Microglia-Muller Glia Cell Interactions Control Neurotrophic Factor Production during Light-Induced Retinal Degeneration

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The Journal of Neuroscience, November 1, 2002, 22(21):9228-9236

Microglia-Müller Glia Cell Interactions Control Neurotrophic Factor Production during Light-Induced Retinal Degeneration
Takayuki Harada¹^,³^,⁴^,⁶^,^*, Chikako Harada¹^,³^,⁴^,⁶^,^*, Shinichi Kohsaka², Etsuko Wada¹, Kazuhiko Yoshida³, Shigeaki Ohno³, Hiroshi Mamada⁴, Kohichi Tanaka⁴^,⁵, Luis F. Parada⁶, and Keiji Wada¹
Departments of ¹ Degenerative Neurological Diseases and ² Neurochemistry, National Institute of Neuroscience, National Center of Neurology and Psychiatry, Kodaira, Tokyo 187-8502, Japan, ³ Department of Ophthalmology and Visual Sciences, Hokkaido University Graduate School of Medicine, Sapporo, Hokkaido 060-8638, Japan, ⁴ Department of Molecular Neuroscience, Medical Research Institute, Tokyo Medical and Dental University, Tokyo 113-8510, Japan, ⁵ PRESTO, Japan Science and Technology Corporation, Kawaguchi, Saitama 332-0012, Japan, and ⁶ Center for Developmental Biology and Kent Waldrep Foundation Center for Basic Research on Nerve Growth and Regeneration, University of Texas Southwestern Medical Center, Dallas, Texas 75390-9133

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Activation of microglia commonly occurs in response to a wide variety of pathological stimuli including trauma, axotomy, ischemia,and degeneration in the CNS. In the retina, prolonged or high-intensityexposure to visible light leads to photoreceptor cell apoptosis.In such a light-reared retina, we found that activated microgliainvade the degenerating photoreceptor layer and alter expressionof neurotrophic factors such as nerve growth factor (NGF), ciliaryneurotrophic factor (CNTF), and glial cell line-derived neurotrophicfactor (GDNF). Because these neurotrophic factors modulate secondarytrophic factor expression in Müller glial cells, microglia-Müllerglia cell interaction may contribute to protection of photoreceptorsor increase photoreceptor apoptosis. In the present study, wedemonstrate the possibility that such functional glia-glia interactionsconstitute the key mechanism by which microglia-derived NGF, brain-derivedneurotrophic factor (BDNF), and CNTF indirectly influence photoreceptorsurvival, although the receptors for these neurotrophic factorsare absent from photoreceptors, by modulating basic fibroblastgrowth factor (bFGF) and GDNF production and release from Müllerglia. These observations suggest that microglia regulate the microglia-Müllerglia-photoreceptor network that serves as a trophic factor-controllingsystem during retinaldegeneration.

Key words: microglia; Müller glial cell; photoreceptor; neurotrophins; glia-glia interaction; glia-neuron interaction; retinal degeneration

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Many growth factors and neurotrophins have been shown to promote the survival of retinal neurons. For example, intraocularinjection of brain-derived neurotrophic factor (BDNF), neurotrophin-3(NT-3), ciliary neurotrophic factor (CNTF), glial cell line-derivedneurotrophic factor (GDNF), or basic fibroblast growth factor(bFGF) rescues photoreceptors in animal models of retinal degeneration(Faktorovich et al., 1990, 1992; LaVail et al., 1992, 1998; Cayouetteet al., 1998; Chong et al., 1999; Frasson et al., 1999). BDNFand NT-3 mediate cell survival via two types of transmembraneglycoproteins, the high-affinity trk tyrosine kinase receptorsand the low-affinity neurotrophin receptor p75 (p75^NTR) (Barbacid, 1994). On the other hand, signal transduction byCNTF requires that it bind first to CNTFR $alpha$ , a receptor anchoredto the cell membrane through a glycosyl-phosphatidylinositol (GPI)linkage (Ip et al., 1993). The binding of CNTF to CNTFR $alpha$ leadsto recruitment and dimerization of gp130 and leukemia inhibitoryfactor receptor (Davis et al., 1993). GDNF and neurturin act throughmulticomponent receptor complexes, namely the ligand-binding GPI-linkedproteins (GFR $alpha$ 1 and GFR $alpha$ 2) and the transmembrane protein tyrosinekinase Ret (Baloh et al., 2000; Harada et al., 2002).

Paradoxically, BDNF and CNTF are consistently reported as neuroprotective for photoreceptor cells, although these cells donot express their receptors (Ugolini et al., 1995; Kirsch et al.,1997; Harada et al., 2000). However, intraocular administrationof BDNF or CNTF activates Müller glial cells exclusively (notphotoreceptors) (Wahlin et al., 2000). In addition, BDNF has nodirect effect on isolated photoreceptor cells (Carwile et al.,1998). Thus, these trophic factors may protect photoreceptors,at least partly, through Müller glial cells (Zack, 2000; Bringmannand Reichenbach, 2001). In fact, Müller cells contain receptorsfor most of the molecules involved in photoreceptor rescue andbecome stimulated after retinal insults such as mechanical injury(Harada et al., 1995; Wen et al., 1995; Yoshida et al., 1995),ischemia (Ju et al., 1999), and light-induced degeneration (Wenet al., 1998). We previously provided additional direct supportfor such a "Müller cell hypothesis" in that Müller cells, actingin response to NT-3 or nerve growth factor (NGF), respectively,increase or decrease their production of bFGF, which in turn resultsin either the protection or increased apoptosis of photoreceptorcells (Harada et al., 2000). However, the origin of endogenoustrophic factors with which Müller cells interact during photoreceptordegeneration remainsunclear.

Inherited retinal degeneration is accompanied by the migration of phagocytic cells into the outer retina where photoreceptordegeneration occurs, and the phagocytic cells are derived fromresident microglial cells and not from peripheral macrophages(Thanos, 1992; Roque et al., 1996). These results suggest thatmicroglial cells play a critical role during photoreceptor degeneration.However, it is still unknown whether microglia contribute to theneuroprotection by producing neurotrophic factors or exert a cytotoxicfunction by releasing reactive oxygen species, nitric oxide, orinflammatory cytokines (Kreutzberg, 1996; Graeber et al., 1998;Ito et al., 1998, 2001; Nakajima et al., 1998, 2001). In the presentstudy, we examine the effect of photoreceptor degeneration onthe production of neurotrophic factors in microglia and proposea possible mechanism for communication between microglia and neighboringMüller glia and photoreceptors. We also examine whether the Müllercell hypothesis holds for BDNF, CNTF, and GDNF, as it does forNGF and NT-3 (Harada et al., 2000).

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experimental animals. Experiments were performed using Wistar rats, C57BL/6J mice, and p75^NTR knock-out mice (purchased from the Jackson Laboratory) in accordancewith the ARVO statement for the Use of Animals in Vision Research.Animals were maintained in either a 12 hr light/dark cycle (LD12:12) or 24 hr of constant illumination. Light intensity insidethe cages ranged from 100 to 200 lux under LD 12:12, whereas 800-1300lux was used for 24 hr of constant illumination to effect light-inducedretinal degeneration (Harada et al., 1996, 1998a).

Immunohistochemistry. Rats were anesthetized with diethylether and perfused transcardially with saline, followed by 4% paraformaldehydein 0.1 M phosphate buffer containing 0.5% picric acid at roomtemperature. Rat eyes were removed and postfixed overnight inthe same fixative and then embedded in paraffin. The posteriorportion of the eye was sectioned sagittally at 7 µm thickness,mounted, and stained with hematoxylin and eosin. For immunohistochemicalstaining, the sections were incubated in PBS containing 10% normalgoat serum for 30 min at room temperature. They were then incubatedovernight with a microglia-specific rabbit polyclonal antibody,iba1 (1.0 µg/ml) (Graeber et al., 1998; Ito et al., 1998, 2001;Nakajima et al., 1998) and a mouse monoclonal antibody againstED1 (Serotec; 100×) and visualized with Cy3-conjugated goat anti-rabbitIgG (Amersham Biosciences) and FITC-conjugated goat anti-mouseIgG (Jackson ImmunoResearch). The sections were examined witha confocal laser scanning microscope (Olympus).

Cell culture. Microglial cells were isolated from postnatal day (P) 35 rat eyes reared under LD 12:12 or 24 hr of constantillumination and cultured as described previously (Roque and Caldwell,1993). These culture cells were examined immunocytochemicallyafter incubation with the rabbit polyclonal antibody iba1 (1.0µg/ml) or a Müller cell-specific antibody against GLAST (1.0µg/ml) (Harada et al., 1998b). A portion of culture medium wasused to quantify NGF (Chemicon), NT-3 (Promega), GDNF (Promega),and bFGF (R & D Systems) protein expression levels using ELISAassaykits.

Müller cells were isolated from P35 rat eyes and cultured according to an established protocol (Hicks and Courtois, 1990).Total RNA for PCR was prepared from these cells that were eitherunstimulated or stimulated with 100 ng/ml of recombinant BDNF,CNTF, bFGF, or GDNF for 12 hr. In some experiments (see Figs.4, 5), these Müller culture cells were incubated with microglia-conditionedmedium (MCM) for 12 hr. MCM was prepared from both normal andlight-damaged retina, and the final medium change was performed72 hr before use. Trk-specific inhibitor K252a (Kyowa Hakko; 100ng/ml), NT-3 blocking antibody (Chemicon; 1 µg/ml), and REX antiserumdirected toward the extracellular domain of the p75^NTR (Weskamp and Reichardt, 1991) (courtesy of L. F. Reichardt, Universityof California San Francisco) (diluted 1:100) were added 30 minbefore MCMtreatment.

Laser capture microdissection. Laser capture microdissection (LCM) was performed as described (Harada et al., 2000). Fiftyfrozen sections (7 µm thick) were made from each P35 eye and stainedwith hematoxylin. LCM system LM200 (Olympus) was used for lasercapture. Following the manufacturer's protocols, samples wereobtained from the outer nuclear layer (ONL) (see Fig. 3A,B), avoidingcontamination from neighboring layers. Total RNA was extractedfrom the LCM samples from three independent animals in both thenormal and light-rearedgroups.

Quantitative RT-PCR analysis. Complementary DNA reverse transcribed from total RNA was amplified by using specific primersas shown in the supplemental Table (available at www.jneurosci.org).Negative controls for PCR were performed using "templates" derivedfrom reverse transcription (RT) reactions lacking either reversetranscriptase or total RNA. Quantitative RT-PCR analysis was performedas reported previously (Harada et al., 1998a). To construct astandard curve, 3.75-30 ng of total RNA was reverse transcribed,and the resulting cDNA was subjected to 20 (G3PDH), 38 [NT-3,Ret, and inducible nitric oxide synthase (iNOS)], or 32 (others)cycles of PCR. Ten microliters of each reaction mixture were removedafter each cycle during cycles 12-20 (G3PDH), 30-38 (NT-3, Ret,and iNOS) or 24-32 (others) and electrophoresed on a 2% Tris borate-EDTAAgarose gel. The gel was stained with ethidium bromide to detectthe bands of amplified fragments, which were quantitated usinga CCD image sensor (ChemiImager, Alpha Innotech). To determinethe linear range of PCR product accumulation, the results wereplotted on a semilogarithmic scale against the PCR cycle numberor on a logarithmic scale against the amount of template RNA usedin the reverse transcription reaction. On the basis of these results,subsequent RT-PCR analyses were performed using 15 ng total RNAwith PCR cycle numbers shown in the supplemental Table (availableat www.jneurosci.org). The intensity of the band from each genewas normalized to the intensity of the band from G3PDH. For thispurpose, the primers for G3PDH mRNA were added to the reactionmixture after some reactions to make its final PCR cycle numberto be 18. This normalized value was used to determine the relativeexpression level in eachgene.

Statistics. Data are presented as mean ± SEM except as noted. When statistical analysis was performed, one-factor ANOVA wasused to estimate the significance of the results. Statisticalsignificance was accepted at p < 0.05.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Microglial cells migrate to the outer retina during light-induced retinal degeneration

We first examined the distribution of microglial cells in normal and light-degenerated rat retinas at P35. In these experiments,we used a microglia-specific antibody that recognizes iba1, anew member of the EF hand family of proteins that are presenton resting as well as activated and phagocytic microglia (Graeberet al., 1998; Ito et al., 1998, 2001; Nakajima et al., 1998).Anti-iba1 recognizes microglial epitopes from a wide variety ofspecies and is suitable for double-labeling experiments in combinationwith monoclonal markers. In normal retina, iba1 immunoreactivitywas observed only in the inner part of the retina, such as theganglion cell layer (GCL) and the inner nuclear layer (INL) (Fig.1A). These immunostained cells are characteristic of "resting,"ramified microglia (Slepko and Levi, 1996). In light-reared retina,photoreceptor degeneration begins after P21, and approximatelyhalf of the photoreceptor nuclei disappear by P35 (Fig. 2A,B)(Harada et al., 1998a). In such light-degenerated retina, iba1immunoreactivity was observed in the outer as well as inner retina(Fig. 1D). Microglial cells in the outer retina appear to changetheir morphology during retinal degeneration (from having definedprocesses to a more amorphous/amoeboid shape). Thus, we next examinedwhether such amoeboid microglial cells are, in fact, "activated"(Slepko and Levi, 1996; Marin-Teva et al., 1998). For this purpose,we used a monoclonal antibody against ED1, an intracellular markerfor activated microglia in vivo (Graeber et al., 1990). In controlretina, all iba1-positive cells were ED1 negative (Fig. 1C, arrows).However, almost all microglial cells in the outer retina weredouble-labeled by iba1 and ED1 (Fig. 1F, arrowheads), althoughthose in the GCL and INL remained ED1 negative (arrows) in thelight-reared retina.

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Figure 1. Activation of microglia during light-induced retinal degeneration. A-F, Immunohistochemical analysis of normal (A-C) and light-reared (D-F) P35 rat retina using the antibodies iba1 (red in A, C, D, F) and ED1 (green in B, C, E, F). In light-degenerated retina, iba1 immunoreactivity was observed in the outer retina and double-labeled with ED1 (yellow) (F, arrowheads). G, Quantitative analysis of the ED1-positive cultured microglial cells from normal (red bar) and light-reared (green bar) P35 rat retina. Each data point represents the mean ± SEM of the values obtained from six independent experiments; *p < 0.05. H, I, Double-label immunocytochemistry of cultured microglial cells using the antibodies iba1 (red) and ED1 (green) from normal (H) and light-reared (I) P35 rat retina. GCL, Ganglion cell layer; INL, inner nuclear layer; ONL, outer nuclear layer. Scale bars, 30 µm.

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Figure 2. Gene expression of CNTF and GDNF receptors during light-induced retinal degeneration. A-C, Light micrograph of retinal sections taken from P35 rats raised under LD 12:12 (A), continuous illumination (B), or continuous illumination to P21 followed by LD 12:12 from P22 to P35 (C). Note the decreased photoreceptor cell number and ONL thickness in B. D, E, Representative data (D) and summary (E) of quantitative RT-PCR analysis using total RNA extracted from whole retina raised under LD 12:12 (black bar), continuous illumination (white bar), and continuous illumination to P21 followed by LD 12:12 from P22 to P35 (hatched bar). Each data point represents the mean ± SEM of the values obtained from six independent experiments. **p < 0.01; *p < 0.05. GCL, Ganglion cell layer; INL, inner nuclear layer; ONL, outer nuclear layer.

Effects of retinal degeneration on the production of trophic factors in microglia

To examine the function of microglia during retinal degeneration, we prepared pure cultured microglial cells from normal andlight-degenerated rat retina at P35. In culture, the number ofED1-positive microglia increases with time (Slepko and Levi, 1996).Interestingly, in our culture system the number of ED1-positivemicroglia (Fig. 1G) was greater in cultures from light-rearedretina (Fig. 1I) than in those from control retina (Fig. 1H).In addition, almost all of the cells analyzed were iba1 positive(>99%). Furthermore, by using the Müller cell-specific antibodyagainst GLAST, we determined that Müller glial cell contaminationwas negligible (data not shown). Using our cultured microglialcells, we examined whether retinal degeneration affects the expressionlevels of cytotoxic agents produced by these cells. Because nitricoxide produced by microglial cells may injure photoreceptors (Goureauet al., 1994; Cotinet et al., 1997), we examined gene expressionof iNOS using quantitative RT-PCR analysis. However, we foundthat the level of iNOS mRNA in microglia from degenerated retinaswas not significantly different from that of normal retinas (Table1). We next examined the effect of retinal degeneration on microgliawith respect to the expression of neurotrophic factors (Shimojoet al., 1991; Frade et al., 1998), which may stimulate photoreceptorsurvival during retinal degeneration (Faktorovich et al., 1990;LaVail et al., 1992; Cao et al., 1997; Fontaine et al., 1998).RT-PCR indicated that mRNA levels for NGF and NT-3, as well asCNTF and GDNF, were significantly increased in light-reared microgliarelative to normal microglia, although this was not the case forBDNF (Table 1). On the other hand, there was an unexpected decreasein bFGF mRNA (Table 1).


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Table 1. Quantification of mRNA productions in microglial cells

In a previous study, we found that exogenous NGF and NT-3 alter bFGF production in Müller glial cells, which act directlyon photoreceptor survival (Harada et al., 2000). To determinewhether mRNA upregulation of NGF and NT-3 in microglial cells(Table 1) really leads to protein upregulation, we examined proteinexpression levels in culture medium by ELISA. NGF protein expressionlevel in light-reared culture medium was upregulated to 138 ±9% (n = 18) compared with that in normal culture medium (p < 0.01).On the other hand, NT-3 protein expression was below detectablelevels in both normal and light-reared culturemedium.

We also examined GDNF and bFGF protein expression levels in culture medium. GDNF protein expression level in light-rearedculture medium was upregulated to 189 ± 23% (n = 24) comparedwith that in normal culture medium (p < 0.01). On the other hand,bFGF protein expression was slightly decreased (93 ± 3%; n = 18)(p < 0.05). These results are consistent with the data from quantitativeRT-PCR analysis (Table 1).

Photoreceptors express receptors for GDNF but not for CNTF in both normal and light-degenerated retina

Because microglial CNTF and GDNF expression is increased during retinal degeneration (Table 1), we examined receptor expressionlevels in whole retina. In light-reared P35 retina (Fig. 2B),the expression of CNTFR $alpha$ (241 ± 23%; n = 6), GFR $alpha$ 1 (140 ± 7%;n = 6), and GFR $alpha$ 2 (147 ± 17%; n = 6) was significantly upregulatedcompared with normal retina (Fig. 2A) reared under a 12 hr light/darkcycle (Fig. 2D,E). In addition, gp130 (134 ± 5%; n = 6) and LIFR $beta$ (179 ± 15%; n = 6) were also upregulated, but this was not thecase for Ret (124 ± 5%; n = 6) (data not shown). When rats wereraised under continuous illumination from P2 to P21, followedby LD 12:12 from P22 to P35, retinal degeneration did not progressafter P22 (Fig. 2C). Under such conditions, only CNTFR $alpha$ expressionwas upregulated (192 ± 26%; n = 6) compared with normal retinareared under LD 12:12 (Fig. 2D,E).

Because our data indicated that CNTF and GDNF receptors are upregulated in light-reared retina, we next determined whetherthese receptors are localized to photoreceptors. We assayed photoreceptor-specificgene expression of the receptors CNTFR $alpha$ , GFR $alpha$ 1, and GFR $alpha$ 2 usinglaser capture microdissection. For this purpose, total RNA wasextracted from cells residing in the ONL (Fig. 3A,B), which iscomposed of photoreceptor nuclei. However, we were unable to detectCNTFR $alpha$ gene expression in the ONL (Fig. 3C, lanes 2, 3), a resultthat is consistent with data from previous reports (Ugolini etal., 1995; Kirsch et al., 1997). In contrast, GDNF receptor geneswere detected in both normal and light-reared ONL (Fig. 3C) (Jinget al., 1996; Jomary et al., 1999). To assess the effect of retinaldegeneration on GFR $alpha$ 1/ $alpha$ 2 expression, we attempted to quantifyexpression levels in both normal and light-reared retina, butfound that levels were too low for accurate determination. Despitethis limitation of our data, these results suggest the possibilitythat microglia-derived GDNF, but not CNTF, has a direct effecton photoreceptor survival.

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Figure 3. Expression of CNTF and GDNF receptors in P35 rat photoreceptors. A, B, Cells residing in the ONL were extracted from normal (A) and light-reared (B) P35 rat retina using a laser-capture microdissection system and then processed for RT-PCR. C, RT-PCR analysis of whole retina (lane 1) or cells in the ONL from either the control (lane 2) or light-reared (lane 3) retina. GCL, Ganglion cell layer; INL, inner nuclear layer; ONL, outer nuclear layer.

Microglia-conditioned medium decreases bFGF production in Müller glial cells

We demonstrated previously that retinal degeneration increases the expression of low-affinity p75^NTR in retinal Müller glial cells, resulting in a decrease of bFGFproduction and photoreceptor apoptosis (Harada et al., 2000).In light of our results that suggest that microglia is a potentialsource of NGF (Table 1), we next examined the effect of microglia-conditionedmedium on bFGF expression in cultured Müller cells (Fig. 4A).As shown in Figure 4F, light-reared MCM (60 ± 15%; n = 3) butnot normal MCM (96 ± 14%; n = 3) caused a decrease in bFGF mRNAin Müller cells. This decrease was reversed by the addition ofa p75^NTR neutralizing antibody (111 ± 5%; n = 3), but not by a trk receptor-specificblocker (K252a) (37 ± 5%; n = 3) (data not shown). These resultssuggest that p75^NTR is involved in the regulation of bFGF expression in Müller cells.To test this hypothesis more definitively, we examined the effectof light-reared MCM on bFGF production in cultured Müller cellsfrom p75^NTR knock-out mice (Fig. 5A). As shown in Figure 5B, although light-rearedMCM significantly reduced bFGF expression in cultured Müllercells from control C57BL/6J mice (61 ± 9%; n = 3), no effect wasobserved in Müller cells from p75^NTR knock-out mice (109 ± 12%; n = 3). These results are consistentwith the idea that p75^NTR is involved in the control of bFGF production in Müller cellsand that a p75^NTR ligand (presumably NGF) reduces bFGF production.

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Figure 4. Effect of microglia-conditioned medium (MCM) on trophic factor expression in cultured Müller glial cells. A, Experimental protocol for examining the effect of MCM prepared from either normal or light-damaged P35 rat retina. Müller cells were incubated with MCM for 12 hr, and mRNA levels of trophic factors were determined by quantitative PT-PCR. B-G, RT-PCR analysis of NGF (B), BDNF (C), NT-3 (D), CNTF (E), bFGF (F), and GDNF (G). Note the upregulation of BDNF (C) and downregulation of bFGF (F) in Müller cells after incubation with light-reared MCM. Each data point represents the mean ± SEM of the values obtained from three independent experiments. *p < 0.01.

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Figure 5. Effect of microglia-conditioned medium (MCM) on bFGF expression in cultured Müller cells from p75^NTR knock-out mice. A, Experimental protocol for examining bFGF mRNA levels in Müller cells from wild-type (p75^+/+) and p75^NTR knock-out (p75^/) mice. Müller cells were incubated with MCM for 12 hr, and bFGF mRNA levels were determined by quantitative RT-PCR. B, RT-PCR analysis of bFGF. Note the stable bFGF expression levels in Müller cells from p75^NTR knock-out (p75^/) mice. Each data point represents the mean ± SEM of the values obtained from three independent experiments. *p < 0.01.

Microglia-conditioned medium increases BDNF production in Müller glial cells

We also examined the effect of MCM on the expression of other trophic factors in cultured Müller cells (Fig. 4A). Figure4C shows that BDNF mRNA increased in Müller cells when culturedwith light-reared MCM (151 ± 18%; n = 3) but not normal MCM (82± 6%; n = 3). However, such was not the case for NGF (Fig. 4B),NT-3 (Fig. 4D), CNTF (Fig. 4E), or GDNF (Fig. 4G). Because bothtrkB and p75^NTR are detected in Müller cells (von Bartheld, 1998; Harada etal., 2000), we next examined whether exogenous BDNF may alterthe expression of secondary trophic factors in cultured Müllercells (Table 2). After BDNF treatment, both CNTF and bFGF wereupregulated. However, given that CNTFR $alpha$ is absent from photoreceptors(Fig. 3C), we further examined the effect of exogenous CNTF onMüller cells after confirming that CNTFR $alpha$ was expressed in thesecells (data not shown). Surprisingly, CNTF treatment upregulatedBDNF as well as bFGF expression in Müller cells (Table 2). Becauseboth GFR $alpha$ 1 and GFR $alpha$ 2 genes were expressed in Müller cells (datanot shown), we also examined the effect of exogenous GDNF on Müllercells and found increased expression of BDNF, GDNF, and bFGF (Table2). These results suggest the possibility that microglia-derivedCNTF and GDNF may increase BDNF production in Müller cells, resulting,in turn, in bFGF upregulation in other Müller cells. Taken togetherwith the fact that GDNF receptors are expressed in photoreceptors(Fig. 3C), microglia-derived GDNF may act through both directand indirect pathways to rescue photoreceptors during light-inducedretinal degeneration.


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Table 2. Quantification of mRNA productions in Müller glial cells

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have shown that retinal degeneration transforms microglia from a resting state to one of "activation." Degenerating photoreceptorsinfluence the migration of microglia from the inner to the outerretina and alter trophic factor production in microglia that maysubsequently affect photoreceptor cell survival. Furthermore,microglia-derived factors influence the production of secondarytrophic factors in another retinal glial cell type, the Müllercell. As summarized in Figure 6, these findings suggest that functionalinteractions between microglia and Müller glial cells may bebidirectional and regulate photoreceptor cell survival duringretinal degeneration.

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Figure 6. Model for the microglia-Müller glia network in light-degenerated retina. Microglial cells constitutively release various agents that may affect surrounding retinal cells. In light-degenerated retina, reduced bFGF may induce photoreceptor apoptosis, but increased GDNF may directly rescue photoreceptors (middle). Microglia-derived GDNF and CNTF increase BDNF and bFGF, whereas BDNF increases CNTF and bFGF production in Müller cells, which may enhance photoreceptor rescue (right). On the other hand, microglia-derived NGF reduces bFGF production in Müller cells, which in turn may induce photoreceptor apoptosis (left).

Migration of microglia and microglia-derived factors during retinal degeneration

Prolonged or high-intensity exposure to visible light leads to photoreceptor cell apoptosis (Noell, 1980; Harada et al., 1996,1998a, 2000; Reme et al., 1998). However, exogenous BDNF, NT-3,CNTF, GDNF, and bFGF can delay this process (Faktorovich et al.,1990, 1992; LaVail et al., 1992, 1998; Cayouette et al., 1998;Chong et al., 1999; Frasson et al., 1999). Our present data suggestthat microglia represent a potential endogenous source of thesefactors (Table 2) and may be available for the protection ofphotoreceptors. Although microglia increase NGF and GDNF proteinproductions during retinal degeneration, the opposite is truefor bFGF. Similar results have been reported in studies with brainmicroglia (Araujo and Cotman, 1992). Release of bFGF from brainmicroglia is reduced by interleukin-3, epidermal growth factor(EGF), and NGF but is slightly augmented by $gamma$ -interferon. Togetherwith our present findings, these results suggest that under conditionssuch as trauma and neurodegeneration, in which there is an imbalancein these molecules, bFGF production in microglial cells may beadversely affected. In addition, the presence of bFGF receptorson photoreceptors (Fontaine et al., 1998) implies that endogenousbFGF release from microglia may serve diverse functions duringretinal degeneration. One important point is that the translationalproducts of bFGF mRNA lack a signal peptide sequence that wouldordinarily direct its secretion. Although it is not fully understood,many reports conclude that bFGF must somehow escape the cell andindicate mechanisms for bFGF secretion (von Heijne, 1983; Kurokawaet al., 1987; Sato and Rifkin, 1988; Klionsky et al., 1992; Mignattiet al., 1992; Florkiewicz et al., 1995; Piotrowicz et al., 1997;Dow and deVere White, 2000). We have determined previously thatthe production and secretion of bFGF by Müller cells can be regulatedby exogenous NGF and NT-3 (Harada et al., 2000).

In the present study, we also examined NGF and NT-3 protein release from microglia during photoreceptor degeneration. NGFprotein expression in culture medium of light-reared microgliawas higher than that of normal microglia, but NT-3 protein expressionwas below detectable levels in both normal and light-reared culturemedium. These results are consistent with the data that NGF mRNAexpression level was much higher than NT-3. The linear range ofPCR product accumulation was 22-26 cycles for NGF (data not shown),so quantification was done at 24 cycles (see supplemental Tableavailable at www.jneurosci.org). On the other hand, it was 32-35cycles for NT-3 (data not shown), and we needed 33 cycles forquantification (see supplemental Table available at www.jneurosci.org).These results suggest that our quantitative RT-PCR method is trulysensitive to small changes in mRNA levels (e.g., ~30% increasein NGF mRNA lead to ~40% increase in NGF protein), but NT-3 mRNAupregulation did not translate into increased release of NT-3protein from microglial cells in vitro. Because we measured onlyreleased NT-3 protein in culture medium, NT-3 protein productionin microglia might be upregulated during photoreceptor degeneration,but not released. Another possibility is that released NT-3 mighthave been consumed by an autocrinemechanism.

The microglia-Müller glia network as a trophic factor regulator during retinal degeneration

We demonstrated previously that trkC and p75^NTR are upregulated in Müller cells during retinal degeneration and that exogenousNT-3 increases bFGF production in Müller cells by activatingtrkC, whereas exogenous NGF decreases bFGF production by activatingp75^NTR (Harada et al., 2000). In this context, microglia-derived NT-3and NGF appear to function in opposition to each other. However,the concentration of microglia-released NGF is much higher thanthat of NT-3, and light-reared MCM decreases bFGF expression incultured Müller cells (Fig. 4F). In addition, light-reared MCMhad no effect on cultured Müller cells taken from p75^NTR knock-out mice (Fig. 5). These results suggest that the NGF pathwaypredominates over the NT-3 pathway during retinal degenerationin vivo. Frade et al. (1996) demonstrated previously that NGFcauses retinal apoptosis during development by activating p75^NTR. Subsequently, these workers identified microglia as the sourceof apoptotic NGF in the developing chick retina (Frade and Barde,1998). Together with our present findings, these results suggestthat activated microglia may also be the source of apoptotic NGFin the degenerating adult retina (Fig. 6).

BDNF and CNTF may stimulate photoreceptor survival via the microglia-Müller glia network (Fig. 6) because their appropriatereceptors are absent from photoreceptors (Fig. 3). In addition,microglia-derived GDNF may participate in both direct and indirectpathways for photoreceptor rescue. Interestingly, Müller cellstreated with GDNF exhibit increased expression of BDNF, bFGF,and GDNF (Table 2). Although enhanced expression of GDNF in responseto GDNF treatment may seem odd, a similar observation was reportedfor bFGF (Cao et al., 1997). We also found that exogenous bFGFupregulates bFGF mRNA (207 ± 16%; n = 6) in Müller cells (datanot shown). Furthermore, in Müller cells, BDNF treatment increasesCNTF expression, and vice versa (Table 2). Because the bindingof BDNF, CNTF, and GDNF to their receptors results in tyrosinephosphorylation of cellular substrates, microglia-Müller gliacell interactions may work as a regulator for these trophic factorsby using both paracrine and autocrine systems (Fig. 6).

One important issue is the sensitivity of LCM in detecting photoreceptor-specific trophic factor receptor mRNAs (Fig. 3).Although a recent study demonstrated trkB protein in cone photoreceptors(Di Polo et al., 2000), we could not identify trkB mRNA in photoreceptorsisolated by LCM (Harada et al., 2000). This suggests the possibilitythat our method is insufficient to identify trkB mRNA in conephotoreceptors. In this regard, we note that previous reportswere also unable to demonstrate trkB mRNA in photoreceptors byin situ hybridization (Jelsma et al., 1993; Perez and Caminos,1995; Gao et al., 1997; Suzuki et al., 1998; Rohrer et al., 1999).Rohrer et al. (1999) recently demonstrated that signaling pathsbetween trkB-expressing retinal cells (ganglion, amacrine, horizontal,retinal pigment epithelium, and Müller glial cells) and the photoreceptorsare required for normal photoreceptor development because photoreceptorsdo not normally express trkB receptors. Although we have to considerthe possibility that photoreceptors may express low levels oftrkB and CNTFR $alpha$ proteins, these results still support the importanceof the glia-neuron network in theretina.

Glia-glia and glia-neuron networks as a new therapeutic target for neurodegeneration

Activated microglial cells are observed in various pathological conditions caused by trauma and ischemia and are also involvedin pathophysiologies of the CNS, including Alzheimer's diseaseand AIDS (Kreutzberg, 1996; McGeer and McGeer, 1998; Stoll andJander, 1999; Le et al., 2001; Nakajima and Kohsaka, 2001). Migrationof microglia is thought to be regulated by various factors suchas extracellular pH (Faff and Nolte, 2000), nitric oxide (Chenet al., 2000), hepatocyte growth factor (Badie et al., 1999),EGF (Nolte et al., 1997), chemokines (Asensio et al., 1999; Crossand Woodroofe, 1999; Hesselgesser and Horuk, 1999; Maciejewski-Lenoiret al., 1999), and NMDA-induced degeneration (Heppner et al.,1998) to name a few. Thus, by controlling these factors throughintervention, microglial migration may be suppressed to an extentsufficient to prevent neural cell apoptosis in various neurologicaldiseases. However, at the same time, such strategies may inhibitthe direct neuroprotective effect by microglia-derived factors.Thus it is clear that further investigation is necessary to revealthe functional importance of microglial migration duringneurodegeneration.

Our present results suggest that although degeneration is a multicellular and multifactorial process, the functional glia-glianetwork may provide a new therapeutic target for the treatmentof neurodegeneration. The primary function of neurotrophic factorsis sustaining the viability of neurons, a process that is counterbalancedby a receptor mechanism that eliminates cells by apoptosis. Suchbidirectional control may be used selectively during developmentand neurodegenerative diseases (Yano and Chao, 2000). Thus, treatmentstrategies that reinforce survival pathways (Fig. 6, blue arrows)or weaken apoptotic pathways (Fig. 6, red arrows) may be usefulfor the prevention of neurodegenerative diseases. Because apoptoticcell death is the final common pathway for photoreceptors in allanimal models of retinitis pigmentosa and light-induced retinaldegeneration (Steele and O'Tousa, 1990; Chang et al., 1993; Portera-Cailliauet al., 1994; Papermaster and Windle, 1995; Reme et al., 1998;Travis, 1998; Alloway et al., 2000; Harada et al., 2000; Kiselevet al., 2000), the present results raise intriguing possibilitiesfor the management of these pathological conditions by controllingthe activity of the microglia-Müller glia-photoreceptornetwork.

  FOOTNOTES

Received Jan. 11, 2002; revised Aug. 5, 2002; accepted Aug. 7, 2002.

^* T.H. and C.H. contributed equally to thiswork.

This work was supported in part by grants from the Ministry of Health, Labour and Welfare of Japan, and the Ministry of Education,Culture, Sports, Science and Technology of Japan. T.H. was supportedby a Human Frontier Science Program long-term fellowship (LT00170/2001-B),and C.H. was supported by a Uehara Memorial Foundation postdoctoralfellowship. We thank M. Watanabe for providing the antibody toGLAST and L. F. Reichardt for providing the antibody to p75^NTR.

Correspondence should be addressed to Dr. Takayuki Harada, Department of Molecular Neuroscience, Medical Research Institute,Tokyo Medical and Dental University, 1-5-45 Yushima, Bunkyo-ku,Tokyo 113-8510, Japan. E-mail: harada.aud{at}mri.tmd.ac.jp.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Alloway PG, Howard L, Dolph PJ (2000) The formation of stable rhodopsin-arrestin complexes induces apoptosis and photoreceptor cell degeneration. Neuron 28:129-138[ISI][Medline].
Araujo DM, Cotman CW (1992) Basic FGF in astroglial, microglial, and neuronal cultures: characterization of binding sites and modulation of release by lymphokines and trophic factors. J Neurosci 12:1668-1678[Abstract].
Asensio VC, Lassmann S, Pagenstecher A, Steffensen SC, Henriksen SJ, Campbell IL (1999) C10 is a novel chemokine expressed in experimental inflammatory demyelinating disorders that promotes recruitment of macrophages to the central nervous system. Am J Pathol 154:1181-1191[Abstract/Free Full Text].
Badie B, Schartner J, Klaver J, Vorpahl J (1999) In vitro modulation of microglia motility by glioma cells is mediated by hepatocyte growth factor/scatter factor. Neurosurgery 44:1077-1083[ISI][Medline].
Baloh RH, Enomoto H, Johnson Jr EM, Milbrandt J (2000) The GDNF family ligands and receptors $---$ implications for neural development. Curr Opin Neurobiol 10:103-110[ISI][Medline].
Barbacid M (1994) The Trk family of neurotrophin receptors. J Neurobiol 25:1386-1403[ISI][Medline].
Bringmann A, Reichenbach A (2001) Role of Müller cells in retinal degenerations. Front Biosci 6:E72-92[Medline].
Cao W, Wen R, Li F, Cheng T, Steinberg RH (1997) Induction of basic fibroblast growth factor mRNA by basic fibroblast growth factor in Müller cells. Invest Ophthalmol Vis Sci 38:1358-1366[Abstract/Free Full Text].
Carwile ME, Culbert RB, Sturdivant RL, Kraft TW (1998) Rod outer segment maintenance is enhanced in the presence of bFGF, CNTF and GDNF. Exp Eye Res 66:791-805[ISI][Medline].
Cayouette M, Behn D, Sendtner M, Lachapelle P, Gravel C (1998) Intraocular gene transfer of ciliary neurotrophic factor prevents death and increases responsiveness of rod photoreceptors in the retinal degeneration slow mouse. J Neurosci 18:9282-9293[Abstract/Free Full Text].
Chang G-Q, Hao Y, Wong F (1993) Apoptosis: final common pathway of photoreceptor death in rd, rds, and rhodopsin mutant mice. Neuron 11:595-605[ISI][Medline].
Chen A, Kumar SM, Sahley CL, Muller KJ (2000) Nitric oxide influences injury-induced microglial migration and accumulation in the leech CNS. J Neurosci 20:1036-1043[Abstract/Free Full Text].
Chong NH, Alexander RA, Waters L, Barnett KC, Bird AC, Luthert PJ (1999) Repeated injections of a ciliary neurotrophic factor analogue leading to long-term photoreceptor survival in hereditary retinal degeneration. Invest Ophthalmol Vis Sci 40:1298-1305[Abstract/Free Full Text].
Cotinet A, Goureau O, Hicks D, Thillaye-Goldenberg B, de Kozak Y (1997) Tumor necrosis factor and nitric oxide production by retinal Müller glial cells from rats exhibiting inherited retinal dystrophy. Glia 20:59-69[ISI][Medline].
Cross AK, Woodroofe MN (1999) Chemokines induce migration and changes in actin polymerization in adult rat brain microglia and a human fetal microglial cell line in vitro. J Neurosci Res 55:17-23[ISI][Medline].
Davis S, Aldrich TH, Stahl N, Pan L, Taga T, Kishimoto T, Ip NY, Yancopoulos GD (1993) LIFR beta and gp130 as heterodimerizing signal transducers of the tripartite CNTF receptor. Science 260:1805-1808[Abstract/Free Full Text].
Di Polo A, Cheng L, Bray GM, Aguayo AJ (2000) Colocalization of TrkB and brain-derived neurotrophic factor proteins in green-red-sensitive cone outer segments. Invest Ophthalmol Vis Sci 41:4014-4021[Abstract/Free Full Text].
Dow JK, deVere White RW (2000) Fibroblast growth factor 2: its structure and property, paracrine function, tumor angiogenesis, and prostate-related mitogenic and oncogenic functions. Urology 55:800-806[ISI][Medline].
Faff L, Nolte C (2000) Extracellular acidification decreases the basal motility of cultured mouse microglia via the rearrangement of the actin cytoskeleton. Brain Res 853:22-31[ISI][Medline].
Faktorovich EG, Steinberg RH, Yasumura D, Matthes MT, LaVail MM (1990) Photoreceptor degeneration in inherited retinal dystrophy delayed by basic fibroblast growth factor. Nature 347:83-86[Medline].
Faktorovich EG, Steinberg RH, Yasumura D, Matthes MT, LaVail MM (1992) Basic fibroblast growth factor and local injury protect photoreceptors from light damage in the rat. J Neurosci 12:3554-3567[Abstract].
Florkiewicz RZ, Majack RA, Buechler RD, Florkiewicz E (1995) Quantitative export of FGF-2 occurs through an alternative, energy-dependent, non-ER/Golgi pathway. J Cell Physiol 162:388-399[ISI][Medline].
Fontaine V, Kinkl N, Sahel J, Dreyfus H, Hicks D (1998) Survival of purified rat photoreceptors in vitro is stimulated directly by fibroblast growth factor-2. J Neurosci 18:9662-9672[Abstract/Free Full Text].
Frade JM, Barde Y-A (1998) Microglia-derived nerve growth factor causes cell death in the developing retina. Neuron 20:35-41[ISI][Medline].
Frade JM, Rodriguez-Tebar A, Barde Y-A (1996) Induction of cell death by endogenous nerve growth factor through its p75 receptor. Nature 383:166-168[Medline].
Frasson M, Picaud S, Leveillard T, Simonutti M, Mohand-Said S, Dreyfus H, Hicks D, Sabel J (1999) Glial cell line-derived neurotrophic factor induces histologic and functional protection of rod photoreceptors in the rd/rd mouse. Invest Ophthalmol Vis Sci 40:2724-2734[Abstract/Free Full Text].
Gao H, Qiao X, Hefti F, Hollyfield JG, Knusel B (1997) Elevated mRNA expression of brain-derived neurotrophic factor in retinal ganglion cell layer after optic nerve injury. Invest Ophthalmol Vis Sci 38:1840-1847[Abstract/Free Full Text].
Goureau O, Hicks D, Courtois Y, de Kozak Y (1994) Induction and regulation of nitric oxide synthase in retinal Müller glial cells. J Neurochem 63:310-317[ISI][Medline].
Graeber MB, Streit WJ, Kiefer R, Schoen SW, Kreutzberg GW (1990) New expression of myelomonocytic antigens by microglia and perivascular cells following lethal motor neuron injury. J Neuroimmunol 27:121-132[ISI][Medline].
Graeber MB, Lopez-Redondo F, Ikoma E, Ishikawa M, Imai Y, Nakajima K, Kreutzberg GW, Kohsaka S (1998) The microglia/macrophage response in the neonatal rat facial nucleus following axotomy. Brain Res 813:241-253[ISI][Medline].
Harada T, Imaki J, Hagiwara M, Ohki K, Takamura M, Ohashi T, Matsuda H, Yoshida K (1995) Phosphorylation of CREB in rat retinal cells after focal retinal injury. Exp Eye Res 61:769-772[ISI][Medline].
Harada T, Imaki J, Ohki K, Ono K, Ohashi T, Matsuda H, Yoshida K (1996) Cone-associated c-fos gene expression in the light-damaged rat retina. Invest Ophthalmol Vis Sci 37:1250-1255[Abstract/Free Full Text].
Harada T, Harada C, Sekiguchi M, Wada K (1998a) Light-induced retinal degeneration suppresses developmental progression of flip-to-flop alternative splicing in GluR1. J Neurosci 18:3336-3343[Abstract/Free Full Text].
Harada T, Harada C, Watanabe M, Inoue Y, Sakagawa T, Nakayama N, Sasaki S, Okuyama S, Watase K, Wada K, Tanaka K (1998b) Functions of the two glutamate transporters GLAST and GLT-1 in the retina. Proc Natl Acad Sci USA 95:4663-4666[Abstract/Free Full Text].
Harada T, Harada C, Nakayama N, Okuyama S, Yoshida K, Kohsaka S, Matsuda H, Wada K (2000) Modification of glial-neuronal cell interactions prevents photoreceptor apoptosis during light-induced retinal degeneration. Neuron 26:533-541[ISI][Medline].
Harada T, Harada C, Mitamura Y, Akazawa C, Ohtsuka K, Ohno S, Takeuchi S, Wada K (2002) Neurotrophic factor receptors in epiretinal membranes after human diabetic retinopathy. Diabetes Care 25:1060-1065[Abstract/Free Full Text].
Heppner FL, Skutella T, Hailer NP, Haas D, Nitsch R (1998) Activated microglial cells migrate towards sites of excitotoxic neuronal injury inside organotypic hippocampal slice cultures. Eur J Neurosci 10:3284-3290[Medline].
Hesselgesser J, Horuk R (1999) Chemokine and chemokine receptor expression in the central nervous system. J Neurovirol 5:13-26[ISI][Medline].
Hicks D, Courtois Y (1990) The growth and behaviour of rat retinal Müller cells in vitro. 1. An improved method for isolation and culture. Exp Eye Res 51:119-129[ISI][Medline].
Ip NY, McClain J, Barrezueta NX, Aldrich TH, Pan L, Li Y, Wiegand SJ, Friedman B, Davis S, Yancopoulos GD (1993) The alpha component of the CNTF receptor is required for signaling and defines potential CNTF targets in the adult and during development. Neuron 10:89-102[ISI][Medline].
Ito D, Imai Y, Ohsawa K, Nakajima K, Fukuuchi Y, Kohsaka S (1998) Microglia-specific localisation of a novel calcium binding protein, Iba1. Mol Brain Res 57:1-9[Medline].
Ito D, Tanaka K, Suzuki S, Dembo T, Fukuuchi Y (2001) Enhanced expression of Iba1, ionized calcium-binding adapter molecule 1, after transient focal cerebral ischemia in rat brain. Stroke 32:1208-1215[Abstract/Free Full Text].
Jelsma TN, Friedman HH, Berkelaar M, Bray GM, Aguayo AJ (1993) Different forms of the neurotrophin receptor trkB mRNA predominate in rat retina and optic nerve. J Neurobiol 24:1207-1214[ISI][Medline].
Jing S, Wen D, Yu Y, Holst PL, Luo Y, Fang M, Tamir R, Antonio L, Hu Z, Cupples R, Louis JC, Hu S, Altrock BW, Fox GM (1996) GDNF-induced activation of the ret protein tyrosine kinase is mediated by GDNFR-alpha, a novel receptor for GDNF. Cell 85:1113-1124[ISI][Medline].
Jomary C, Thomas M, Grist J, Milbrandt J, Neal MJ, Jones SE (1999) Expression patterns of neurturin and its receptor components in developing and degenerative mouse retina. Invest Ophthalmol Vis Sci 40:568-574[Abstract/Free Full Text].
Ju WK, Lee MY, Hofmann HD, Kirsch M, Chun MH (1999) Expression of CNTF in Müller cells of the rat retina after pressure-induced ischemia. NeuroReport 10:419-422[ISI][Medline].
Kirsch M, Lee MY, Meyer V, Wiese A, Hofmann HD (1997) Evidence for multiple, local functions of ciliary neurotrophic factor (CNTF) in retinal development: expression of CNTF and its receptors and in vitro effects on target cells. J Neurochem 68:979-990[ISI][Medline].
Kiselev A, Socolich M, Vinos J, Hardy RW, Zuker CS, Ranganathan R (2000) A molecular pathway for light-dependent photoreceptor apoptosis in Drosophila. Neuron 28:139-152[ISI][Medline].
Klionsky DJ, Cueva R, Yaver DS (1992) Aminopeptidase I of Saccharomyces cerevisiae is localized to the vacuole independent of the secretory pathway. J Cell Biol 119:287-299[Abstract/Free Full Text].
Kreutzberg GW (1996) Microglia: a sensor for pathological events in the CNS. Trends Neurosci 19:312-318[ISI][Medline].
Kurokawa T, Sasada R, Iwane M, Igarashi K (1987) Cloning and expression of cDNA encoding human basic fibroblast growth factor. FEBS Lett 213:189-194[ISI][Medline].
LaVail MM, Unoki K, Yasumura D, Matthes MT, Yancopoulos GD, Steinberg RH (1992) Multiple growth factors, cytokines, and neurotrophins rescue photoreceptors from the damaging effects of constant light. Proc Natl Acad Sci USA 89:11249-11253[Abstract/Free Full Text].
LaVail MM, Yasumura D, Matthes MT, Lau-Villacorta C, Unoki K, Sung CH, Steinberg RH (1998) Protection of mouse photoreceptors by survival factors in retinal degenerations. Invest Ophthalmol Vis Sci 39:592-602[Abstract/Free Full Text].
Le WD, Rowe D, Xie W, Ortiz I, He Y, Appel SH (2001) Microglial activation and dopaminergic cell injury: an in vitro model relevant to Parkinson's disease. J Neurosci 21:8447-8455[Abstract/Free Full Text].
Maciejewski-Lenoir D, Chen S, Feng L, Maki R, Bacon KB (1999) Characterization of fractalkine in rat brain cells: migratory and activation signals for CX3CR-1-expressing microglia. J Immunol 163:1628-1635[Abstract/Free Full Text].
Marin-Teva JL, Almendros A, Calvente R, Cuadros MA, Navascues J (1998) Tangential migration of ameboid microglia in the developing quail retina: mechanism of migration and migratory behavior. Glia 22:31-52[Medline].
McGeer PL, McGeer ED (1998) Glial cell reactions in neurodegenerative diseases: pathophysiology and therapeutic interventions. Alzheimer Dis Assoc Disord 12[Suppl 2]:S1-6[ISI].
Mignatti P, Morimoto T, Rifkin DB (1992) Basic fibroblast growth factor, a protein devoid of secretory signal sequence, is released by cells via a pathway independent of the endoplasmic reticulum-Golgi complex. J Cell Physiol 151:81-93[ISI][Medline].
Nakajima K, Kohsaka S (2001) Microglia: activation and their significance in the central nervous system. J Biochem (Tokyo) 130:169-175[Abstract/Free Full Text].
Nakajima K, Kikuchi Y, Ikoma E, Honda S, Ishikawa M, Liu Y, Kohsaka S (1998) Neurotrophins regulate the function of cultured microglia. Glia 24:272-289[ISI][Medline].
Noell WK (1980) Possible mechanism of photoreceptor damage by light in mammalian eyes. Vision Res 20:1163-1171[ISI][Medline].
Nolte C, Kirchhoff F, Kettenmann H (1997) Epidermal growth factor is a motility factor for microglial cells in vitro: evidence for EGF receptor expression. Eur J Neurosci 9:1690-1698[ISI][Medline].
Papermaster DS, Windle J (1995) Death at an early age. Apoptosis in inherited retinal degenerations. Invest Ophthalmol Vis Sci 36:977-983[Free Full Text].
Perez MT, Caminos E (1995) Expression of brain-derived neurotrophic factor and of its functional receptor in neonatal and adult rat retina. Neurosci Lett 183:96-99[ISI][Medline].
Piotrowicz RS, Martin JL, Dillman WH, Levin EG (1997) The 27-kDa heat shock protein facilitates basic fibroblast growth factor release from endothelial cells. J Biol Chem 272:7042-7047[Abstract/Free Full Text].
Portera-Cailliau C, Sung C-H, Nathans J, Adler R (1994) Apoptotic photoreceptor cell death in mouse models of retinitis pigmentosa. Proc Natl Acad Sci USA 91:3273-3281.
Reme CE, Grimm C, Hafezi F, Marti A, Wenzel A (1998) Apoptotic cell death in retinal degenerations. Prog Retin Eye Res 17:443-464[ISI][Medline].
Rohrer B, Korenbrot JI, LaVail MM, Reichardt LF, Xu B (1999) Role of neurotrophin receptor TrkB in the maturation of rod photoreceptors and establishment of synaptic transmission to the inner retina. J Neurosci 19:8919-8930[Abstract/Free Full Text].
Roque RS, Caldwell RB (1993) Isolation and culture of retinal microglia. Exp Eye Res 12:285-290.
Roque RS, Imperial CJ, Caldwell RB (1996) Microglial cells invade the outer retina as photoreceptors degenerate in Royal College of Surgeons rats. Invest Ophthalmol Vis Sci 37:196-203[Abstract/Free Full Text].
Sato Y, Rifkin DB (1988) Autocrine activities of basic fibroblast growth factor: regulation of endothelial cell movement, plasminogen activator synthesis, and DNA synthesis. J Cell Biol 107:1199-1205[Abstract/Free Full Text].
Shimojo M, Nakajima K, Takei N, Hamanoue M, Kohsaka S (1991) Production of basic fibroblast growth factor in cultured rat brain microglia. Neurosci Lett 123:229-231[ISI][Medline]<