In vivo multi-modal imaging of experimental autoimmune uveoretinitis in transgenic reporter mice reveals the dynamic nature of inflammatory changes during disease progression

Background

Experimental autoimmune uveoretinitis (EAU) is a widely used experimental animal model of human endogenous posterior uveoretinitis. In the present study, we performed in vivo imaging of the retina in transgenic reporter mice to investigate dynamic changes in exogenous inflammatory cells and endogenous immune cells during the disease process.

Methods

Transgenic mice (C57Bl/6 J Cx ₃ cr1 ^GFP/+, C57Bl/6 N CD11c-eYFP, and C57Bl/6 J LysM-eGFP) were used to visualize the dynamic changes of myeloid-derived cells, putative dendritic cells and neutrophils during EAU. Transgenic mice were monitored with multi-modal fundus imaging camera over five time points following disease induction with the retinal auto-antigen, interphotoreceptor retinoid binding protein (IRBP_1–20). Disease severity was quantified with both clinical and histopathological grading.

Results

In the normal C57Bl/6 J Cx ₃ cr1 ^GFP/+ mouse Cx₃cr1-expressing microglia were evenly distributed in the retina. In C57Bl/6 N CD11c-eYFP mice clusters of CD11c-expressing cells were noted in the retina and in C57Bl/6 J LysM-eGFP mice very low numbers of LysM-expressing neutrophils were observed in the fundus. Following immunization with IRBP_1–20, fundus examination revealed accumulations of Cx₃cr1-GFP⁺ myeloid cells, CD11c-eYFP⁺ cells and LysM-eGFP⁺ myelomonocytic cells around the optic nerve head and along retinal vessels as early as day 14 post-immunization. CD11c-eYFP⁺ cells appear to resolve marginally earlier (day 21 post-immunization) than Cx₃cr1-GFP⁺ and LysM-eGFP⁺ cells. The clinical grading of EAU in transgenic mice correlated closely with histopathological grading.

Conclusions

These results illustrate that in vivo fundus imaging of transgenic reporter mice allows direct visualization of various exogenously and endogenously derived leukocyte types during EAU progression. This approach acts as a valuable adjunct to other methods of studying the clinical course of EAU.

Uveitis is the fourth leading cause of blindness in the working age population in developed countries [1,2]. Endogenous posterior uveoretinitis makes up 22% of uveitis cases [3]. The aetiology of non-infectious uveoretinitis is unknown in most cases and has been considered to have an autoimmune basis [4,5]. Well-established animal models of experimental autoimmune uveoretinitis have provided a valuable experimental platform for improving our understanding of the disease pathogenesis and mechanisms of autoimmune uveoretinitis [4-8].

Experimental autoimmune uveoretinitis (EAU) is an organ-specific, T-cell mediated disease that can be induced in susceptible mouse strains by direct immunization with retinal antigens, including interphotoreceptor retinoid binding protein (IRBP) or arrestin (retinal soluble antigen, S-antigen), in complete Freund’s adjuvant and a simultaneous intraperitoneal injection of pertussis toxin. Alternatively, EAU can be induced indirectly by adoptive transfer of retinal antigen-specific effector T cells [4]. Disease usually develops around 10 to 14 days after immunization and is clinically evident within the retina as inflammatory cell infiltration which will include macrophages [9], dendritic cells (DCs) [10], neutrophils [11] and T cells [9,11]. In addition to the influx of blood-derived leukocytes, the resident myeloid-derived macrophages, retinal microglia, are also activated during EAU [7,8].

The Cx₃cr1^gfp/+ transgenic knock-in mouse [12] has enabled exquisite in vivo and ex vivo visualization of the dynamic changes in microglia in steady and diseased states in the eye [13-17], as well as in the brain [18,19], and in particular their rapid responsiveness to injury and presence of noxious stimuli [14,15]. The study of Cx ₃ cr1-bearing brain microglia in vivo in these reporter mice requires the surgical creation of a defect or window in the calvaria and two-photon microscopic examination of the superficial cortex [20]. By contrast, the eye offers unique advantages for direct in vivo visualization of infiltrating and resident immune cells in reporter mice with minimal experimental manipulation [16,21-23]. However, to date there has been limited use of reporter mice to investigate the dynamics of infiltrating leukocytes and resident myeloid cells in an ocular model of autoimmunity.

In the present study, we demonstrate that in vivo fundus examination of transgenic reporter mice facilitates monitoring of the dynamic changes in various exogenously and endogenously derived cells of myeloid lineage during EAU progression. In particular we chose to examine EAU in transgenic mice (C57Bl/6 J Cx ₃ cr1 ^GFP/+, C57Bl/6 CD11c-eYFP, and C57Bl/6 J LysM-eGFP) in which promoter elements of the myeloid-specific Cx ₃ cr1, CD11c and lysM genes are expressed alongside a specific fluorescent reporter in an attempt to characterize the relative temporal pattern of resident and infiltrating myeloid cells, DCs, and neutrophils, respectively. Whilst we appreciate that none of these transgenic reporter mice provide definitive identification of any of the above myeloid cell subsets and thus have their limitations [24], our results do provide novel insights into the cell mediated immune events in this model of human endogenous posterior uveoretinitis and allow accurate clinical grading of disease severity that correlates with histopathological changes.

Mice

Transgenic reporter mice in which the myeloid-specific promoter of the Cx ₃ cr1, CD11c, and lysM genes drives the expression of fluorescent reporters (C57Bl/6 J Cx ₃ cr1 ^GFP/+, C57Bl/6 N CD11c-eYFP, and C57Bl/6 J LysM-eGFP mice, respectively) were used in this study at an age of between 8 and 10 weeks. The details of the myeloid promoter and reporter mice used in this study are summarized in Table 1. C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice were created by crossing homozygous C57Bl/6 J Cx ₃ cr1 ^GFP/GFP mice, originally obtained from Professor Steffen Jung [12], to wild-type C57Bl/6 J mice. C57Bl/6 N CD11c-eYFP mice express enhanced yellow fluorescent protein (eYFP) under the promoter for the Itgax (CD11c) gene and are widely regarded as a valuable model for investigating the distribution of DCs with the caveat that other cells are capable of limited expression of CD11c [25]. C57Bl/6 N CD11c-eYFP breeding pairs were kindly provided by Associate Professor Michael Hickey (Monash University, Clayton, VIC, Australia) with permission from Professor Michel Nussenzweig (The Rockefeller University, New York, NY, USA) from whom the original mice were obtained [25]. C57Bl/6 J Cx ₃ cr1 ^GFP/+ and C57Bl/6 CD11c-eYFP mice were bred at the Monash Large Animal Facility (Monash University). C57Bl/6 J LysM-eGFP mice were kindly provided by Associate Professor Michael Hickey. C57Bl/6 J LysM-eGFP mice were created by cloning enhanced green fluorescent protein (eGFP) into the lysozyme M (LysM) locus where LysM is expressed in myelomonoytic cells (macrophages and neutrophil granulocytes) [26]. C57Bl/6 J Cx ₃ cr1 ^GFP/+ and C57Bl/6 J LysM-eGFP mice were screened by PCR [22] and determined to be negative for retinal degeneration 8 (rd8) mutation in the crumbs 1 (Crb1) gene (data not shown). C57Bl/6 N CD11c-eYFP mice were found to carry the rd8 mutation and this has been described in detail elsewhere [22]. All experimental animals were maintained under 12:12-hour light/dark cycle with ad libitum access to food and water. All procedures in this study were approved by the Monash Animal Ethics Committee (MARP/2011/094) and were performed in accordance with the ARVO Statement for the Use of Animals in Ophthalmic and Vision Research.

Induction of experimental autoimmune uveoretinitis

EAU was induced using a standard protocol, previously described by others [8]. Briefly mice received a subcutaneous (s.c.) injection of a total of 100 μl emulsion, containing a 50:50 mix of 400 μg human IRBP peptide 1–20 (IRBP_1–20; GPTHLFQPSLVLDMAKVLLD; China Peptides, Shanghai, China) in complete Freund’s adjuvant (CFA; Sigma-Aldrich, St Louis, MO, USA) supplemented with Mycobacterium tuberculosis H37RA (2.5 mg/ml; BD PharMingen, San Diego, CA, USA), distributed between the base of the tail and the right flank of each mouse. Mice simultaneously received an intraperitoneal (i.p.) injection of 1.5 μg pertussis toxin (Sigma-Aldrich) in phosphate-buffered saline (PBS). Control mice received s.c. injection of a total of 100 μl emulsion containing 50:50 mixture of CFA and PBS (no IRBP) and i.p. injection of pertussis toxin.

Clinical examination of eyes

Mice were clinically examined on day (d) 0, 14, 21, 28 and 35 post-immunization (p.i.). Mice were anesthetized by an i.p. injection of a mixture of ketamine (80 mg/kg; Troy Laboratories, Glendenning, NSW, Australia) and xylazine (10 mg/kg; Troy Laboratories). The pupils were dilated with 0.5% tropicamide (Mydriacil, Alcon Laboratories, Vilvoorde, Belgium), and the cornea was kept moist with the application of sterile lubricant GenTeal gel (Novartis, North Ryde, NSW, Australia). The fundus was examined using the Micron III camera (Phoenix Research Laboratories, Pleasanton, CA, USA) with StreamPix 5 software. Examination consisted firstly of capturing short 5 seconds videos with 100 frames in brightfield, followed by a sequence of GFP⁺ or YFP⁺ cells using the green fluorescent barrier filters, and lastly by a short sequence following a 20 μl s.c. injection of 10% fluorescein isothiocyanate (Alcon Laboratories, Frenchs Forest, NSW, Australia) to visualize the retinal vasculature. The brightness and contrast of all fundus images were adjusted equally using ImageJ 1.48C software [27].

Clinical assessment of experimental autoimmune uveoretinitis

The severity of disease was graded based on examination of the three modes of clinical fundus images (brightfield, fluorescent, and fluorescein angiography) by two masked observers using a modification of a previously described clinical grading scheme for EAU [6]. The modifications to the grading criteria (Table 2) were primarily a consequence of having both traditional brightfield fundus views augmented by the fluorescent capability offered by the Micron III camera.

Histological assessment of experimental autoimmune uveoretinitis

Mice were euthanized on d35 p.i. with an i.p. injection of sodium pentabarbitone (Lethabarb; Virbac, Milperra, NSW, Australia) and were perfused with 1% heparin in PBS followed by 4% paraformaldehyde (PFA) in PBS. Eyes were enucleated and stored in 4% PFA at 4°C. The right eye from each animal was post-fixed with Karnovsky fixative (4% PFA: 1% glutaraldehyde) for 48 hours and processed for resin histology. Tissues were embedded in Technovit glycol methacrylate resin (Heraeus Kulzer, Wehrheim, Germany), sectioned at 5 μm thickness through the optic nerve-pupillary axis and stained with haematoxylin and eosin. Sections from three different levels of each eye separated by a minimum distance of 50 μm were examined by light microscopy and disease severity was scored by a masked observer using the previously published histopathology grading system for mouse EAU [28].

Imaging of experimental autoimmune uveoretinitis disease progression in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice

In vivo clinical examination of eyes in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice prior to immunization revealed a normal fundus using brightfield ophthalmoscopy (Figure 1A), and revealed the distribution of the retinal microglia network in green fluorescent mode (Figure 1B) and normal retinal vasculature following fluorescein angiography (FA; Figure 1C). The time course of EAU was monitored in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice immunized with IRBP_1–20 over four time points (d14, d21, d28, and d35 p.i.). EAU disease was first observed on d14 p.i. (Figure 1D-F), was maximal at d21 p.i. (Figure 1G-I) and d28 p.i. (Figure 1J-L), and was only slightly reduced in severity at d35 p.i. (Figure 1M-O). All IRBP_1–20 immunized mice developed EAU while adjuvant treated control mice appeared normal at all time points (Additional file 1: Figure S1A-C).

Time-course monitoring of experimental autoimmune uveoretinitis disease with multi-modal imaging in one representative C57Bl/6 J Cx ₃ cr1 ^GFP/+ mouse. Fundus images of a C57Bl/6 J Cx ₃ cr1 ^GFP/+ mouse immunized with IRBP_1–20 in brightfield (BF) (A,D,G,J,M), fluorescent (Fluor) (B,E,H,K,N), and fluorescein angiography (FA) (C,F,I,L,O) taken over five time points illustrated experimental autoimmune uveoretinitis disease progression and GFP⁺ myeloid cell perivascular infiltrates during disease progression. d, Day; p.i. post-immunization. GFP, green fluorescent protein; IRBP, interphotoreceptor retinoid binding protein.

Full size image

Clinical examination of C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice during experimental autoimmune uveoretinitis reveals different disease severities

EAU disease severity can vary in IRBP_1–20 immunized C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice from mild (Additional file 1: Figure S1D-F), moderate (Additional file 1: Figure S1G-I) to severe (Additional file 1: Figure S1J-L) at all time points. Mild disease is characterized by swelling of the optic nerve head and mild vasculitis or perivenular cuffing (Additional file 1: Figure S1D), both evident due to accumulations of Cx₃cr1-GFP⁺ myeloid cells (Additional file 1: Figure S1E). However, no fluorescein leakage was noted in FA at this point although only the early filling phase was examined (Additional file 1: Figure S1F). Moderate grades are characterised by multiple small focal retinal lesions with moderate vasculitis affecting all retinal vessels evident in brightfield (Additional file 1: Figure S1G) and as Cx₃cr1-GFP⁺ perivenular infiltrates (Additional file 1: Figure S1H) with an absence of fluorescein leakage (Additional file 1: Figure S1I). Despite the presence of Cx₃cr1-GFP⁺ perivenular infiltrates, Cx₃cr1-GFP⁺ cellular infiltrates were absent in some focal retinal lesions seen in brightfield (Additional file 1: Figure S1G). Severe EAU can occasionally be detected as early as d14 p.i. and in the eyes where EAU disease was seen to be severe, multiple large retinal lesions and vasculitis affecting all retinal veins was noted (Additional file 1: Figure S1J). Marked Cx₃cr1-GPF⁺ peri-vascular infiltrates (Additional file 1: Figure S1K) sometimes correlated with leakage of fluorescein (Additional file 1: Figure S1L). The short 5 second brightfield fundus video also demonstrated rolling and migration of Cx₃cr1-GFP⁺ cells and non-Cx₃cr1-GFP⁺ cells in the retinal veins (Additional file 2: Supplementary video 1).

To eliminate the possibility that the hyperfluorescent perivascular infiltrates in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice are due to autofluorescence inflammatory cells we have provided clinical fundus images of IRBP_1–20 immunized Wildtype C57Bl/6 J taken at d21 p.i. (Additional file 3: Figure S2).

Clinical grading strongly correlates with histopathological grade of experimental autoimmune uveoretinitis disease in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice at day 35 post-immunization

EAU clinical disease scores from all clinical imaging time points were determined by two masked observers using the grading criteria (Table 2). All adjuvant controls appeared normal at all time points (Figure 2A) and no histopathological changes were observed at d35 p.i. (Figure 2C). In IRBP_1–20 immunized C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice EAU began to develop around d14 p.i. with grade 1.86 ± 0.33 (mean ± SEM) disease then gradually progressed over time and remained at grade 2.81 ± 0.24 until d35 p.i. (Figure 2A).

Comparison of experimental autoimmune uveoretinitis clinical and histopathological score in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice. No adjuvant controls developed experimental autoimmune uveoretinitis (EAU). EAU clinical disease score (A) in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice revealed a grade 2.8 disease by day 35 (d35) post-immunization (p.i.) (adjuvant controls: d0, d14, and d28: n = 14, d21 and 35: n = 24; IRBP_1–20: d0: n = 33, d14: n = 24, d21: n = 32, d28: n = 20, d35: n = 28). (B) Correlation between total histopathological disease score in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice on d35 p.i. and the clinical grade in the same mice (IRBP_1–20: n = 8). Pearson’s correlation was applied to analyse the correlation and the correlation coefficient (r) illustrate a strong positive linear correlation that is significant, P < 0.05. (C) Histology demonstrated no pathology in adjuvant controls. Representative histology images from C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice immunized with IRBP_1-20 illustrate key histopathological features of EAU including vasculitis (D; arrows), granuloma (D; arrowhead), retinal folds (E; arrows), vitritis (E; arrowheads), loss of retinal outer nuclear layer and photoreceptor layer (F; arrow), and cellular infiltrates of the retinal pigment epithelium and choroid (F; arrowheads). IRBP, interphotoreceptor retinoid binding protein.

Full size image

Histopathological disease scores in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice at d35 p.i. revealed a mean infiltrative grade of 2.38 ± 0.60 and a structural grade of 2.00 ± 0.38. Total histopathological score shows a significant positive correlation (r = 0.73; P = 0.019) with the clinical scores (Figure 2B). C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice immunized with IRBP_1–20 displayed classical histopathological features of EAU (Figure 2D-F), which have been described previously by several authors [6,28-30].

Clinical examination of experimental autoimmune uveoretinitis in C57Bl/6 N CD11c-eYFP mice

The C57Bl/6 N CD11c-eYFP mouse has been extensively used to map putative DCs in a variety of tissues [25,31-36]. We have recently described our discovery of the presence of the rd8 mutation in the Crb1 gene in the C57Bl/6 N CD11c-eYFP mice [22]. Multiple retinal lesions (Figure 3A) were observed in the fundus of naïve C57Bl/6 N CD11c-eYFP mice and we illustrated that these lesions co-localized with CD11c-eYFP⁺ cells (Figure 3B) [22]. At the time of our experiments to investigate the course of EAU in C57Bl/6 N CD11c-eYFP mice we were unaware of the rd8 mutation. It was during clinical examination of d0 naïve animals that we became suspicious of a baseline pathological status. Despite the presence of retinal degeneration, EAU was readily induced and typical EAU changes were noted in C57Bl/6 N CD11c-eYFP mice on d14 and d21 p.i. By d14 p.i. severe vasculitis was seen on brightfield fundoscopy (Figure 3C) and a large influx of perivascular CD11c-eYFP⁺ cells along retinal veins was observed in the fluorescent mode (Figure 3D) as well as in the brightfield due to the strong eYFP signal. Clinical examination on d21 p.i. revealed that vasculitis and the large influx of CD11c-eYFP⁺ cells was partly resolved but multiple retinal lesions were still present, and CD11c-eYFP⁺ cells were more evenly distributed in the retina (Figure 3E,F). FA examination revealed absence of fluorescein leakage (data not shown). All IRBP_1–20 immunized mice developed EAU while adjuvant treated control mice appeared normal at all time points.

Clinical fundus examination of C57Bl/6 N CD11c-eYFP mice in normal and diseased state. Fundus images of naïve C57Bl/6 N CD11c-eYFP (Crb1 ^rd8) mice in brightfield (BF) (A) and fluorescent mode (Fluor) (B) displaying multiple retinal lesions and accumulation of CD11c-eYFP⁺ cells in the retinal lesions attributable to the rd8 mutation. Fundus images of C57Bl/6 N CD11c-eYFP mice (n = 10) immunized with IRBP_1–20 on day 14 post-immunization (d14 p.i.) (C-D) and d21 p.i. (E-F) demonstrated perivascular infiltrates. eYFP, enhanced yellow fluorescent protein; rd8, retinal degeneration 8.

Full size image

Visualization of LysM-eGFP⁺ myelomonocytic cell infiltration during experimental autoimmune uveoretinitis in C57Bl/6 J LysM-eGFP mice

In C57Bl/6 J LysM-eGFP mice, eGFP is cloned into the LysM locus which is expressed in myelomonocytic cells (macrophages-eGFP^low and neutrophils-eGFP^high) [26] and have been used for in vivo imaging of neutrophils in healthy and diseased states [37]. In vivo imaging of the naïve C57Bl/6 J LysM-eGFP mouse fundus (n = 5) revealed a normal appearance (Figure 4A) and genotyping of these mice demonstrated that they did not carry the rd8 mutation (data not shown). In the naïve retina of these mice there were 16.6 ± 1.18 (mean ± SEM) LysM-eGFP⁺ cells present in the entire normal fundus (Figure 4B). However, upon examination of the clinical fundus video, transient LysM-eGFP⁺ cells were observed travelling at high velocity through the lumina of the retinal vessels (Additional file 4: Supplementary video 2). In vivo imaging of IRBP_1–20 immunized C57Bl/6 J LysM-eGFP mouse fundus on d14 p.i. illustrated mild EAU with swelling of the optic nerve head, mild vasculitis (Figure 4C) and accumulations of the LysM-eGFP⁺ cells around the optic nerve head and along the retinal vessels (Figure 4D). Clinical fundus examination on d21 p.i. revealed multiple large retinal lesions and moderate vasculitis (Figure 4E) and the LysM-eGFP⁺ cells were found along the retinal vessels and in retinal lesions (Figure 4F). FA examination revealed absence of fluorescein leakage (data not shown). All IRBP_1–20 immunized mice developed EAU while adjuvant treated control mice appeared normal at all time points.

Clinical fundus examination of C57Bl/6 J LysM-eGFP mice in normal and diseased state. Fundus images of naïve C57Bl/6 J LysM-eGFP mouse fundus in brightfield (BF) (A) and fluorescent mode (Fluor) (B) appears normal (n =5). Fundus images of C57Bl/6 J LysM-eGFP mouse (n = 4) immunized with IRBP_1–20 on day 14 post-immunization (d14 p.i.) (C-D) and d21 p.i. (E-F) illustrated the peripapillary infiltrates of vasculitis. eGFP, enhanced green fluorescent protein.

Full size image

Intravital imaging using genetically modified reporter mice in which leukocyte subtypes are endogenously labelled with a fluorescent reporter gene transcript has greatly enhanced our understanding of cellular and immunological mechanisms during inflammation of several tissues [38-40]. Many of these experimental approaches are partly hindered or complicated by the potential effects of surgical intervention needed to exteriorise or surgically alter the tissue under investigation such as mesentery [41,42], cremaster muscle [42-44], liver [45], lung [37], kidney [40,43], and skin [46]. In the case of intravital imaging of the brain a craniotomy window is required [47,48]. The eye has several advantages over most organs because by its very nature it provides a clear transparent window on both neural tissue (retina) and connective tissues (cornea, iris) [33,49], thus avoiding surgical intervention. We sought to exploit the recent development of multi-modal imaging techniques which allow high-quality examination of the mouse fundus [16,22] to investigate the behaviour of cells of myeloid origin during the course of EAU, a widely used model of ocular autoimmune disease.

Disease severity of EAU is routinely determined using histopathological grading methods [28,29,50]. To circumvent the issue of single time point post-mortem grading, several research groups have developed non-invasive clinical grading methods including topical endoscopic fundus imaging [51], otoscope imaging [6], scanning laser ophthalmoscopy [52] and optical coherence tomography [53-55]. In this present study, multi-modal fundus ophthalmoscopy was chosen to grade the disease severity as it has the advantages of being relatively inexpensive and has the capability of capturing both video and still frame images in brightfield, together with green and red fluorescence wavelengths.

Many previous phenotypic analyses of the inflammatory cell infiltrate during EAU have used multi-parameter flow cytometry to show that the majority of infiltrating cells are myeloid-derived with a peak in T cell infiltration around d14 p.i. [11,56,57]. Alternative approaches to visualize leukocyte trafficking in vivo in the eye during EAU have included use of acridine orange, a non-specific nuclear dye which can be visualized by fluorography. This method revealed leukocytes rolling along the retinal veins as early as d14 p.i. [58,59]; however, their specific phenotype was obviously not determined. More recently, in vivo imaging of the leukocyte subtypes with more specificity has become easier with the availability of genetically modified mouse models in which genes regulating leukocyte subtypes are used as promoters to express fluorescent reporter proteins. Although these transgenic mouse models are useful for providing insights to myeloid lineage cell types in normal and diseased state, some authors have warned of cautious interpretation of these mice as the sole means of identifying and distinguishing macrophages and DCs [24]. Such limitations are also true of the three transgenic mouse lines chosen for the present study.

There are several subpopulations of Cx₃cr1-GFP⁺ myeloid-derived cells in the normal retina including the hyalocytes on the retinal surface [60], subretinal macrophages on the other aspect of the neural retinal [61-63], and the extensive network of microglial populations in the retinal parenchyma [13,64]. C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice [12] have been widely used to investigate the role of microglia in numerous ocular conditions that may have an inflammatory element in their pathogenesis including potential models of retinal degeneration [65], retinopathy of prematurity [66,67] and diabetic retinopathy [16]. In the present study we demonstrate highly distinctive perivenular infiltrates of Cx₃cr1-GFP⁺ cells at d14 p.i. to d35 p.i. which is in agreement with previous studies [8,68]. The perivenular infiltrate could theoretically represent haematogenous Cx₃cr1-GPF⁺ (GFP^low) myeloid cells recently extravasated into the retina or the chemotactic migration of resident Cx₃cr1-GPF⁺ (GFP^high) microglia towards the vasculature. We believe the former is the case as the Cx₃cr1-GPF⁺ (GFP^high) microglia network seemed largely undisturbed, something that was subsequently confirmed by retinal whole mount analysis (data not shown).

The difficulty in distinguishing subpopulations of macrophages from cells of DC lineage was the motivation for the creation of CD11c transgenic reporter mice, specifically the CD11c-eYFP [25] and CD11c-DTR/GFP mice [69]. In these transgenic mice the promoter for the Itgax (CD11c) gene is used to drive eYFP expression (CD11c-eYFP mice) or GFP and diphtheria toxin receptor (DTR) expression (CD11c-DTR/GFP mice). CD11c is a leukocyte integrin comprised of an alpha X subunit that along with CD18, a leukocyte beta 2 integrin polypeptide, forms the CD11c/CD18 heterodimer which is important in leukocyte adhesion, migration and cell to cell interaction during immune responses. CD11c is expressed heterogeneously by different populations of DCs [25] and is important in T cell priming [69]. However, it is also expressed to at least one log lower than DCs on other immune cells such as natural killer cells, subpopulations of macrophages and activated T cells [25]. As such immune cells are not normally a feature of the resting central nervous system, we, like other previous investigators [31,32,70], thought is reasonably safe to assume that in the resting and disease state CD11c-eYFP⁺ cells may represent predominantly DCs. The view that CD11c-eYFP mice are valuable for examining the distribution of DCs has recently been strongly challenged by Hume [24] who points out that CD11c has no function in antigen presentation; not all DCs are CD11c⁺ and that not all CD11c⁺ cells are antigen-presenting cells. It was thus with caution that we chose to take advantage of the transgenic C57Bl/6 N CD11c-eYFP mice to examine the dynamic of DCs in EAU. Indeed at the commencement of this study we had the further complication of discovering that these mice had a pre-existing retinal dystrophy due to the presence of the rd8 mutation in the crb1 gene [71] and that the CD11c-eYFP⁺ cells in the retina represented activated microglia [22]. In the present study, CD11c-eYFP⁺ cells were recruited into the eye at d14 and d21 p.i. in a similar pattern to that observed in C57Bl/6 J Cx ₃ cr1 ^GFP/+ mice leading us to conclude that these CD11c-eYFP⁺ cells are likely a mixture of myeloid-derived cells.

Interestingly, despite the C57Bl/6 N CD11c-eYFP mice carrying the rd8 mutation and the pre-existing disrupted retinal architecture prior to immunization, they did not develop a more severe form of EAU as may have been predicted if one were to assume that this dystrophic condition compromised the immune status of the retina as we have previously concluded [22], although we have not specifically proven that the blood-ocular barrier was compromised.

In the C57Bl/6 J LysM-eGFP mouse line generated by Faust and colleagues [26], homologous recombination was used to insert the eGFP gene into the LysM locus. This was chosen because LysM is expressed specifically in the myelomonocytic cell lineage (macrophages and neutrophil granulocytes). Characterization of LysM-eGFP⁺ cells in the blood revealed that the eGFP^high polymorphonuclear granulocytes outnumbered LysM-eGFP⁺ monocytes by 50:1. In the present study, we observed exceedingly small numbers (16.6 ± 1.18) of largely static LysM-eGFP⁺ myelomonocytic cells around the optic nerve head in the normal C57Bl/6 J LysM-eGFP fundus. We propose that these are likely of monocyte lineage as it is highly unusual to detect extravasated neutophils in the normal retina. However, video analysis (not shown) revealed many LysM-eGFP⁺ travelling at high velocity in retinal vessel lumina, which we conclude are likely to be circulating neutrophils. In these mice we demonstrated increased numbers of LysM-eGFP⁺ cells in the peripapillary retinal vessels at d14 to d21 of EAU. Closer examination of the high power images (see inset, Figure 4) suggests that many of these are marginating in vessel lumina, a pattern which differs from the perivascular infiltrates observed in the C57Bl/6 J Cx ₃ cr1 ^GFP/+ and C57Bl/6 N CD11c-eYFP mice. Subsequent flow cytometry of retinal tissue during EAU in C57Bl/6 J LysM-eGFP mice revealed these cells to be largely a neutrophilic infiltrate (Goldberg and colleagues, unpublished data).

In conclusion, in vivo fundus imaging of C57Bl/6 J Cx ₃ cr1 ^GFP/+ and C57Bl/6 N CD11c-eYFP mice revealed the dynamics of the myeloid cell infiltrates in EAU, particularly the perivenular accumulations. In contrast, the C57Bl/6 J LysM-eGFP mice revealed intravascular margination of LysM-eGFP^hi neutrophils as well as less distinctive perivascular infiltrates. The grading of disease using in vivo imaging of these genetically modified reporter mice correlated strongly with the histopathological changes.

CFA:

complete Freund’s adjuvant

Crb1:

crumbs 1

d:

day

DC:

dendritic cell

DTR:

diphtheria toxin receptor

EAU:

experimental autoimmune uveoretinitis

eGFP:

enhanced green fluorescent protein

eYFP:

enhanced yellow fluorescent protein

FA:

fluorescein angiography

i.p.:

intraperitoneal

IRBP:

interphotoreceptor retinoid binding protein

LysM:

lysozyme M

PBS:

phosphate-buffered saline

PCR:

polymerase chain reaction

PFA:

paraformaldehyde

p.i.:

post-immunization

rd8:

retinal degeneration 8

s.c.:

subcutaneous

The authors would like to acknowledge Ms Katherine Lim and Dr Jimmy Leong (Monash University, Clayton, VIC, Australia) for masking the clinical fundus images and histological slides for disease grading, and Ms Manpreet Sidhu (Monash University) for assisting with the fundus imaging. The C57Bl/6 CD11c-eYFP and C57Bl/6 J LysM-eGFP mice were kindly provided by Associate Professor Michael Hickey. XC is a recipient of National Health and Medical Research Council (NH&MRC) Dora Lush Biomedical postgraduate scholarship (1039575). GLG is a recipient of the NH&MRC Career Development Fellowship (1034598). CCB is supported by grants from the NH&MRC (1053621), the Victoria/CIRM Joint Project (RMI-01739) and the Department of Industry (AISRF06680), Commonwealth of Australia. PGMcM receives support from the NH&MRC (1069979).

Authors and Affiliations

1. Department of Anatomy and Developmental Biology, School of Biomedical Sciences, Faculty of Medicine, Nursing and Health Sciences, Monash University, Clayton, Victoria, Australia

   Xiangting Chen, Jelena M Kezic & Paul G McMenamin

2. Section of Immunology and Infection, Division of Applied Medicine, School of Medicine and Dentistry, Institute of Medical Science, Foresterhill, University of Aberdeen, Scotland, UK

   John V Forrester

3. Ocular Immunology Program, Centre for Ophthalmology and Visual Science, The University of Western Australia, Crawley, Western Australia, Australia

   John V Forrester

4. Centre for Experimental Immunology, Lions Eye Institute, Nedlands, Crawley, Western Australia, Australia

   John V Forrester

5. Walter and Eliza Hall Institute of Medical Research, Parkville, Victoria, Australia

   Gabrielle L Goldberg & Ian P Wicks

6. Australian Regenerative Medicine Institute, Monash University, Clayton, Victoria, Australia

   Claude C Bernard

Corresponding author

Correspondence to Paul G McMenamin.

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

XC performed the immunization, in vivo analysis, tissue collection and subsequent histology, and drafted the manuscript. JMK was part supervisor of XC during her PhD studies and helped plan the study. JVF and CCB were also part supervisors of XC and advised on the experimental approach and reviewed the manuscript. GLG and IPW provided data from the C57Bl/6 J LysM-eGFP mice. PGM is the principle chief investigator in whose laboratory the studies were performed, and was primarily responsible with XC for the clinical grading, data analysis, data interpretation and writing of the manuscript. All authors read and approved the final manuscript.

Open Access  This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons licence, and indicate if changes were made.

The images or other third party material in this article are included in the article’s Creative Commons licence, unless indicated otherwise in a credit line to the material. If material is not included in the article’s Creative Commons licence and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder.

To view a copy of this licence, visit https://creativecommons.org/licenses/by/4.0/.

The Creative Commons Public Domain Dedication waiver (https://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated in a credit line to the data.

Reprints and permissions