1. Introduction
A large body of experimental results from clinical and experimental studies has strongly suggested an aberrant activity of the immune system in glaucoma. The roles of the innate immune responses in glaucoma are unclear and have been controversial about the concept of neuroprotection or neurodestruction. Protective immunity has been suggested occurring as a homeostatic response to injury, which can prevent disease progression. Neurodegeneration of retinal ganglion cells (RGCs) may be the consequence from a failure of proper controls for the initial immune response right after injury in some glaucoma patients. Long-term tissue stress in glaucomatous eyes appears to be important for the balance between neuroprotective and neurodestructive immunity. The onset, progression, and termination of retinal specific immune responses are predominantly regulated by the interaction among the RGCs and different glia (astrocytes, Müller cells and microglia) in the glaucomatous eyes. As immunocompetent cell in the central nervous system (CNS), microglia have diverse phenotypes and produce beneficial or destructive factors depending on the microenvironments they encounter. In response to injury, activated microglia have been shown to trigger neuronal death by producing high levels of cytotoxic factors such as nitric oxide, superoxide and tumor necrosis factor-α (TNF-α). However, increasing lines of evidence have shown that microglia can elicit protective effects by releasing trophic and anti-inflammatory factors. To transform microglia into neuroprotective or neurodestructive depends on the disease state or the type of stimulus to trigger them into “classically activated” proinflammatory (M1) or “alternatively activated” anti-inflammatory (M2) cells (Polazzi and Monti, 2010).
2. Immunoregulation determines the fate of RGC in glaucoma
Glaucoma is an aging-associated neurodegenerative disease. In 2002, statistics gathered by WHO shows that glaucoma is the second leading cause of blindness worldwide, after cataract (Resnikoff et al., 2004). Glaucoma accounts for 12.3% of 37 million people affected by blindness, and 82% of which were 50 years or older. The number of glaucoma will increase to 79.6 million and the resulting blindness will increase to 11.1 million by 2020 (Quigley and Broman, 2006).Glaucoma results in irreversible loss of retinal ganglion cells (RGCs) and their axons, thus it is even a greater challenge than cataract for public health system. Therefore, investigation on potential neuroprotective agents is critical to prevent this blind leading visual impairment.
Glaucoma is defined as a group of optic neuropathies characterized by the irreversible loss of RGCs and their axons, accompanied by the excavation and degeneration of the optic nerve head (ONH) (Quigley, 1996). Elevated intraocular pressure (IOP)-related factors play an important role in initiation and progression of glaucoma. The glaucomatous neurodegeneration may be mediated via a combination of IOP-dependent compressive effects of the cribriform plates in the lamina cribosa on the axons of the RGCs, pressure-induced tissue ischemia, andvariouslocal cellular responses. The fate of RGCs may involve two or more cell stressors with additive or even synergistic effects. Increasing lines of evidence obtained from clinical and experimental studies strongly suggests diverse roles of the immunesystem in glaucoma as beneficial or destructive(Tezel, 2010, doi:10.1016/j.exer.2010.07.009).It is now commonly recognizedthatthere is an increased risks of failure in immune regulationunder glaucomatous stress conditions(Schwartz and Ziv, 2008; Wax and Tezel, 2009).
2.1. Autoimmune neurodegeneration in glaucoma
Autoimmune neurodegeneration results from a failure to properly rectify an aberrant and stress-induced immune response. Neuronal antigens can initiate immune responses by recruiting cytotoxic T cells. This occurs primarily in low tension glaucoma patients as evident by abnormal T cell subsets (Yang et al., 2001a).
Humoral immune response is also involved in the onset and the progression of neurodegeneration in some glaucoma patients. There is an increased prevalence of monoclonal gammopathy (Wax et al., 1994), elevated serum titers of auto-antibodies to optic nerve head glycosaminoglycans (Tezel et al., 1999), auto-antibodies to retinal antigen such as rhodopsin (Romano et al., 1995), small heat shock protein (Tezel et al., 1998; Tezel et al., 2004), glutathione S-transferase (Yang et al., 2001b), gamma-enolase (Maruyama et al., 2000) and phosphatidylserine (Kremmer et al., 2001). Immunoglobulin has also been detected in the glaucomatous retina (Wax et al., 1998a). Heat shock protein antibodies (e.g. hsp60, hsp27, and α-crystallins) have direct pathological potential to facilitate apoptotic RGC death in vitro and ex vivo(Tezel et al., 1998; Tezel and Wax, 1999, 2000). In addition, clinical findings show that serum titers of auto-antibodies to heat shock proteins were independent of the severity of glaucomatous damage (Wax et al., 2001). Antibody-mediated neuronal damage may occur indirectly by molecular mimicry of self-antigen from pathogen(Romano et al., 1995; Wax et al., 1998b; Romano et al., 1999). This is supported by the finding of elevated auto-antibodies to bacterial heat shock proteins, including hsp60 (Wax et al., 1998b), and the increased expressions of HLA-DR/CD8 circulating T cells in low tension glaucoma patients (Yang et al., 2001a). In addition, significant alterations of serum Th1 and Th2 cytokines are detected, suggesting abbreant immune responsesof glaucomatous neuropathy(Huang et al., 2010).
2.2. Neuroprotective immune response – involvement of retinal microglia
Protective immunity has been suggested to occur as a homeostatic response to injury with the intent of preventing disease progression (Schwartz, 2007). The most important sites for immune modulation in glaucoma are retina and the optic nerve, which are thought to have an actively regulated immune privilege mechanism(Forrester, 2009). As the major immunocompetent cells in the CNS, the principal function of microglia is the quick response to thepresence of pathogens and to CNS damage.In both human glaucomatous eye samples and animal models, the involvement of microglia in glaucoma has been reported(Schwartz et al., 2006). In human glaucomatous ocular specimens, microglia in the ONH and the parapapillary chorioretinal region of the ONH are activated and redistributed (Neufeld, 1999). In rat glaucoma model induced by cauterization, microglia in retinas exposed to chronic ocular hypertension appear as early as three days and last for about two months after IOP elevation (Wang et al., 2000; Naskar et al., 2002). Whether these retinal microglia play a protective or cytotoxic role in glaucoma deserve further investigation.
The balance between beneficial and deleterious immune responses is a critical issue for the treatment of neurodegenerative diseases. The use of immune-modulation drugs which are able to shift the immune response towards neuroprotection will be an effective therapeutic approach. As an FDA-approved drug for multiple sclerosis, glatiramer acetate (GA), also known as Copolymer-1 (Cop-1), was used as a treatment for autoimmune diseases and as a therapeutic vaccine for neurodegenerative diseases (Polazzi and Monti, 2010). GA is a synthetic oligopeptide of four naturally occurring amino acids, its activity derives from its ability to serve as a “universal antigen’that weakly activates a wide spectrum of self-reactive T-cells (Kipnis and Schwartz, 2002). T-cell-based vaccination with GA resulted in decreased plaque formation, reduction of excitotoxicity and induction of neurogenesis in Alzheimer’s disease (AD) mouse model (Butovsky et al., 2006a; 2006b). This GA vaccination caused a phenotype switch in brain microglia to dendritic-like morphology, with the ability to produce insulin-like growth factor 1 (IGF-1) that counteracted the adverse Aβ-induced effects (Butovsky et al., 2006a; 2006b; 2007). Vaccination with GA significantly reduces loss of RGCs in rodent models of optic nerve crush injury, intraocular glutamate toxicity,glaucoma and macular degeneration(Schori et al., 2001). These results suggest that GA induced recruitment of dendritic-like microglia from bone marrow might contribute significantly to the anti-neurodegenerative effect. Vaccination has the impact on the entire body, how about using other immune-modulation drugs locally? Our laboratory has investigated the modulation of retinal microglia in a rat glaucoma model through intravitreous application of chemokine, monocyte chemoattractant protein-1 (MCP-1)(Chiu et al., 2010a). Furthermore, we also tested the involvement of retinal microglial cells in this glaucoma model which oral application of herbal medicine wolfberry polysaccharides have proved to be neuroprotective (Chan et al., 2007; Chiu et al., 2009). Our data showed that when the retinal microglia was tune to a neuroprotective state, named as police-state, there was a positive correlation with an increase in RGC survival under ocular hypertension (Chang et al., 2009).
3. Diverse activation of retinal microglia associated with divergent effects on retinal ganglion cell survival under chronic ocular hypertension (COH)
In the normal mature brain, microglia typically exist in a resting state that is highly ramified. In contrast to their non-moving cell body, processes of the “resting” microglia display high mobility, especially extension and retraction (Davalos et al., 2005). The brain microglia perform tissue surveillance and can patrol the entire neural parenchyma every few hours (Nimmerjahn et al., 2005). Use of Z-stack mode by multiphoton to scan different layers of retina from the nerve fiber layer to the outer segment on whole mounted retina allows us to observe the morphology of the resting state microglia. Similar to other reports in the brain, the resting microglia in the normal rat retina are highly ramified shape with small nuclei and long thin processes and was located in the inner retina with almost no overlapping of processes (diameter: ~50 μm, scattered throughout the retinal ganglion cell layer and the inner plexiform layer). They may also play a surveillance role in the retina(Chang et al., 2009; Chiu et al., 2009).
Upon activation, microglia emerged from a resting state and underwent morphological transformation from ramified to different activated forms, such as dendritic or amoeboid. Microglia constitute a family of cells with diverse phenotypes, some are beneficial and others are detrimental to surrounding cells (Schwartz et al., 2006). Like macrophages, microglia can exhibit different activated phenotypes: “classically activated” proinflammatory (M1) or “alternatively activated” anti-inflammatory (M2) (Benoit et al., 2008; Geissmann et al., 2008; Kigerl et al., 2009; Polazzi and Monti, 2010).
Although it has been shown that it is possible to manipulate the activation state of microglia in vitro so that their activation can be beneficial - protecting rather than destroying neurons(Polazzi et al., 2001; 2009). It is difficult to achieve this goal in vivo, especially in chronic neurodegenerative model. Our group managed to use a chronic ocular hypertension (COH) model to mimic glaucoma in rats. We tested differential activation of microglia in the retina under COH and their co-relationship with RGC survival in this chronic neurodegenerative model.
Adult female Sprague-Dawley (SD) rats (250-280 g) were grouped and used. Ocular hypertension (OH) was induced in the right eye of each animal using laser photocoagulation according to our previous publications(Chan et al., 2007; Chiu et al., 2007; Chiu et al., 2009; Chiu et al., 2010a; Chiu et al., 2010b). Schematic diagram (Fig. 1) shows the front and back view of laser photocoagulation applied (indicated as red spots) to the limbal veins (front veiw) and the three episcleral veins (two at the superior and one at the inferior quadrant, back view).After two weeks of laser photocoagulation, the limbal veins were replaced by scar tissue and could not be seen in the limbal area except the nasal 90 degrees where no laser photocoagulation was applied. The corneas of the OH eyes were healthy and transparent, with no neovascularization existed. The OH eyes were free of infection, cataract, intraocular bleeding or retinal detachment.
Photocoagulation using the argon laser increased the IOP of the righteyes (OH eyes) from the baseline around 15 mmHg to 22 mmHg for up to one month. There was significant loss of RGCs in the experimental eyes starting at 2 weeks after the first laser treatment. The density of RGCs was decreased from 2,241 to 1,964/mm2 (#P = 0.002), this loss was only about 17% of total RGC in normal retina at one month after the first laser(Luo et al., 2009).Since ocular hypertension is not an acute injury causing massive neuronal death, microglia in the glaucomatous retina were not activated as they were in the optic nerve axotomy model. The microglia detected in the inner retina of the OH eyes were in resting state under elevated IOP (Luo et al., 2009). The morphology of iba-1 positive microglia in the cross retinal sections was similar with the ramified one in the Naskar et al. (2002) study. The resting state morphology of microglia was also supported by Lam et al. (2003) in which they could not detect the phagocytic microglia in glaucomatous retina by using ED1 immunohistochemical staining. The microglial responses in this laser photocoagulation-induced COH model are similar to the situation in human glaucomatous retina where activated microglia are detected in the ONH and the parapapillary chorioretinal region of the ONH, where this region is not considered to be retina. Therefore, this model provides a good opportunity for us to investigate different morphologies of microglia modulated by different factors.
3.1. Classical activation of retinal microglia is detrimental to RGC under COH
Conventional stimulation of microglia/macrophages by classical pathogens such as bacterialendotoxin lipopolysaccharide (LPS) or zymogen can be neurodestructive, becausemassive production of free-radicals triggered by these stimulican induce both apoptosis and necrosis of neurons.Activated microglia have been considered to be endogenous malefactors in the CNS because they play important roles in neurological diseases such as Alzheimer’s disease and amyotrophiclateral sclerosis (Sargsyan, et al., 2005). In response to injury, activated microglia have been shown to induce neuronal death by releasing excess cytotoxic factors such as superoxide (Lee, et al., 1993; Block, et al., 2007), nitric oxide (NO) and tumor necrosis factor-α (TNF-α) (Chang, et al., 2000a; 2000b; Colton and Gilbert, 1987).This kind ofstimulation can eventually result in activation-induced celldeath depleting the pool of these innate immune cells in theCNS. This is similar to the stimulation of LPS applied to the macrophages in vitro. LPS promotes the differentiation of “classically activated” M1 macrophages. These M1 macrophages secrete high levels of pro-inflammatory cytokines, release oxidative metabolites such as superoxide radicals (O2-) and NO, and reduce production of neurotrophic factor (Benoit et al., 2008; Geissmann et al., 2008; Kigerl et al., 2009; Polazzi and Monti, 2010). Therefore, conventional stimulation of microglia/macrophages not only produces cytotoxic pro-inflammatoryfactors, but also depletes the pool of the innate immune cellsto elicit possible neuroprotective effects.
In this COH model, a single intravitreous injection of 50 μgof LPS or MCP-1 1000 nggreatly alerted microglia to transform themselves from a resting state to a fully activated state in the glaucomatous eye up to four weeks under ocular hypertension (Chiu et al., 2010). The immunoreactivity of iba-1 in the microglia was dramatically increased. The microglia displayed enlarged nuclei and remarkably thick and short processes. With marked increase in the number of processes, their short processes displayed overlapping. Concomitantly, fully activated microglia were found in the nerve fiber layer and retinal ganglion cell layer corresponding to the area of retinal injury in animals with ocular hypertension. RGC loss was significantly increased from 17.4% in PB control OH retina to 28.3% in LPS group (# p=0.007). The increased RGC death should not be due to direct neurotoxic effect of LPS as it has been shown that LPS did not exert direct neurotoxicity (Bronstein et al., 1995).Dysregulated responses or over-activation of microglia is considered to be destructive and dangerous for neighboring neurons because of the harmful effects of free-radicals produced by fully activated microglia (Ladeby et al., 2005; Block et al., 2007).
3.2. Restricted activation of microglia is neuroprotective to RGC under COH
In contrast to conventional stimulation, activation ofmicroglia/macrophages can be modulated by the cytokinessecreted by infiltrated T-lymphocytes, or the local CNSenvironment, which is named as restricted (appropriate)stimulation. Immune suppressive cytokines that released from CD4+/CD25+ regulatoryT cells or Th2 cells, such as IL-4, IL-10 or TGF-β canmarkedly modulate the activation state of microglia/macrophages(Kipnis et al., 2004). The macrophages are at an “alternative activated” M2 phenotype. These M2 macrophages promote angiogenesis, matrix remodeling and suppress destructive immunity (Sica et al., 2006).
MCP-1/CCL2 is a β-chemokine involved in the activation and recruitment of monocytic cells to injury sites (Zhang and Koninck, 2006). MCP-1/CCL2 can either induce neuroprotection or neurodestruction depending on the experimental model (Galasso et al., 2000; Eugenin et al., 2003; Kalehua et al., 2004). Using MCP-1/CCL2, the activation states of microgliacan be manipulated, they can exert divergent effects on RGC survival under COH. Our results demonstrated different morphologies of microglia, which are correlated to the severityof neuronal loss in an experimental rat glaucoma model. Compared to fully activated state of microglia in the retina (1000 ng MCP-1), a unique semi-activated phenotype of microglia was found in the 10/100 ngMCP-1 group(s) (Chiu et al., 2010). The nuclei were slightly enlarged and processes of microglia were significantly shortened with moderate thickening, and there was no overlapping of processes. Concomitant to the changes in microglial morphology, RGC loss appeared to be correlated with the activation status of microglia. Two weeks after the first laser, OH with intravitreous injection of PB resulted in 17.4% RGC loss. Injection of 10 ng of MCP-1 decreased the RGC loss to 10.3%, and 100 ng of MCP-1 significantly reduced RGC loss to 3.4% (** p<0.001, MCP-1 100 ng vs. PB).Further increase of MCP-1 to 1000 ng did not decrease but significantly increased RGC loss to 21.2%. At one month after the first laser treatment, compared to the PB control,MCP-1 100 ng significantly reduced RGC loss from 19.1% to 5.1% (* p<0.001).
The protective effects of microglia can be accomplished by producing neurotrophic molecules such as IGF-1 (Streit, 2005; Butovsky, et al., 2006a). Previous brain ischemia studies have shown that activated microglia can produce neurotrophic molecules such as IGF-1 (O'Donnell et al., 2002; Butovsky et al., 2006a; Lalancette-Hebert et al., 2007). Our study showed that after four weeks under COH, IGF-1 immunoreactivity was markedly reduced in the retinas with PB. In the 100 ng MCP-1-treated group, the immunoreactivity of IGF-1 was up-regulated and restored to normal level.
Similar phenomenon is also observed in oral feeding of herbal medicine, wolfberry polysaccharides, in this model (Chiu et al., 2009). One to 100 mg/kg LBP exertedthe best neuroprotection and elicited moderately activatedmicroglia in the inner retina with ramified appearance butthicker and focally enlarged processes.When activationof microglia was attenuated by intravitreous injection ofmacrophage/microglia inhibitory factor (MIF), protective effect of10 mg/kg LBP was attenuated. Therefore, restricted activation of microglia under ocular hypertension is neuroprotective to the survival of RGCs.
4. Conclusion
Taken together, it is the time for us to reconsider how to categorize the activation state of microglia(Chang et al., 2009). First, theresting state with lots of processes and small size of cell bodyin morphology; second, the semi-activated state (police state or M2 phenotype) with thick and shortprocesses and large size of cell body; third, the fully activated state(army state or M1 phenotype) with very thick processes and very large size of cell bodywith sometimes amoeboid shape. The army state of microglia can produce free-radicalsincluding nitric oxide, superoxide and different pro-inflammatorycytokines. In contrast,the police state of microgliacan produce trophic factor without releasing free-radicals. While resting microglia can be consideredto be a securityguard for immune surveillance, semi-activated (M2 activated) microglia canbe regarded as a police officer to prevent any bad situation forfurther neuroinflammation and to protect citizen neuronswithout miss-firing by-stander neurons, and fully activated(M1 activated) microglia can function as army responsible to fight in a battle.Nevertheless, the by-stander neurons will be damagedunavoidably.
Our findings using the COH model, demonstrate a distinct morphology of microgliain response to neuroprotective dose of MCP-1/CCL2, and wolfberry. Definition of thisdistinct morphology will help future studies to understand the biologicalmechanisms of neuroprotective microglia, opening up a newavenue of manipulating microglia to elicit neuroprotective effects inneurodegeneration.
Acknowledgments
The work done by this laboratory has been or is currentlysupported by The Glaucoma Foundation, USA; AmericanHealth Assistant Foundation, USA; HKU Alzheimer’sDisease Research Network under Strategic Theme Researchon Healthy Aging; University Strategic Research Theme onDrug Discovery; Research Fund for the Control of InfectiousDiseases (09080822) from Food and Health Bureau of HongKong SAR Government; General Research Fund (761609M) from Research Grant Council; Azalea (1972) Endowment Fund, HKUSeed Funding for Basic Research (201011159058), and HKU Small Project Funding (200907176185).
References
- 1.
Benoit M. Desnues B. Mege-L J. 2008 Macrophage Polarization in Bacterial Infections. The Journal of Immunology181 3733 3739 - 2.
Block M. L. Zecca L. Hong J. S. 2007 Microglia-mediated neurotoxicity: uncovering the molecular mechanisms. Nature Reviews Neuroscience8 57 69 - 3.
Bronstein D. M. Perez-Otano I. Sun V. Mullis Sawin. S. B. Chan J. Wu G. C. Hudson P. M. Kong L. Y. Hong J. S. Mc Millian M. K. 1995 Glia-dependent neurotoxicity and neuroprotection in mesencephalic cultures. Brain Res704 112 116 - 4.
Butovsky O. Koronyo-Hamaoui M. Kunis G. Ophir E. Landa G. Cohen H. Schwartz M. 2006a From the Cover: Glatiramer acetate fights against Alzheimer’s disease by inducing dendritic-like microglia expressing insulin-like growth factor 1. Proc Natl Acad Sci U S A103 11784 11789 - 5.
Butovsky O. Kunis G. Koronyo-Hamaoui M. Schwartz M. 2007 Selective ablation of bone marrow-derived dendritic cells increases amyloid plaques in a mouse Alzheimer’s disease model. Eur J Neurosci26 413 416 - 6.
Butovsky O. Landa G. Kunis G. Ziv Y. Avidan H. Greenberg N. Schwartz A. Smirnov I. Pollack A. Jung S. Schwartz M. 2006b Induction and blockage of oligodendrogenesis by differently activated microglia in an animal model of multiple sclerosis. J Clin Invest116 905 915 - 7.
Chan H. C. Chang R. C. C. Ip A. K. C. Chiu K. Yuen W. H. Zee S. Y. So K. F. 2007 Neuroprotective effects of Lycium barbarum Lynn on protecting retinal ganglion cells in an ocular hypertension model of glaucoma. Exp Neurol203 269 273 - 8.
Chang R. C. C. Chiu K. Ho Y. S. So K. F. 2009 Modulation of Neuroimmune Responses on Glia in the Central Nervous System: Implication in Therapeutic Intervention against Neuroinflammation. Cellular & Molecular Immunology6 317 326 - 9.
Chiu K. Chan H. C. Yeung S. C. Yuen W. H. Zee S. Y. Chang R. C. C. So K. F. 2009 Modulation of microglia by Wolfberry on the survival of retinal ganglion cells in a rat ocular hypertension model J Ocul Biol Dis Inform2 127 136 - 10.
Chiu K. Chang R. C. C. So K. F. 2007 Laser induced rat chronic ocular hypertension model. Journal of Visualized Experiments10: - 11.
Chiu K. Yeung S. C. So K. F. Chang R. C. C. 2010a Modulation of morphological changes of microglia and neuroprotection by monocyte chemoattractant protein-1 in experimental glaucoma. Cellular & Molecular Immunology7 61 68 - 12.
Chiu K. Zhou Y. Yeung S. C. Lok C. K. M. Chan O. O. C. Chang R. C. C. So K. F. Chiu J. F. 2010b Up-Regulation of Crystallins is Involved in the Neuroprotective Effect of Wolfberry on Survival of Retinal Ganglion Cells in Rat Ocular Hypertension Model. J Cell Biochem110 311 320 - 13.
Davalos D. Grutzendler J. Yang G. Kim J. V. Zuo Y. Jung S. Littman D. R. Dustin M. L. Gan W. B. 2005 ATP mediates rapid microglial response to local brain injury in vivo. Nat Neurosci8 752 758 - 14.
Eugenin E. A. D’Aversa T. G. Lopez L. Calderon T. M. Berman J. W. 2003 MCP-1 (CCL2) protects human neurons and astrocytes from NMDA or HIV-tat-induced apoptosis. J Neurochem85 1299 1311 - 15.
Forrester JV. 2009 Privilege revisited: an evaluation of the eye’s defence mechanisms. Eye23 756 766 - 16.
Galasso J. M. Liu Y. Szaflarski J. Warren J. S. Silverstein F. S. 2000 Monocyte chemoattractant protein-1 is a mediator of acute excitotoxic injury in neonatal rat brain. Neuroscience101 737 744 - 17.
Geissmann F. Auffray C. Palframan R. Wirrig C. Ciocca A. Campisi L. Narni-Mancinelli E. Lauvau G. 2008 Blood monocytes: distinct subsets, how they relate to dendritic cells, and their possible roles in the regulation of T-cell responses. Immunol Cell Biol86 398 408 - 18.
Huang P. Qi Y. Xu Y. S. Liu J. H. Liao D. P. Zhang S. S. M. Zhang C. 2010 Serum Cytokine Alteration is Associated With Optic Neuropathy in Human Primary Open Angle Glaucoma. J Glaucoma19 324 330 - 19.
Kalehua AN, Nagel JE, Whelchel LM, Gides JJ, Pyle RS, Smith RJ, Kusiak JW, Taub DD. 2004 Monocyte chemoattractant protein-1 and macrophage inflammatory protein-2 are involved in both excitotoxin-induced neurodegeneration and regeneration. Exp Cell Res297 197 211 - 20.
Kigerl KA, Gensel JC, Ankeny DP, Alexander JK, Donnelly DJ, Popovich PG. 2009 Identification of Two Distinct Macrophage Subsets with Divergent Effects Causing either Neurotoxicity or Regeneration in the Injured Mouse Spinal Cord. The Journal of Neuroscience29 13435 13444 - 21.
Kipnis J. Avidan H. Caspi R. R. Schwartz M. 2004 Dual effect of CD4(+)CD25(+) regulatory T cells in neurodegeneration: A dialogue with microglia. Proc Natl Acad Sci U S A101 14663 14669 - 22.
Kipnis J. Schwartz M. 2002 Dual action of glatiramer acetate (Cop-1) in the treatment of CNS autoimmune and neurodegenerative disorders. Trends in Molecular Medicine8 319 323 - 23.
Kremmer S. Kreuzfelder E. Klein R. Bontke N. Henneberg-Quester K. B. Steuhl K. P. Grosse-Wilde H. 2001 Antiphosphatidylserine antibodies are elevated in normal tension glaucoma. Clin Exp Immunol125 211 215 - 24.
Ladeby R. Wirenfeldt M. Garcia-Ovejero D. Fenger C. Dissing-Olesen L. Dahnau I. Finsen B. 2005 Microglial cell population dynamics in the injured adult central nervous system. Brain Research Reviews48 196 206 - 25.
Lalancette-Hebert M. Gowing G. Simard A. Weng Y. C. Kriz J. 2007 Selective ablation of proliferating microglial cells exacerbates ischemic injury in the brain. J Neurosci27 2596 2605 - 26.
Lam TT, Kwong JMK, Tso MOM. 2003 Early glial responses after acute elevated intraocular pressure in rats. Invest Ophthalmol Vis Sci44 638 645 - 27.
Luo X. G. Chiu K. Lau F. H. S. Lee V. W. H. Yung K. K. L. So K. F. 2009 The Selective Vulnerability of Retinal Ganglion Cells in Rat Chronic Ocular Hypertension Model at Early Phase. Cell Mol Neurobiol29 1143 1151 - 28.
Maruyama I. Ohguro H. Ikeda Y. 2000 Retinal ganglion cells recognised by serum autoantibody against gamma-enolase found in glaucoma patients. Invest Ophthalmol Vis Sci41 1657 1665 - 29.
Naskar R. Wissing M. Thanos S. 2002 Detection of early neuron degeneration and accompanying microglial responses in the retina of a rat model of glaucoma. Invest Ophthalmol Vis Sci43 2962 2968 - 30.
Neufeld AH. 1999 Microglia in the optic nerve head and the region of parapapillary chorioretinal atrophy in glaucoma. Arch Ophthalmol117 1050 1056 - 31.
Nimmerjahn A. Kirchhoff F. Helmchen F. 2005 Resting microglial cells are highly dynamic surveillants of brain parenchyma in vivo. Science308 1314 1318 - 32.
O’Donnell SL, Frederick TJ, Krady JK, Vannucci SJ, Wood TL. 2002 IGF-I and microglia/macrophage proliferation in the ischemic mouse brain. Glia39 85 97 - 33.
Polazzi E. Altamira L. E. P. Eleuteri S. Barbaro R. Casadio C. Contestabile A. Monti B. 2009 Neuroprotection of microglial conditioned medium on 6-hydroxydopamine- induced neuronal death: Role of transforming growth factor beta-2. J Neurochem110 545 556 - 34.
Polazzi E. Gianni T. Contestabile A. 2001 Microglial cells protect cerebellar granule neurons from apoptosis: Evidence for reciprocal signaling. Glia36 271 280 - 35.
Polazzi E. Monti B. 2010 Microglia and neuroprotection: From in vitro studies to therapeutic applications. Prog Neurobiol92 293 315 - 36.
Quigley HA. 1996 Number of people with glaucoma worldwide. Br J Ophthalmol80 389 393 - 37.
Resnikoff S. Pascolini D. Etya’ale D. Kocur I. Pararajasegaram R. Pokharel G. P. Mariotti S. P. 2004 Global data on visual impairment in the year 2002.. Bull World Health Organ82 844 851 - 38.
Romano C. Barrett D. A. Li Z. Z. Pestronk A. Wax M. B. 1995 Anti-rhodopsin antibodies in sera from patients with normal-pressure glaucoma. Invest Ophthalmol Vis Sci36 1968 1975 - 39.
Romano C. Li Z. Z. Arendt A. Hargrave P. A. Wax M. B. 1999 Epitope mapping of anti-rhodopsin antibodies from patients with normal pressure glaucoma. Invest Ophthalmol Vis Sci40 1275 1280 - 40.
Schori H. Kipnis J. Yoles E. Wolde Mussie. E. Ruiz G. Wheeler L. A. Schwartz M. 2001 Vaccination for protection of retinal ganglion cells against death from glutamate cytotoxicity and ocular hypertension: Implications for glaucoma. Proc Natl Acad Sci U S A98 3398 3403 - 41.
Schwartz M. 2007 Modulating the immune system: a vaccine for glaucoma? Can J Ophthalmol42 439 441 - 42.
Schwartz M. Butovsky O. Bruck W. Hanisch U. K. 2006 Microglial phenotype: is the commitment reversible? Trends Neurosci29 68 74 - 43.
Schwartz M. Ziv Y. 2008 Immunity to self and self-maintenance: a unified theory of brain pathologies. Trends in Immunology29 211 219 - 44.
Sica A. Schioppa T. Mantovani A. Allavena P. 2006 Tumour-associated macrophages are a distinct M2 polarised population promoting tumour progression: Potential targets of anti-cancer therapy. Eur J Cancer42 717 727 - 45.
Tezel G. 2010 The immune response in glaucoma: A perspective on the roles of oxidative stress. Exp Eye Res In Press, Corrected Proof.doi:10.1016/j.exer.2010.07.009. - 46.
Tezel G. Edward D. P. Wax M. B. 1999 Serum autoantibodies to optic nerve head glycosaminoglycans in patients with glaucoma. Arch Ophthalmol117 917 924 - 47.
Tezel G. Seigel G. M. Wax M. B. 1998 Autoantibodies to small heat shock proteins in glaucoma. Invest Ophthalmol Vis Sci39 2277 2287 - 48.
Tezel G. Wax M. B. 1999 Inhibition of caspase activity in retinal cell apoptosis induced by various stimuli in vitro. Invest Ophthalmol Vis Sci40 2660 2667 - 49.
Tezel G. Wax M. B. 2000 The mechanisms of hsp27 antibody-mediated apoptosis in retinal neuronal cells. J Neurosci20 3552 3562 - 50.
Tezel G. Yang J. J. Wax M. B. 2004 Heat shock proteins, immunity and glaucoma. Brain Res Bull62 473 480 - 51.
Wang X. Tay S. S. W. Ng Y. K. 2000 An immunohistochemical study of neuronal and glial cell reactions in retinae of rats with experimental glaucoma. Exp Brain Res132 476 484 - 52.
Wax M. B. Barrett D. A. Pestronk A. 1994 Increased incidence of paraproteinemia and autoantibodies in patients with normal-pressure glaucoma. Am J Ophthalmol117 561 568 - 53.
Wax M. B. Tezel G. 2009 Immunoregulation of retinal ganglion cell fate in glaucoma. Exp Eye Res88 825 830 - 54.
Wax M. B. Tezel G. Edward P. D. 1998a Clinical and ocular histopathological findings in a patient with normal-pressure glaucoma. Arch Ophthalmol116 993 1001 - 55.
Wax M. B. Tezel G. Kawase K. Kitazawa Y. 2001 Serum autoantibodies to heat shock proteins in glaucoma patients from Japan and the United States. Ophthalmology108 296 302 - 56.
Wax M. B. Tezel G. Saito I. Gupta R. S. Harley J. B. Li Z. Z. Romano C. 1998b Anti-Ro/SS-A positivity and heat shock protein antibodies in patients with normal-pressure glaucoma. Am J Ophthalmol125 145 157 - 57.
Yang J. J. Patil R. V. Yu H. Gordon M. Wax M. B. 2001a T cell subsets and sIL-2R/IL-2 levels in patients with glaucoma. Am J Ophthalmol131 421 426 - 58.
Yang J. J. Tezel G. Patil R. V. Romano C. Wax M. B. 2001b Serum autoantibody against glutathione S-transferase in patients with glaucoma. Invest Ophthalmol Vis Sci42 1273 1276 - 59.
Zhang J. Koninck Y. 2006 Spatial and temporal relationship between monocyte chemoattractant protein-1 expression and spinal glial activation following peripheral nerve injury. J Neurochem97 772 783