Expression pattern of Ccr2 and Cx3cr1 in inherited retinal degeneration

Background

Though accumulating evidence suggests that microglia, resident macrophages in the retina, and bone marrow-derived macrophages can cause retinal inflammation which accelerates photoreceptor cell death, the details of how these cells are activated during retinal degeneration (RD) remain uncertain. Therefore, it is important to clarify which cells play a dominant role in fueling retinal inflammation. However, distinguishing between microglia and macrophages is difficult using conventional techniques such as cell markers (e.g., Iba-1). Recently, two mouse models for visualizing chemokine receptors were established, Cx3cr1 ^GFP/GFP and Ccr2 ^RFP/RFP mice. As Cx3cr1 is expressed in microglia and Ccr2 is reportedly expressed in activated macrophages, these mice have the potential to distinguish microglia and macrophages, yielding novel information about the activation of these inflammatory cells and their individual roles in retinal inflammation.

Methods

In this study, c-mer proto-oncogene tyrosine kinase (Mertk)^−/− mice, which show photoreceptor cell death due to defective retinal pigment epithelium phagocytosis, were employed as an animal model of RD. Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were established by breeding Mertk ^−/−, Cx3cr1 ^GFP/GFP, and Ccr2 ^RFP/RFP mice. The retinal morphology and pattern of inflammatory cell activation and invasion of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were evaluated using retina and retinal pigment epithelium (RPE) flat mounts, retinal sections, and flow cytometry.

Results

Four-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice showed Cx3cr1-GFP-positive microglia in the inner retina. Cx3cr1-GFP and Ccr2-RFP dual positive activated microglia were observed in the outer retina and subretinal space of 6- and 8-week-old animals. Ccr2-RFP single positive bone marrow-derived macrophages were observed to migrate into the retina of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. These invading cells were still observed in the subretinal space in 18-week-old animals.

Conclusions

Cx3cr1-GFP-positive microglia and Ccr2-RFP-positive macrophages were distinguishable in the retinas of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. In addition, Ccr2 expression in Cx3cr1 positive microglia is a feature of microglial activation in RD. Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice enabled observation of microglial activation over time during RD and may be useful for developing inflammation-targeted treatment strategies for RD in the future.

Since photoreceptor cell death (PCD) is the proximal cause of blindness in retinal degenerative disorders such as retinitis pigmentosa and age-related macular degeneration, the mechanism of PCD should be clarified. Though traditionally PCD is thought to occur due to genetic predisposition, environmental risk factors, and old age [1], accumulating clinical and experimental evidence suggests that retinal inflammation can accelerate PCD [2–5]. Retinal inflammation is mediated by the retinal innate immune system, including microglia, which are resident macrophages in the central nervous system (CNS) and the complement system [1]. In the healthy retina, the retinal innate immune system plays a beneficial role in maintaining retinal homeostasis [1]. However, once a pro-inflammatory cascade is triggered, this retinal innate immune system can cause PCD [3]. The molecular details of the retinal inflammatory cascade, PCD, and the relationship between the two are not yet entirely understood. However, it is clear that not only microglia but also bone marrow-derived macrophages which invade to retina via a damaged blood-retina barrier play principal roles in this process [3].

We recently reported migration of microglia and macrophages into the subretinal space in during retinal degeneration (RD) [3]. As both of these cell types are stained by the Iba-1 Ab, it is unclear which is the dominant cell type in the subretinal space. To differentiate the contributions of microglia and macrophages in PCD, we administered the microglia suppressive drug “minocycline” or depleted macrophages systemically by injection of clodronate-liposomes in an RD animal model. However, interestingly, both of these treatments ameliorated PCD in light exposed Abca4 ^−/− Rdh8 ^−/− mice which show drastic RD [3, 6], indicating that both microglia and macrophages play important roles in retinal inflammation and degeneration. Therefore, it is still uncertain which cell type initially triggers retinal inflammation and which plays a more dominant role in driving subsequent PCD.

In the current study, we employed two fluorescein protein knock in mouse models, namely Cx3cr1 ^GFP/GFP and Ccr2 ^RFP/RFP mice [7, 8] to distinguish microglia and macrophage in the retina. Cx3cr1 is the sole receptor for Cx3cl1, also called fractalkine. Cx3cr1 is expressed by dendritic cells, natural killer cells, and macrophages [9]. Ccr2 is also the sole receptor for Ccl2. Ccr2 is required for macrophage infiltration to injure cites [10]. Furthermore, both Cx3cr1 and Ccr2 are upregulated in RD [3, 11]. In a study of the brain, Cx3cr1 but not Ccr2 was expressed in microglia from embryonic development throughout adulthood [12]. However, whether this principle applies to retinal degeneration remains unknown. To shed light on microglia activation and to test whether microglia and macrophages are distinguishable in retinal degeneration, c-mer proto-oncogene tyrosine kinase (Mertk)^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ or Mertk ^+/+ Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were established by breeding Mertk ^−/−, Cx3cr1 ^GFP/GFP, and Ccr2 ^RFP/RFP mice. Mertk plays an essential role in retinal pigment epithelium (RPE) phagocytosis [13], and Mertk deficiency causes RD [14]. Furthermore, Mertk ^−/− mice show retinal inflammation associated with microglia and macrophage accumulation in the subretinal space [3, 11]. The retinal morphology and expression pattern of Cx3cr1-GFP and Ccr2-RFP in Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice was examined by retinal sectioning, retina and RPE flat mounts, and flow cytometry.

Animals

Mertk ^−/−, Cx3cr1 ^GFP/GFP, and Ccr2 ^RFP/RFP mice were obtained from Jackson Lab (Bar Harbor, Maine). Genotyping for Mertk was performed with primers: for wild type, forward 5′-GCTTTAGCCTCCCCAGTAGC-3′, reverse 5′-GGTCACATGCAAAGCAAATG-3′ and for mutant, forward 5′-CGTGGAGAAGGTAGTCGTACATCT-3′ and reverse 5′-TTTGCCAAGTTCTAATTCCATC-3′. Genotyping was performed for Cx3cr1 with primers; for wild type, forward 5′-TCCACGTTCGGTCTGGTGGG-3′ and reverse 5′-GGTTCCTAGTGGAGCTAGGG-3′ and for Cx3cr1 mutant, forward 5′-GATCACTCTCGGCATGGACG-3′ and reverse 5′-GGTTCCTAGTGGAGCTAGGG-3′. Genotyping for Ccr2 was performed with primers: for common, forward 5′-TAAACCTGGTCACCACATGC-3′; for wild type, reverse 5′-GGAGTAGAGTGGAGGCAGGA-3′; and for Ccr2 mutant, reverse 5′-CTTGATGACGTCCTCGGAG-3′, according to the protocol from Jackson Lab. Mertk ^−/− mice were crossed with C57BL/6 mice to make Mertk ^+/− mice. Mertk ^−/− and littermate control (Mertk ^+/+) mice, which were used as WT mice, were derived from Mertk ^+/− parents. Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ and Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were established from the same mouse lines. Briefly, since Cx3cr1 and Ccr2 are on the same mouse chromosome (Chr 9), Mertk ^+/− Cx3cr1 ^GFP/+ and Mertk ^+/− Ccr2 ^RFP/+ mice were established first from breeding Mertk ^−/− mice with Cx3cr1 ^GFP/GFP mice or Mertk ^−/− mice with Ccr2 ^RFP/RFP mice, respectively. Mertk ^−/− Cx3cr1 ^GFP/GFP and Cx3cr1 ^GFP/GFP (littermate control of Mertk ^−/− Cx3cr1 ^GFP/GFP) were obtained from Mertk ^+/− Cx3cr1 ^GFP/+ parents. Mertk ^−/− Ccr2 ^RFP/RFP and Ccr2 ^RFP/RFP (littermate control of Mertk ^−/− Ccr2 ^RFP/RFP) were obtained from Mertk ^+/− Ccr2 ^RFP/+ parents. Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were established by breeding Mertk ^−/− Cx3cr1 ^GFP/GFP and Mertk ^−/− Ccr2 ^RFP/RFP mice. Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were established by breeding Cx3cr1 ^GFP/GFP (littermate control of Mertk ^−/− Cx3cr1 ^GFP/GFP) and Ccr2 ^RFP/RFP (littermate control of Mertk ^−/− Ccr2 ^RFP/RFP).

Equal numbers of males and females were used. All mice were housed in the animal facility at the Jikei University School of Medicine, where they were maintained either under complete darkness or on a 12-h light (~10 lux)/12-h dark cycle. All animal procedures and experiments were approved by the Jikei University School of Medicine Animal Care Committees and conformed to both the recommendations of the American Veterinary Medical Association Panel on Euthanasia and the Association of Research for Vision and Ophthalmology.

Flat mount retina and RPE preparation

All procedures for retina and RPE flat mounts were described previously [3]. Images of flat mounts were captured by a confocal microscope (LSM, Carl Zeiss, Thornwood, NY, USA). For retina flat mount, the entire retina was captured at 5 μm intervals and all photographs were projected in one slice. For RPE flat mounts, the entire visible RPE was captured at 3 μm intervals and projected in one slice.

Histological analysis

All procedures to make sections for light microscopy were performed using a previously described method [15]. Rabbit anti-Iba-1 Ab (1:400, Wako, Osaka, Japan) was used for immunohistochemistry (IHC). Cell number was counted using ImageJ (National Institutes of Health, Bethesda, MD, USA). To observe microglia cell bodies, low melting point agarose-embedded (Sigma, St. Louis, MO, USA) thick sections (100 μm thickness) were prepared [16]. Images of IHC were captured on a confocal microscope (LSM, Carl Zeiss, Thornwood, NY, USA).

Quantitative RT-PCR (qRT-PCR)

All procedures for qRT-PCR were described previously [3]. Briefly, retinal samples from each group were collected from 16 eyes. Total RNA was isolated using a RiboPure Kit (Applied Biosystems, Austin, TX, USA), and cDNA was synthesized with SuperScript™ II Reserve Transcriptase (Invitrogen) following the manufacturer’s instructions. Real-time PCR amplification was performed using iQ™ SYBR II Green Supermix (Bio-Rad). Primers were designed using the web tool Primer 3 and synthesized by Eurofins MWG Operon (Hunstville, AL, USA). The following primers were used for analyses: Cx3cr1 (202 bp), forward 5′-CACCATTAGCTGGGCGTCT-3′, reverse 5′-GATGCGGAAGTAGCAAAAGC-3′; Ccr2 (227 bp), forward 5′-ATTCTCCACACCCTGTTTCG-3′, reverse 5′-ATGCAGCAGTGTGTCATTCC-3′. Relative expression of genes was normalized by comparison to the housekeeping gene Gapdh.

Flow cytometry

The neural retina was isolated from the eyecup with minimal inclusion of RPE cells, and the choroid plexus and ciliary body were carefully removed. The retina was then incubated in 0.25 % trypsin/PBS at 37 °C for 15 min. After stopping the activity of trypsin by the addition of 10 % FBS/PBS with 0.1 % DNaseI (Invitrogen, Waitham, MA, USA), the cells were mechanically dissociated into a single-cell suspension by gentle pipetting. The dissociated cells were stained with 0.1 % propidium iodide (PI)/PBS, and 100,000 cells were analyzed by FACSCalibur (BD, Franklin Lakes, NJ, USA). Peripheral blood samples were collected from the orbital venous plexus. After the lysis of erythrocytes in an isotonic solution of ammonium chloride, white blood cells (WBC) were stained with PI and used for flow cytometric analysis. Data analysis was performed using FlowJo software.

Data analysis

Data represent the mean ± SD. At least three independent experiments were compared by the one-way analysis of variance test.

First, the retinal phenotype of Ccr2 ^RFP/RFP and Cx3cr1 ^GFP/GFP mice was analyzed. No Ccr2-RFP-positive cells were detected in the retina of Ccr2 ^RFP/RFP mice, but Cx3cr1-GFP-positive microglia were ubiquitous in the inner retina (from the ganglion cell layer to the inner nuclear layer) of Cx3cr1 ^GFP/GFP mice. Ccr2-RFP-positive cells were found in Ccr2 ^RFP/RFP mice in the blood cell fraction corresponding to the monocyte population. No retinal degeneration was observed in either Ccr2 ^RFP/RFP or Cx3cr1 ^GFP/GFP mice (data not shown).

Retinal degeneration, microglia migration, and increase of Cx3cr1 and Ccr2 in Mertk^−/− mice

Next, the retinal phenotype of Mertk ^−/− and WT (Mertk ^+/+; littermate control of Mertk ^−/−) mice was evaluated. Eight-week-old Mertk ^−/− mice showed a decrease in photoreceptor nuclei number in the outer nuclear layer (ONL) and disorganized inner segments (IS) and outer segments (OS) (Fig. 1a). Iba-1-positive cells were found to migrate to the IS, OS, and subretinal space in 8-week-old Mertk ^−/− mice (Fig. 1b) indicating microglia/macrophage migration [3]. Because Iba-1 is expressed in both microglia and macrophages, these cells were not distinguishable. qPCR was used to compare Cx3cr1 and Ccr2 mRNA levels in the retinas of 3- and 8-week-old Mertk ^−/− and WT (Fig 1c). No significant differences in Cx3cr1 or Ccr2 expression were observed between 3- and 8-week-old WT mice. In contrast, for Mertk ^−/− mice, these mRNAs were increased in 8-week-old mice as compared to 3-week-old animals (Fig. 1c, left). At both the 3- and 8-week time points, expression of Cx3cr1 was increased in Mertk ^−/− mice compared to WT mice, and Ccr2 levels were increased in 8-week-old Mertk ^−/− mice as compared to WT controls (Fig. 1c, right).

Retinal phenotype and increase of Cx3cr1 and Ccr2 mRNA levels in Mertk ^−/− mice. Mertk ^−/− or WT (Mertk ^+/+) mice were established from Mertk ^+/− mice. a Retinal sections of 8-week-old Mertk ^−/− (left) and WT (right) mice were prepared. Eight-week-old Mertk ^−/−mice developed retinal degeneration, represented by thinning of the outer nuclear layer (ONL) and migration of inflammatory cells (arrow) (left panel). The insets are magnified images of the area within the broken rectangle. GCL ganglion cell layer, INL inner nuclear layer, ONL outer nuclear layer, IS inner segments, OS outer segments, RPE retinal pigment epithelium. b IHC was performed using rabbit anti-Iba-1-Ab. Eight-week-old Mertk ^−/− mice showed Iba-1-positive microglia/macrophages in the outer retina, though no Iba-1-positive cells were observed in WT mice. c Cx3cr1 and Ccr2 mRNA levels in the retina of Mertk ^−/− and WT were measured by qPCR. RNA samples were collected from 16 retinas at each time point. qPCR was performed 3–6 times (n = 3–6). Expression levels were compared between 3- and 8-week-old animals and between WT and Mertk ^−/− mice at each age. Error bars indicate the SD of the mean (n > 3). Asterisk indicates P < 0.05 vs 3-week-old Mertk ^−/− mice

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Migration of Cx3cr1-GFP-expressing microglia and invasion of Ccr2-RFP-positive monocyte-derived macrophage in degenerating retinas

To test the expression pattern of Ccr2 and Cx3cr1 in the degenerating retina and to determine whether microglia and macrophages are distinguishable in RD using Ccr2 ^RFP/RFP and Cx3cr1 ^GFP/GFP mice (as previously reported in the brain [12]), Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were established. Retinal sections of 4-, 6-, and 8-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown in Fig. 2. Four-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice, at the onset of RD, showed only Cx3cr1-GFP-positive microglia in the retina, and migration of some of these cells to the ONL was observed. No Ccr2-RFP-positive macrophages were observed (Fig. 2a, upper panels). Breakdown of the blood-retina barrier during the progression of retinal degeneration in Mertk ^−/− mice was previously reported [11]. Six-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice showed not only Cx3cr1-GFP-positive microglia but also Ccr2-RFP-positive macrophages in the outer retina, including the ONL, IS, OS, and RPE layers (Fig. 2a, middle panels). Interestingly, some RPE cells also expressed Ccr2-RFP. At 8 week of age, abundant Cx3cr1-GFP-positive and Ccr2-RFP-positive cells were observed. The majority of invading cells in the subretinal space (between the OS and RPE layers) were Cx3cr1-GFP and Ccr2-RFP dual positive (Fig. 2a, lower panels). Retinal sections of Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ 8-week-old mice at are shown as negative control (Fig. 2b). Cell numbers in the outer retina (from ONL to OS) and RPE were counted (Fig. 2c). Ccr2-RFP-positive and Cx3cr1-GFP and Ccr2-RFP dual positive cells increased in 8-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice (Fig. 2a, lower panels, and Fig. 2c).

Cx3cr1-GFP-positive microglia and Ccr2-RFP-positive macrophages in the retinas of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. a Retinal sections of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice at 4 (upper panels), 6 (middle panels), and 8 weeks of age (lower panels) are shown. Cx3cr1-GFP is shown in green, and Ccr2-RFP is shown in red. GCL ganglion cell layer, INL inner nuclear layer, ONL outer nuclear layer, IS inner segments, OS outer segments, RPE retinal pigment epithelium. The ONL boundaries are marked with broken lines. b Retinal sections of 8-week-old Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown as a negative control. c The numbers of Cx3cr1-GFP, Ccr2-RFP, and Cx3cr1-GFP and Ccr2-RFP dual positive cells in 500 μm of the outer retina (from ONL to OS), and RPE of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were counted. Five different sections from different mice were used to count cell number. Asterisk indicates P < 0.05 vs 4-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. n.d. not detected

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Microglia that have migrated to the subretinal space are Cx3cr1-GFP and Ccr2-RFP double positive

Retinal and RPE flat mounts of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were prepared to examine Cx3cr1-GFP-positive and Ccr2-RFP-positive cells in more detail (Fig. 3). Retinal and RPE flat mounts of Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown as negative controls (Fig. 3a, b, lower panels). At 6 weeks, Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice showed Cx3cr1-GFP-positive cells in the retina, which showed a ramified or amoeboid shape, corresponding to microglia. In addition, Ccr2-RFP-positive cells, which showed a round shape corresponding to monocyte-derived macrophages, were observed at this age (Fig. 3a, middle panels; Fig. 4a (a) and (b)). In contrast, only Cx3cr1-GFP-positive ramified-shaped microglia were observed in retina flat mounts of 4-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice (Fig. 3a (a), upper panels). RPE flat mounts of 6-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice showed amoeboid-shaped Cx3cr1-GFP-positive cells which co-express Ccr2-RFP, indicating that the microglia that had migrated to the subretinal space (the area just above the RPE) were Cx3cr1 and Ccr2 dual positive (Fig. 3b, middle panels, and Fig. 4a (c-1)). These Cx3cr1-GFP and Ccr2-RFP dual positive cells were morphologically distinct from Cx3cr1-GFP single positive ramified resting microglia and Ccr2-RFP single positive round-shaped macrophages (Fig. 4a). Amoeboid-shaped cells (Fig. 4a (c-1)), rather than round-shaped cells (Fig. 4a (c-2)), were the major cell population observed in RPE flat mounts from 6-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice, indicating that microglia are the dominant inflammatory cell type in the subretinal space at 6 weeks of age. The cell number of amoeboid Cx3cr1-GFP and Ccr2-RFP dual positive cells is significantly higher than round-shaped Cx3cr1-GFP and Ccr2-RFP dual positive cells in RPE flat mounts of 6-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice (Fig. 4b). Neither Cx3cr1-GFP-positive nor Ccr2-RFP-positive cells were observed in RPE flat mounts from 4-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice (Fig. 3b, upper panels). Cx3cr1-GFP-positive and Ccr2-RFP-positive cells were counted. In 6-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice, 18 and 61 % of the cells observed were Cx3cr1-GFP and Ccr2-RFP double positive in the retina and RPE, respectively (Fig. 4c). Taken together, Cx3cr1-GFP-positive microglia and Ccr2-RFP-positive macrophages were distinguishable in the sensory retina. However, microglia and macrophages that had migrated to the subretinal space, where accumulated OS and dying photoreceptors reside [3], co-expressed Cx3cr1-GFP and Ccr2-RFP, presumably indicating that activated microglia and macrophages that are actively phagocytizing photoreceptor OS express both of these factors.

Retina and RPE flat mounts from Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. Retina and RPE flat mounts from Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were prepared to analyze Cx3cr1-GFP and Ccr2-RFP-positive cells in more detail. a Retina flat mounts from 4- (upper panels) and 6-week-old (middle panels) Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown. Retina flat mounts from 6-week-old Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice (lower panels) are shown as negative controls. Cx3cr1-GFP is shown in green, and Ccr2-RFP is shown in red. b RPE flat mounts from 4- (upper panels) and 6-week-old (middle panels) Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown. RPE flat mounts from 6-week-old Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice (lower panels) are shown as negative controls. Cx3cr1-GFP is shown in green, and Ccr2-RFP is shown in red

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Analysis of retina and RPE flat mount. a Representative Cx3cr1-GFP (a), Ccr2-RFP (b), and Cx3cr1-GFP and Ccr2-RFP dual positive cells (amoeboid shape (c-1) and round shape (c-2)) observed in the retina and RPE flat mounts of 6-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown. Cx3cr1-GFP and Ccr2-RFP merged images are shown. b, c The number of amoeboid- (a-c-1) or round-shaped (a-c-2) Cx3cr1-GFP and Ccr2-RFP dual positive cells observed in RPE flat mounts (1 mm²) of 6-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice was counted. Five different RPE flat mounts from different mice were used to count cell number. Asterisk indicates P < 0.05. b Bar graph shows the abundance of amoeboid- and round-shaped dual positive cells in RPE flat mounts. c Pie chart displays the ratios of Cx3cr1-GFP-positive, Ccr2-RFP-positive, and dual positive cells in the retina (upper) and RPE (lower)

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Age dependence of Cx3cr1-GFP and Ccr2-RFP-positive cell localization in the retina and RPE in Mertk^−/−Cx3cr1^GFP/+Ccr2^RFP/+ mice

Retina and RPE flat mounts from 5-, 6-, and 18-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown (Fig. 5). In retina flat mounts, the number of Ccr2-RFP-positive cells peaked at 6 weeks of age and slightly decreased in 18-week-old animals, though no significant difference in the number of Cx3cr1-GFP-positive cells was observed from 5 to 18 weeks (Fig. 5a). In RPE flat mounts, a small number of Cx3cr1-GFP-positive cells were observed at 5 weeks, and this number progressively increased in 6- and 18-week-old mice. A small number of Ccr2-RFP-positive cells were observed in the RPE at 5 weeks. Similar to the retina, this number peaked at 6 weeks and decreased slightly at 18 weeks (Fig. 5b).

Retina and RPE flat mounts from Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice of different ages. a Retina flat mounts from 5-, 6-, and 18-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown. The number of Cx3cr1-GFP and Ccr2-RFP-positive cells in retina flat mounts of 5-, 6-, and 18-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice was counted. b RPE flat mounts of 5-, 6-, and 18-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice are shown. The number of Cx3cr1-GFP and Ccr2-RFP-positive cells in RPE flat mounts of 5-, 6-, and 18-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice was counted. Asterisk indicates P < 0.05 vs 4-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice

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Flow cytometric analysis of Cx3cr1-GFP and Ccr2-RFP expression in white blood cells (WBC) and the retina

Since bone marrow-derived macrophages infiltrate the injured retina [17], circulating WBC in Cx3cr1 ^GFP/GFP, Ccr2 ^RFP/RFP, and Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were examined. The proportion of Cx3cr1-GFP and Ccr2-RFP cells in WBC from Cx3cr1 ^GFP/GFP, Ccr2 ^RFP/RFP, and Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice was analyzed by flow cytometry. GFP- and RFP-positive WBC were observed in Cx3cr1 ^GFP/GFP and Ccr2 ^RFP/RFP mice, respectively (Fig. 6a, left and middle panels). WBC from Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice showed the presence of Cx3cr1-GFP single positive cells (1.39 %), Ccr2-RFP single positive cells (0.15 %), and Cx3cr1-GFP and Ccr2-RFP dual positive cells (0.47 %) (Fig. 6a, right panel). The proportion of Cx3cr1-GFP and Ccr2-RFP cells in the retinas of Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice was examined. The fraction of Ccr2-RFP-positive cells was increased in 6- and 8-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice compared to 3-week-old animals (Fig. 6b, upper panels). The fraction of Cx3cr1-GFP-positive cells and Cx3cr1-GFP and Ccr2-RFP dual positive cells peaked at 6 weeks and returned to basal levels at 8 weeks (Fig. 6b, lower graphs). The proportion of Cx3cr1-GFP and Ccr2-RFP-positive cells in the retina of 6-week-old Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice is shown as a negative control.

Flow cytometric analyses of WBC from Cx3cr1 ^GFP/GFP, Ccr2 ^RFP/RFP, and Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice and of the retinas from Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. a WBC were harvested from Cx3cr1 ^GFP/GFP, Ccr2 ^RFP/RFP, and Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. Cx3cr1-GFP and Ccr2-RFP are presented on the X and Y axes, respectively. Representative results from multiple flow cytometry analyses are shown. Boxes (a), (b), and (c) correspond to Ccr2-RFP, Ccr2-RFP, and Cx3cr1-GFP dual, and Cx3cr1-GFP-positive cells, respectively. b Neural retinas were obtained from 3-, 6-, and 8-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice and 6-week-old Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. Cx3cr1-GFP and Ccr2-RFP are presented on the X and Y axes, respectively. Representative results from multiple flow cytometry analyses are shown. Boxes (a), (b), and (c) correspond to Ccr2-RFP, Ccr2-RFP, and Cx3cr1-GFP dual, and Cx3cr1-GFP-positive cells, respectively. Quantitative results are shown for each gate. Single asterisk indicates P < 0.05, double asterisks indicate P < 0.005, and triple asterisks indicate P < 0.001 vs 3-week-old Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice. +/+ indicates 8-week-old Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice

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Mutations in the MERTK gene cause retinal dystrophies in humans and in animal models [18]. MERTK belongs to a family of receptor tyrosine kinases that includes AXL and TYRO3 and plays an indispensable role in the clearance of photoreceptor debris by RPE phagocytosis [19]. Accumulation of photoreceptor debris in the subretinal space due to RPE phagocytosis deficiency is closely associated with the photoreceptor cell death seen in Royal College of Surgeons (RCS) rats (with disabled Mertk) and in Mertk ^−/− mice [14]. Recently, we reported that Mertk ^−/− mice show migration of microglia and retinal inflammation, which exacerbated retinal degeneration [3, 11]. Chemokines and cytokines including Ccl2, Ccl3, Ccl12, and Il1b are increased in the degenerating retinas of Mertk ^−/− mice [3, 11]. Furthermore, blockade of Ccl2 and Ccl3 can attenuate the retinal phenotype of Mertk ^−/− mice, clearly indicating that retinal inflammation contributes to PCD and RD [11].

To visualize inflammatory cells in a tissue, staining or immunohistochemistry procedures are required. However, tissue staining is limited for detecting inflammatory cells and immunohistochemistry requires clean and selective antibodies. Cx3cr1 and Ccr2, especially Ccr2, are difficult to detect by immunohistochemistry due to the lack of an appropriate antibody [7]. Newly developed fluorescent protein knock-in mouse models, including Cx3cr1 ^GFP/GFP and Ccr2 ^RFP/RFP mice have the potential to overcome the limitations of tissue staining and immunohistochemistry, and these mice will be instrumental for developing new treatment strategies, especially neuroinflammation-targeted therapy. From our current data, Cx3cr1-GFP and Ccr2-RFP dual positive cells were visualized not only by histology (Figs. 2 and 3) but also flow cytometry (Fig. 6).

To date, several studies used a combination of Cx3cr1 ^GFP/GFP and Ccr2 ^RFP/RFP mice in experimentally induced disease models such as experimental autoimmune encephalomyelitis (EAE), an animal model of multiple sclerosis [7, 12]. However, these mouse models have yet to be employed in naturally occurring neurodegenerative disease models such as retinal degeneration or Alzheimer’s disease. In experimentally induced disease models such as EAE, inflamed monocyte-derived macrophages play a dominant role in neuroinflammation and degeneration; hence, disease onset occurs outside the CNS. In contrast, in naturally occurring neurodegenerative diseases including retinal degeneration, microglia presumably play the dominant role at the onset of neuroinflammation and degeneration because the blood-retina barrier or blood-brain barrier is maintained at early disease stages [3, 11, 20]. This study provides evidence that microglia is the dominant inflammatory cell during the early stages of retinal degeneration (Figs. 2, 3, and 4). The precise mechanisms underlying microglial activation and morphological alteration during RD still remain unclear. However, evidence suggests that exposure to dead photoreceptor debris and subsequent phagocytosis is an important trigger for microglial activation in RD, as administration of photoreceptor OS proteins induced increased cytokine and chemokine production in microglia in vitro [3]. Currently, it remains unclear how Ccr2-RFP-positive macrophages infiltrate the retina. However, they likely invade via either the inner or outer blood-retina barrier. The inner blood-retina barrier is composed of tight junctions between neighboring capillary endothelial cells which rest on a basal lamina covered by the foot processes of astrocytes and Müller glia and tight junctions between RPE cells comprise the outer blood-retina barrier [21]. We previously reported disruption of the inner blood-retina barrier during RD [3], and the tight junctions between RPE cells are also reportedly damaged during this process [11, 22].

Ccr2 is a therapeutic target for retinal degenerative disorders including AMD and RP because deletion of Ccl2, a cognate ligand for Ccr2, can rescue PCD in Mertk ^−/− mice [11] and deletion of Ccr2 ameliorated retinal degeneration in another model [23]. These observations are consistent with the co-expression of Ccr2-RFP in amoeboid-shaped Cx3cr1-GFP-positive microglia in Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice (Figs. 2, 3, and 4). Our results suggest that amoeboid-shaped activated microglia, which express both Cx3cr1 and Ccr2, are the dominant cell type in the subretinal space where they are activated by dead photoreceptors. Thus, Ccr2 expression in microglia is a feature of their activation during retinal degeneration. Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice enabled us to observe the switch of microglial phenotype from resting to activated state by monitoring Ccr2-RFP expression in vivo. However, other chemokines and chemokine receptors should also be tested. Previously, we reported an early peak of MIP-1 chemokines including C-C motif ligand (CCL)3 and CCL4 (compared to CCL2 or other chemokines) in light-induced Abca4 ^−/− Rdh8 ^−/− mice, which show dramatic PCD [11]. The Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice described here will be useful to develop future microglia-targeted treatment strategies for retinal degeneration.

Newly developed Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice were used to monitor the migration of Cx3cr1-GFP-positive microglia from the inner retina to the outer retina and subretinal space. Round-shaped Ccr2-RFP-positive monocyte-derived macrophages also invaded the retina. Activated microglia and macrophages that had migrated to the OS layer and subretinal space were Cx3cr1-GFP and Ccr2-RFP dual positive. Initiation of CCR2 expression in CX3CR1-positive microglia is a feature of microglial activation in RD. Currently, microglia suppressive approaches are being evaluated as new treatment strategies for retinal diseases including AMD, RP, and diabetic macular edema [3, 24, 25]. Mertk ^−/− Cx3cr1 ^GFP/+ Ccr2 ^RFP/+ mice will be a suitable model to assist in the development of future microglia-targeted treatment strategies.

CCL:

C-C motif ligand

CNS:

central nervous system

EAE:

experimental autoimmune encephalomyelitis

IHC:

immunohistochemistry

IS:

inner segments

Mertk :

c-mer proto-oncogene tyrosine kinase

ONL:

outer nuclear layer

OS:

outer segments

PCD:

photoreceptor cell death

RCS:

Royal College of Surgeons

RD:

retinal degeneration

WBC:

white blood cells

We thank Drs. A. Maeda, D. Mustafi, (Case Western Reserve University), N. Akiyama (the Jikei University School of Medicine), and M. Yoshida (Tokyo Hospital) for their comments and technical support. This work was supported by funding from the JSPS KAKENHI Grant-in-Aid for Young Scientists (Start-up) Grant Number 25893253 (for HK), Grant-in-Aid for Young Scientists (B) Grant Number 15K20288 (for HK) and Grant-in-Aid for Young Scientists (B) Grant Number 14451866 (for KO).

Authors and Affiliations

1. Department of Ophthalmology, The Jikei University School of Medicine, 105-8461, Tokyo, Japan

   Hideo Kohno, Kiichiro Okano, Hiroshi Tsuneoka & Tsutomu Sakai

2. Department of Molecular Immunology, The Jikei University School of Medicine, 105-8461, Tokyo, Japan

   Saburo Saito

3. Tokyu Hospital, 145-0062, Tokyo, Japan

   Hideo Kohno

4. Division of Molecular and Developmental Biology, The Institute of Medical Science, The University of Tokyo, 108-8639, Tokyo, Japan

   Hideto Koso & Sumiko Watanabe

5. Department of Pharmacology, School of Medicine, Case Western Reserve University, Cleveland, OH, USA

   Thomas R. Sundermeier

Corresponding authors

Correspondence to Hideo Kohno or Tsutomu Sakai.

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

HK and TS designed the study. HK and HK performed experiments. HK, HK, KO, and SW analyzed the data. SS and HT provided reagents. HK and TS wrote the manuscript. All authors read and approved the final manuscript.

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