials. 29:418–426.[CrossRef][Medline]
Nickerson, P.E., J.G. Emsley, T. Myers, and D.B. Clarke. 2007. Proliferation and expression of progenitor and mature retinal phenotypes in the adult mammalian ciliary body after retinal ganglion cell injury. Invest. Ophthalmol. Vis. Sci. 48:5266–5275.
Ohashi, K., V. Burkart, S. Flohe, and H. Kolb. 2000. Cutting edge: heat shock protein 60 is a putative endogenous ligand of the toll-like receptor-4 complex. J. Immunol. 164:558–561.
Okamura, Y., M. Watari, E.S. Jerud, D.W. Young, S.T. Ishizaka, J. Rose, J.C. Chow, and J.F. Strauss III. 2001. The extra domain A of fibronectin activates Toll-like receptor 4. J. Biol. Chem. 276:10229–10233.
Reh, T.A., and A.J. Fischer. 2006. Retinal stem cells. Methods Enzymol. 419:52–73.[CrossRef][Medline]
Rolls, A., R. Shechter, A. London, Y. Ziv, A. Ronen, R. Levy, and M. Schwartz. 2007. Toll-like receptors modulate adult hippocampal neurogenesis. Nat. Cell Biol. 9:1081–1088.[CrossRef][Medline]
Rose, D., X. Zhu, H. Kose, B. Hoang, J. Cho, and A. Chiba. 1997. Toll, a muscle cell surface molecule, locally inhibits synaptic initiation of the RP3 motoneuron growth cone in Drosophila. Development. 124:1561–1571.[Abstract]
Shechter, R., Y. Ziv, and M. Schwartz. 2007. New GABAergic interneurons supported by myelin-specific T cells are formed in intact adult spinal cord. Stem Cells. 25:2277–2282.[CrossRef][Medline]
Takeda, K., and S. Akira. 2005. Toll-like receptors in innate immunity. Int. Immunol. 17:1–14.
Tropepe, V., B.L. Coles, B.J. Chiasson, D.J. Horsford, A.J. Elia, R.R. McInnes, and D. van der Kooy. 2000. Retinal stem cells in the adult mammalian eye. Science. 287:2032–2036.
Vabulas, R.M., H. Wagner, and H. Schild. 2002. Heat shock proteins as ligands of toll-like receptors. Curr. Top. Microbiol. Immunol. 270:169–184.[Medline]
Wadachi, R., and K.M. Hargreaves. 2006. Trigeminal nociceptors express TLR-4 and CD14: a mechanism for pain due to infection. J. Dent. Res. 85:49–53.
Yang, X.J. 2004. Roles of cell-extrinsic growth factors in vertebrate eye pattern formation and retinogenesis. Semin. Cell Dev. Biol. 15:91–103.[CrossRef][Medline]
Young, M.J. 2005. Stem cells in the mammalian eye: a tool for retinal repair. APMIS. 113:845–857.[CrossRef][Medline]
Young, R.W. 1985. Cell differentiation in the retina of the mouse. Anat. Rec. 212:199–205.[CrossRef][Medline]
Zhao, X., A.V. Das, F. Soto-Leon, and I. Ahmad. 2005. Growth factor-responsive progenitors in the postnatal mammalian retina. Dev. Dyn. 232:349–358.[CrossRef][Medline]
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