Increased CD68/TGFβ Co-expressing Microglia/ Macrophages after Transient Middle Cerebral Artery Occlusion in Rhesus Monkeys.

The function of microglia/macrophages after ischemic stroke is poorly understood. This study examines the role of microglia/macrophages in the focal infarct area after transient middle cerebral artery occlusion (MCAO) in rhesus monkeys. We measured infarct volume and neurological function by magnetic resonance imaging (MRI) and non-human primate stroke scale (NHPSS), respectively, to assess temporal changes following MCAO. Activated phagocytic microglia/macrophages were examined by immunohistochemistry in post-mortem brains (n=6 MCAO, n=2 controls) at 3 and 24 hours (acute stage), 2 and 4 weeks (subacute stage), and 4, and 20 months (chronic stage) following MCAO. We found that the infarct volume progressively decreased between 1 and 4 weeks following MCAO, in parallel with the neurological recovery. Greater presence of cluster of differentiation 68 (CD68)-expressing microglia/macrophages was detected in the infarct lesion in the subacute and chronic stage, compared to the acute stage. Surprisingly, 98~99% of transforming growth factor beta (TGFβ) was found co-localized with CD68-expressing cells. CD68-expressing microglia/macrophages, rather than CD206+ cells, may exert anti-inflammatory effects by secreting TGFβ after the subacute stage of ischemic stroke. CD68+ microglia/macrophages can therefore be used as a potential therapeutic target.

INTRODUCTION

Stroke is the second leading cause of mortality globally, causing 6.7 million deaths each year [1, 2]. Treatments that can reperfuse the ischemic brain regions as early as possible after stroke onset are critical for the prevention of brain-cell death. As an example, recombinant tissue plasminogen activator is a clot-dissolving agent approved by the Food and Drug Administration despite its limited utility [3]. Another therapeutic option for acute ischemic stroke caused by an abrupt obstruction of a large vessel is endovascular recanalization, which involves the use of various intra-arterial devices to mechanically re-open the steno-occlusive lumen. However, few treatments can be effectively applied in the later stage of ischemic stroke. Moreover, little is known about the therapeutic potential of endogenous recovery mechanisms, warranting further study.

The ischemic brain lesions, visualized as abnormalities on diffusion magnetic resonance imaging (MRI), are complex pathological structures. A patient’s prognosis may depend on the activation of inflammatory cells in the infarcted brain region following the acute ischemic stroke [4]. Many studies using mouse models of ischemic stroke have identified the cluster of differentiation 68 (CD68) as a general marker of activated phagocytic microglia/ macrophages [5], which are the main inflammatory cells in the central nervous system [6]. However, very few studies have investigated the anti-inflammatory activities of CD68-expressing cells during the course of ischemic stroke in rodent models. High numbers of CD68-expressing microglia/macrophages were detected in the infarct core and the border zone at 24 hours and 7 days after ischemic stroke, respectively [7, 8]. In the chronic stage, cells in the ischemic penumbra express transforming growth factor beta (TGFβ), a cytokine involved in neuroprotective functions such as scar formation, inhibition of apoptosis and excitotoxicity, and promotion of angiogenesis and neurogenesis.

Additionally, microglia, particularly the M2 type, secrete cyto-kines with anti-inflammatory functions [9]. The representative M2 microglial marker, CD206, has been identified in central nervous system disorders such as Alzheimer’s disease [10], Parkinson’s disease [11], and acquired immunodeficiency syndrome [12]. In fact, the number of CD206-positive (CD206+) cells in the cortex and striatum significantly increases 3~7 days after middle cerebral artery occlusion (MCAO) [13]. The expression of TGFβ, inter-leukin-10 (IL10), and CD206 mRNA also increases at 24 hours, reaching peak levels 4~6 days after ischemic stroke [14]. The anti-inflammatory activities of CD206+ cells generally decrease around 7 days after ischemic stroke [15]. Elucidation of the progressive alterations in immune cells during the clinical course of stroke are essential for the development of effective therapies.

Histopathological investigations of microglial activation in patients who underwent endovascular recanalization treatment after stroke onset are challenging. To overcome the limitations of clinical studies, we used a non-human primate transient MCAO model established in our previous study [15], which exhibits physiological, anatomical, behavioral, imaging, and genetic properties similar to those observed in humans stroke patients.

MATERIALS AND METHODS

Experimental animals

Eleven rhesus monkeys (Macaca mulatta) were analysed, with brain immunohistological analysis performed in 8 animals postmortem and the remaining 3 monkeys surviving the study to date. Seven animals (R326, R330, R328, R315, R305, R306, and R313) from our previously published experiments [15] and additional two monkeys (R324 and R307) were included in this study. Two age-matched healthy monkeys (R310 and R322) were used as controls (Table 1). The acute (<7 days), subacute (7~30 days), and chronic stages (>30 days) of ischemic stroke were defined based on clinical observations of symptoms and recovery [16]. All experimental animals were considered “young” according to the age classification standards for humans and macaques [17, 18]. The rhesus monkeys (obtained from Gaoyao Kangda Laboratory Animals Science & Technology Co., Ltd., Gaoyao, China), were housed indoors in individual cages at the National Primate Research Center of the Republic of Korea and provided with commercial monkey chow (Harlan, USA) along with a daily supplement of various fruits and water ad libitum. Environmental conditions were controlled to maintain a temperature of 24±2°C, relative humidity of 50±5%, 100% fresh air at a rate of ≥12 room changes per hour, and a 12:12-hour light-dark cycle, as described in our previous studies [15, 19, 20]. All procedures were approved and conducted according to the guidelines set by the Korea Research Institute of Bioscience and Biotechnology Institutional Animal Care and Use Committee (Approval No. KRIBB-AEC-14004). Reporting of the work complies with Animal Research Reporting of In Vivo Experiments (ARRIVE) guidelines.

Table 1

Experimental animals

Group	Animal ID	Sex	*Age (y)	*Body weight (kg)	**Occlusion (duration)	***MRI f/u	NHPSS	†Histological-analysis
Control (n=2)	R310	M	5	4.0	X	X	X	O
	R322	F	6	3.3	X	X	X	O
Acute (n=2)	R324	F	5	5.5	135 min	3h	X	3 h
	R307	M	5	6.1	109 min	24h	X	24 h
Subacute (n=2)	R326	F	5	4.9	82 min	1w	X	2 w
	R330	F	4	5.3	111 min	3w	X	1 m
Chronic (n=5)	R328	F	7	5.7	152 min	4w	O	4 m
	R315	M	5	6.7	137 min	4w	O	20 m
	R305	M	5	4.6	135 min	4w	O	††Survival
	R306	M	5	7.0	128 min	4w	O	††Survival
	R313	M	5	6.2	162 min	4w	O	††Survival

Nine rhesus monkeys were assessed at different time points following the induction of ischemic stroke (2 acute, 2 subacute, and 5 chronic) with 2 age-matched controls.

Data were obtained shortly before surgery.

Occlusion time was determined after evaluation of plateau (three consecutive ADC-derived lesion volumes) by MRI scans at 15-minute intervals.

In vivo follow-up MRI (FLAIR, ADC, and DWI) was performed once a week starting 1 day post-infarct until 4 weeks after reperfusion to measure the infarct volume.

Histological analyses were conducted by post-mortem examination after the animal’s natural death.

Animals still surviving at the time of manuscript submission (approximately 3 years) with no corresponding MRI data.

h, hours; w, weeks; m, months; f/u, follow-up; FLAIR, fluid-attenuated inversion recovery; ADC, apparent diffusion coefficient; DWI, diffusion weighted imaging; NHPSS, non-human primate stroke scale; MRI, magnetic resonance imaging.

Ischemic stroke model and MRI

Ischemic stroke was induced using our previously reported endovascular MCAO technique [15]. Immediately after MCAO induction, the animal was transported to the MRI suite while maintaining the endovascular MCAO and scanned using 3.0 T MRI (Achieva 3.0 T, Philips Medical Systems, Best, Netherlands). To identify the infarct core in acute stage and diffusion-perfusion mismatch, diffusion weighted imaging (DWI) was performed at 30 minutes after the MCAO procedure, and MRI acquisition was repeated every 15 minutes thereafter. After the in-bore reperfusion and repeated MRI, postoperative veterinary care was provided to each animal. Infarct volume was measured by follow-up fluid-attenuated inversion recovery (FLAIR) MRI imaging performed once a week until 4 weeks post-infarct. Neuroimaging protocols used for the procedures performed on the day of stroke induction and the follow-up MRI studies were the same as those previously described.

Infarct volume measurement

Whole-head FLAIR images were cropped to box dimensions (x=79.50 mm, y=129.75 mm, and z=78.96 mm) to facilitate subsequent analysis (Fig. 1A). Hyper-intense regions were identified, and regions of interest (ROIs) were segmented using the Inveon Research Workplace (IRW; Siemens Medical Solutions, USA) software. Representative ROIs and 3D maximum intensity projection (MIP) views (66o, 0.96 scale; Fig. 1B and 1C), as well as raw data (Table 2), are shown. The following formula was used to calculate the infarct percentage:

Fig. 1

Regions of interest (ROIs) based on fluid-attenuated inversion recovery (FLAIR) images. ROIs were semi-automatically calculated using the Inveon Research Workplace (IRW) (A). Four ROIs were selected for the whole brain (green; RGB, 0.255.0), infarct lesion (red; RGB, 255.0.0), brain template (light blue; RGB, 0.204.204), and infarct lesion template (purple; RGB, 255.0.255). Representative 3D maximum intensity projection (MIP) views (66°, 0.96 scale) of the whole brain (B) and infarct lesion (C) are shown. The left scale bar represents 140.0 mm in Fig. 1A and 120.0 mm in Fig. 1B and 1C, and the right scale bar represents the window level (−1.6/268.6). R, Right; L, Left; A, Anterior; P, Posterior; S, Superior; I, Inferior.

Table 2

3D infarct volume calculation with a threshold

	ROI	Volume (mm3)	Volume (%)	Mean	SD	Min	Max	Threshold Min/Max
R326 (24h)	Whole Brain	90615.50	100.00	57.3	16.0	38.0	132.5	38.0/251.0
	Infarct lesion	10273.90	11.34	95.8	8.0	81.0	132.5	81.0/251.0
R326 (1w)	Whole Brain	94266.70	100.00	69.6	20.1	38.0	148.3	38.0/251.0
	Infarct lesion	15770.70	16.73	108.4	12.1	81.0	148.3	81.0/251.0
R330 (24h)	Whole Brain	87765.20	100.00	65.2	14.1	38.0	193.0	38.0/251.0
	Infarct lesion	3060.40	3.49	120.5	19.8	81.0	193.0	81.0/251.0
R330 (1w)	Whole Brain	86865.00	100.00	63.8	12.1	38.0	152.3	38.0/251.0
	Infarct lesion	3062.00	3.53	107.5	13.2	81.0	152.3	81.0/251.0
R330 (2w)	Whole Brain	86345.10	100.00	66.3	10.7	3.3	160.1	38.0/251.0
	Infarct lesion	1063.70	1.23	109.1	15.0	81.0	160.1	81.0/251.0
R330 (3w)	Whole Brain	82786.50	100.00	55.4	7.6	38.0	128.6	38.0/251.0
	Infarct lesion	385.40	0.47	94.3	9.8	81.0	128.6	81.0/251.0
R328 (24h)	Whole Brain	109550.00	100.00	49.6	8.7	1.0	114.0	38.0/251.0
	Infarct lesion	1260.70	1.15	90.2	5.9	81.0	114.0	81.0/251.0
R328 (1w)	Whole Brain	107460.00	100.00	59.2	9.0	8.8	128.7	38.0/251.0
	Infarct lesion	1745.40	1.62	94.7	7.9	81.0	128.7	81.0/251.0
R328 (2w)	Whole Brain	107650.00	100.00	61.2	8.4	1.6	134.4	38.0/251.0
	Infarct lesion	464.80	0.43	98.1	10.9	81.0	134.4	81.0/251.0
R328 (3w)	Whole Brain	107520.00	100.00	63.5	8.9	3.0	139.3	38.0/251.0
	Infarct lesion	400.50	0.37	96.0	10.6	81.0	139.3	81.0/251.0
R328 (4w)	Whole Brain	105290.00	100.00	58.3	8.3	32.0	122.0	38.0/251.1
	Infarct lesion	241.50	0.23	90.6	7.3	81.0	122.0	81.0/251.1
R315 (24h)	Whole Brain	105500.00	100.00	61.6	14.3	0.0	151.0	38.0/251.0
	Infarct lesion	5755.40	5.46	108.0	10.5	81.0	151.0	81.0/251.0
R315 (1w)	Whole Brain	104140.00	100.00	55.7	10.6	1.1	112.0	38.0/251.0
	Infarct lesion	4280.80	4.11	90.2	5.6	81.0	112.0	81.0/251.0
R315 (2w)	Whole Brain	103990.00	100.00	56.8	9.8	10.7	136.1	38.0/251.0
	Infarct lesion	1649.90	1.59	97.3	10.0	81.0	136.1	81.0/251.0
R315 (3w)	Whole Brain	104270.00	100.00	58.4	9.8	0.9	124.3	38.0/251.0
	Infarct lesion	1453.70	1.39	92.7	7.1	81.0	124.3	81.0/251.0
R315 (4w)	Whole Brain	100810.00	100.00	54.5	8.4	7.1	98.9	38.0/251.1
	Infarct lesion	109.20	0.11	83.9	3.3	80.1	98.9	81.0/251.1

The whole brain, infarct lesion, brain template, and infarction template were selected for ROIs. Infarct volume (%)=infarct lesion (mm3) / whole brain (mm3)×100 without template volume. Mean, SD, min, and max were also automatically calculated by IRW in the infarct lesion for the brain excluding the template.

To retain experimental objectivity, ROIs were automatically determined using equivalent thresholds: whole brain (38.0/251.0), infarct area (81.0/251.0), and window level (−1.6/268.6). To avoid areas affected by noise, ROI templates were applied manually, excluding the contralateral hemisphere, cerebrospinal fluid, peri-ventricle, and edge signals. ROIs based on representative FLAIR images focused on slice 315/512 coronal section (axial field of view (FOV)=12.98×19.47 cm, coronal FOV=13×19.47 cm, sagittal FOV=13×19.47 cm, and scale=1.15; Fig. 1A). Four ROIs were selected, representing the whole brain (green; RGB, 0.255.0), infarct lesion (red; RGB, 255.0.0), brain template (light blue; RGB, 0.204.204), and infarction template (purple; RGB, 255.0.255). Mean, standard deviation (SD), minimum, and maximum were automatically calculated using IRW for the brain regions, excluding the template region (Table 2).

Behavioral assessment

Neurological scoring was conducted using the validated Non-human Primate Stroke Scale (NHPSS) [21, 22]. NHPSS comprises ratings of state of consciousness, defense reaction, grasp reflex, extremity movement, gait, circling, bradykinesia, balance, neglect, visual field cut/hemianopsia, and facial weakness. Many of the NHPSS ratings reflect the National Institutes of Health Stroke Scoring system in humans. Total scores range from 0 to 41, with 0 corresponding to normal behavior and 41 to severe bilateral neurological impairment. Five monkeys which survived (R328 and R315) or still survive (R305, R306, and R313) beyond 4 weeks into the later chronic stage were evaluated at 1, 3, 7, 9, 13, 16, 20, 23, 27, and 30 days after reperfusion.

Tissue fixation and slice preparation

The post-mortem brains obtained within our previous study [15] (n=4, subacute and chronic groups), comprising an additional acute (n=2) and control groups (n=2), were evaluated. As described in our histological study [20], the brains of experimental animals were fixed with 10% neutral buffered formaldehyde (NBF). The brains were subsequently harvested and post-fixed for 7 days in 10% NBF. The whole brains were sliced in the coronal plane; 4-mm-thick slices were obtained and embedded in a rhesus monkey brain matrix (Ted Pella Inc., Redding, CA, US). Coronal slices (15 to 17) were acquired and numbered from rostral to caudal. Subsequently, the tissues were embedded in paraffin using a routine procedure.

Immunohistochemistry analysis

For immunohistochemistry, 5-μm sections were de-paraffinized, and heat-induced antigen retrieval was performed at 110°C in citrate buffer (pH 6.0; Vector Laboratories, Peterborough, UK). The sections were blocked for 45 minutes with 2% normal goat serum and then incubated for 12 hours at 4°C with the following primary antibodies: polyclonal rabbit anti-ionized calcium binding adaptor molecule 1 (Iba1; 1:500; Abcam, Cambridge, UK), monoclonal mouse anti-CD68 (1:500; Abcam), polyclonal rabbit anti-CD206 (1:100; Abcam), monoclonal rabbit anti-inducible nitric oxide synthase (iNOS; 1:500; Cell Signaling, Danvers, US), polyclonal rabbit anti-tumor necrosis factor-alpha (TNFα; 1:100; Antibodies, Atlanta, US), polyclonal rabbit anti-IL6 (1:100; Antibodies), polyclonal rabbit anti-TGFβ (1:500; Antibodies), polyclonal rabbit anti-IL10 (1:100; Abcam), monoclonal rabbit anti-CD13 (1:500; LSBio, Seattle, US), monoclonal mouse anti-Ki67 (1:100; Abcam), and monoclonal rabbit anti-Ki67 (1:100; Cell Marque, Darmstadt, Germany). For immunofluorescence analysis, sections were incubated at 25°C with CFTM488/594A-labeled goat anti-rabbit and anti-mouse secondary antibody (Biotium, Hayward, CA, US) in darkness for 1 hour. Next, sections were mounted with 4, 6-diamidino-2-phenylindole (DAPI) Vectashield Hard Set Mounting Medium (Vector Laboratories) for nuclei counterstaining, and images were acquired using an Olympus BX51 microscope.

Histological data analysis and quantification

Twenty-five ROIs (400× magnification, FOV=69×52 μm) were selected in the infarct core, peri-infarct core, and the contralateral hemisphere. Representative images were classified into three areas (1, infarct core; 2, peri-infarct; 3, contralateral hemisphere) based on the histological study [23]. Signal intensity was quantified using Image J histogram with inverted 8-bit. Threshold values were as follows: Iba1, 16~23; CD68, 20~25; CD206, 15~20; and TGFβ, 15~20. To remove outliers, both radius (4) and threshold (10) were identically applied. The microglial cells, phagocytic cells, inflammatory cytokine-secreting cells, M1/M2 type microglia/macrophages, and proliferating cells were counted using Image J cell counter plugin.

Statistical analysis

Statistical analysis was performed using the Statistical Package for the Social Sciences for Windows Version, 18.0 (SPSS Inc., Chicago, IL, USA). Wilcoxon signed-rank test was used for pairwise analyses when the Friedman p-value was <0.05. Data were presented as mean±SEM. Linear regression was used for two-group comparisons.

RESULTS

Changes in the infarct volume and behavioral assessments

We performed MRI once a week until 4 weeks after ischemic stroke to confirm the presence of the infarct lesion and calculate the infarct volume based on FLAIR images. Representative DWI and FLAIR images are shown in Fig. 2A. The acquired MR data were used to calculate changes in the infarct volume from 24 hours to 4 weeks after reperfusion (Fig. 2B). Interestingly, the infarct volumes exhibited significant reductions between 1 and 2 weeks post-reperfusion compared to the early time points.

Fig. 2

Gradual reduction in the infarct volume is associated with neurological recovery. (A) Follow-up MRI with fluid-attenuated inversion recovery (FLAIR) imaging was performed in six rhesus monkeys from 24 hours until 4 weeks after reperfusion. Diffusion weighted imaging is shown at 3 hours after reperfusion. (B) Changes in the infarct volume calculated from the FLAIR images in the subacute and chronic groups (R326, R330, R328, and R315). (C) Changes in the neurological scores measured by Non-human Primate Stroke Scale (NHPSS) in the chronic group (n=5). Data are presented as mean±standard error of mean (SEM).

Neurobehavioral assessments were conducted using the NHPSS at 1~30 days after stroke (Fig. 2C). Animals subjected to MCAO/ reperfusion showed an initial peak in score at 1 day, followed by a gradual reduction between 9 and 30 days. Since NHPSS total score of 0 corresponds to normal behavior, these results suggest that the neurological impairment in animals recovers almost to the baseline between 9 and 30 days after MCAO. The pattern of change in behavioral outcomes is similar to that of infarct volumes measured by MRI, suggesting that the infarct size reduction may be beneficial.

CD68 expression in Iba1+ microglial cells in the ipsilateral hemisphere

First, we analysed the function of activated microglial cells using Iba1 and CD68 as markers for microglia and phagocytic microglia/macrophages, respectively. We detected significantly more cells that were positive for both CD68 and Iba1 in MCAO animals in the subacute and chronic stages, compared to the acute stage, as well as to controls (Fig. 3). Moreover, CD68+ cells were frequently surrounded by cells expressing Iba1 (Fig. 3A). Most of the Iba1+ microglial cells (82~88%) were positive for CD68 in the infarct core during the subacute and chronic stages (Fig. 3D and 3E). Linear regression analysis revealed that the staining intensities of CD68 and Iba1 were significantly correlated in the subacute and chronic stages (Fig. 3F), but not in the acute stage (data not shown). Cells positive for only one of the markers (CD68+/Iba1− or CD68−/ Iba1+ cells) were also found (Fig. 3B and 3C).

Fig. 3

Cluster of differentiation 68 (CD68) expression in ionized calcium binding adapter molecule 1 (Iba1)-positive microglial cells. (A) Paraffin-embedded brain sections were immunostained with Iba1 (green) for microglial cells and CD68 (red) for phagocytic cells, and subsequently counter-stained with 4, 6-diamidino-2-phenylindole (DAPI) (blue) for cell nuclei at 2 weeks after reperfusion. Both reactive and phagocytic microglial cells are shown in the inset images. 1, infarct core; 2, peri-infarct core; 3, contralateral hemisphere. Representative images were obtained from animal R326. Scale bar represents 10 μm. (B~D) Quantification of CD68- and Iba1-positive cells. The number of CD68-specific (B), Iba1-specific (C), and CD68+/Iba1+-co-expressing (D) cells was quantified using Image J cell counter. (E) The ratio of CD68+/Iba1+ cells over total Iba1+ cells is shown. Data are presented as mean±SEM. Each line chart symbol represents 50 regions of interest, with 2 animals in each group. (F) Linear regression analysis of the intensities of CD68- and Iba1-positive cells in the ipsilateral hemisphere from subacute and chronic groups.

TGFβ expression in activated CD68+ cells in the ipsilateral hemisphere

We next evaluated the expression of cytokines to determine whether CD68-expressing cells exhibit inflammatory activity. Immunohistochemistry was performed for pro-inflammatory cytokines, including IL6 and TNFα, and for anti-inflammatory cytokines, including IL10 and TGFβ (Fig. 4 and 5). We detected a significantly higher number of cells positive for both CD68 and TGFβ in the subacute and chronic stages, compared to the acute stage or control animals (Fig. 4D). Indeed, most of the TGFβ+ cells (98~99%) co-expressed CD68 in the chronic stage (Fig. 4E) with significant (p<0.001) linear regression of the intensity observed in the ipsilateral hemisphere of animals in subacute and chronic groups (Fig. 4F), suggesting their anti-inflammatory function. In contrast, cells expressing pro-inflammatory cytokines, such as IL6 and TNFα, were not significantly correlated with CD68-expressing cells (Fig. 5). Interestingly, cells expressing IL10 did not co-express CD68 but were abundantly detected, suggesting that other brain cells, such as astrocytes or effector T cells, may show anti-inflammatory functions.

Fig. 4

Transforming growth factor beta (TGFβ) expression in activated CD68-positive cells in the chronic stage. (A) Paraffin-embedded brain sections were immunostained with CD68 (red) for phagocytic cells and TGFβ (green) for anti-inflammatory cytokines and counterstained with DAPI (blue) for cell nuclei at one month after reperfusion. Both phagocytic and anti-inflammatory cytokine-expressing cells are shown in the inset images. 1, infarct core; 2, peri-infarct core; 3, contralateral hemisphere. Representative images were obtained from animal R330. Scale bar represents 10 μm. (B~D) Quantification of CD68- and TGFβ-positive cells. The number of CD68-specific (B), TGFβ-specific (C), and CD68+/TGFβ+-coexpressing (D) cells was quantified using Image J cell counter. (E) The ratio of CD68+/TGFβ+ cells over total TGFβ+ cells is shown. Data are presented as mean±SEM. Each line chart symbol represents 50 regions of interest, with 2 animals in each group. (F) Linear regression analysis of the intensities of CD68- and TGFβ-positive cells in the ipsilateral hemisphere from the subacute and chronic groups.

Fig. 5

Correlation between phagocytic cells and pro/anti-inflammatory cytokines in the ischemic lesion. Paraffin-embedded brain sections were im-munostained with CD68 for phagocytic cells, TNFα/IL6 for pro-inflammatory cytokines, and IL10 for anti-inflammatory cytokines, and subsequently counterstained with DAPI for cell nuclei at one month after reperfusion. IL10-expressing cells were not correlated with phagocytosis (arrowheads). Scale bar represents 10 μm. The representative images were obtained from animal R330.

Characterization of M1 and M2 polarization of CD68+ cells

Next, we performed additional histological analyses to determine whether CD68-expressing cells represented the M1 or M2 microglial phenotype. According to the immunological studies [24, 25], a panel of markers for identifying M1 (inducible nitric oxide synthase: iNOS) and M2 (CD206) macrophage phenotypes was used (Fig. 6). Only a few CD68/CD206 double-positive cells were detected in the infarct core (Fig. 6D). Notably, 10~34% of iNOS was co-expressed in the CD68-expressing cells in the ipsilateral hemisphere from the subacute and chronic groups. Single positive cells (CD68+/CD206−, CD68−/CD206+, CD68+/iNOS−, and CD68−/ iNOS+ cells) were also found (Fig. 6B, 6C, 6E and 6F).

Fig. 6

CD68-positive phagocytic cells have low correlation with the M2 type microglia/macrophage marker, CD206. (A) Paraffin-embedded brain sections were immunostained with CD68 for phagocytic cells, CD206 for M2 type, and iNOS for M1-type microglia/macrophages, followed by coun-terstaining with DAPI for cell nuclei at one month after reperfusion. Merged cells (inset image) were specifically detected in the subacute and chronic stage. 1, infarct core; 2, peri-infarct core; 3, contralateral hemisphere. Representative images were obtained from animal R330. Scale bar represents 10 μm. (B~D) Quantification of CD68- and CD206-positive cells. The number of CD68-specific (B), CD206-specific (C), and CD68+/CD206+-coexpressing (D) cells was quantified using Image J cell counter. (E~G) Quantification of CD68- and iNOS-positive cells. CD68-specific (E), iNOS-specific (F), and CD68+/iNOS+-co-expressing (G) cells were detected. (H) The ratio of CD68+/iNOS+ cells over the total CD68+ cells are shown. Data are presented as mean±SEM. Each line chart symbol represents 50 regions of interest, with 2 animals in each group.

Cell proliferation in the ipsilateral hemisphere after stroke

Lastly, we examined Ki67 expression, a marker of proliferation, in CD68-expressing cells, Iba1+ microglial cells, and CD13+ pericytes (Fig. 7 and 8) after ischemic stroke. Although most of the proliferating cells were negative for CD68 (Fig. 7D) and CD13 (Fig. 8) after ischemic stroke, a few CD68+ proliferating cells were present in the subacute stage. We also observed cells positive for only one of the markers (CD68+/Ki67− cells, Fig. 7B; CD68−/Ki67+ cells, Fig. 7C). Some of the Iba1+ microglial cells exhibited Ki67+ nuclei (Fig. 8).

Fig. 7

Several proliferating CD68-expressing cells are observed in the subacute stage. (A) Paraffin-embedded brain sections were immunostained with CD68 (red) for phagocytic cells and Ki67 (green) for cell proliferation and counterstained with DAPI (blue) for cell nuclei at 2 weeks after reperfusion. Several proliferating phagocytic cells (inset image) were detected in the subacute stage. 1, infarct core; 2, peri-infarct core; 3, contralateral hemisphere. Representative images were obtained from animal R326. Scale bar represents 10 μm. (B~D) Quantification of CD68- and Ki67-positive cells. The number of CD68-specific (B), ki67-specific (C), and CD68+/Ki67+-coexpressing (D) cells was quantified using Image J cell counter. Data are presented as mean±SEM. Each line chart symbol represents 50 regions of interest, with 2 animals in each group.

Fig. 8

Ki67 expression in microglia and pericytes. Paraffin-embedded brain sections were immunostained with Iba1 for microglial cells, CD13 for pericytes, and Ki67 for cell proliferation, and subsequently counter-stained with DAPI (blue) for cell nuclei at 2 weeks after reperfusion. Several proliferating microglial cells were detected in the infarct lesion, but no proliferating pericytes were observed (inset images). Scale bar represents 10 μm. Representative images were obtained from animal R326.

DISCUSSION

In our previous study, we established an experimental non-human primate stroke model to examine the reversibility of diffusion abnormalities [15]. Clinically, it is difficult to study the alterations in cellular pathology that occur in parallel with diffusion changes in the human brain following the recanalization of the occluded vessel. Therefore, the non-human primate MCAO model can help improve our understanding of how reversible changes in diffusion interact with cellular pathology. Using MRI analysis, Liu et al. identified a true permanent reversal in a non-human primate ischemic stroke model induced by endovascular techniques [26]. However, most experimental ischemic stroke studies have used rodent MCAO models [27-31].

The results of the present study suggest that CD68-expressing microglia/macrophages may elicit long-term anti-inflammatory effects by secreting TGFβ. Although we did not present any results regarding neuronal recovery, numerous studies have reported a decrease in infarct volume, neuronal cell death, and behavioral deficits following intra-carotid [32], intranasal [33], intra-ventricular [34], or adenoviral [35] delivery of TGFβ in various animal models of ischemic stroke.

Moreover, we analysed the M1/M2 polarization of CD68+ cells using iNOS and CD206. Interestingly, CD206 mRNA and protein expression, in accordance with the increased expression of TGFβ, is detected at 1~3 days, peaks at 3~5 days, and gradually diminishes at 14 days after MCAO [13]. Notably, although CD206 expression decreases in the ischemic area between 5 and 14 days after ischemia, TGFβ expression increases in CD68-expressing cells. These findings suggest that most of the TGFβ is produced by CD68-expressing microglia/macrophages but not by CD206-expressing cells in the chronic stage after stroke.

iNOS is one of the isoforms of NOS, an enzyme family which includes endothelial NOS (eNOS) and neuronal NOS (nNOS) [36]. This enzyme is expressed in the macrophages/microglia, astrocytes, and various tumor cells in response to pro-inflammatory cytokines or endotoxin, and is primarily considered as a marker of M1 macrophage polarization. In our study, despite the relatively few detected iNOS+ cells, 10~34% of iNOS was co-expressed in the CD68-expressing cells in the ipsilateral hemisphere after the subacute stage, suggesting that their polarization corresponds to the M1 phenotype. According to previous studies on microglia [37, 38], these chronic M1 macrophages phagocytize the cellular debris and clear the damaged tissue in the chronic stages of stroke.

CD68 is a microglia/macrophage marker related to lysosomal glycoproteins that shuttles in vesicles between lysosomes, endosomes, and the plasma membrane [39, 40]. For this reason, various studies [41-43], in addition to our results, detected CD68 staining in the cytosol.

Our data suggest that CD68-specific cells can be considered blood-derived macrophages. Previous studies showed that blood-derived macrophages were abundantly expressed 3~7 days after MCAO, although it was difficult to distinguish them from CD68+ microglial cells [44, 45]. Subsequent studies using green fluorescent protein transgenic mice or microglia-specific markers [46] have resolved this issue [47, 48].

A study using a Rgs5gfp/+ mouse model has shown that pericytes are recruited from the blood vessels and differentiate into microglial cells [49]. In particular, activated pericytes located on the capillary wall migrate to the lesion 7 days after infarction and express several microglial markers (including CD11b, Iba1, and galectin-3) at 7~21 days after MCAO. In fact, the same study also demonstrated that the pericytes may not correlate with CD68+ cells at 1~7 days after ischemic stroke. Thus, our data collectively suggest that the proliferating CD68− (Fig. 7C) or Iba1+ microglial cell (Fig. 8) can be considered as pericyte-derived microglia/macrophages.

MRI protocols, including ADC, T1, T2, DWI, and FLAIR imaging, are highly dependent on the occlusion and reperfusion time during ischemic stroke, especially in the acute periods after ischemic cerebral infarction [50]. Therefore, suitable MRI sequences are required for use in MCAO animal models. Among these sequences, ADC and DWI exhibit high contrast in the hyperacute and acute stages of stroke but are not useful in the late stages [51]; conversely, the FLAIR sequence is a reliable method in the chronic stage [52, 53]. Consequently, in the present study we employed FLAIR imaging to measure infarct volumes and their association with immunohistochemical factors after 24 hours post-reperfusion. It should be noted that we also identified ventriculomegaly in the contralateral hemisphere on FLAIR images (data not shown). Ventriculomegaly is a common finding in patients with stroke, traumatic injury, and infectious disease, although it is difficult to determine whether ventricular enlargement is related to hydrocephalus [54]. Previous studies which analysed the contralateral hemisphere damage, such as periventricle changes from astrocytic and microglial inflammation [55] did not report any significant effects on cell death.

IRW is widely utilized for analysis of positron emission tomography data based on the threshold of contrast using radioactive isotope injections (e.g., 11C and 18F); therefore, the same approach could be applied to our MRI data obtained from a non-human primate stroke model to quantify the 3D infarct volume. Indeed, lesions were successfully detected in FLAIR images using the IRW threshold, likely because of the high contrast in four ROIs (including the whole brain, infarct lesion, brain template, and infarction template). To our knowledge, this is the first study to semi-automatically determine the infarct volume from FLAIR images by equivalent thresholds. This method may be particularly useful in the clinical setting, with applications in examinations of the chronic stage of stroke.

In the present study, moreover, we analysed the proliferation patterns of CD68+, Iba1+ macrophage/microglia, and CD13+ pericytes. Specifically, several proliferating CD68+ cells were observed in the subacute stage. Interestingly, these cells were also found at specific time points in a number of other CNS diseases. For instance, 29% of the CD68+ cells co-expressed Ki67 on day 4 after the ischemic injury [56]. Moreover, they were observed on day 7 after spinal cord injury [57], or at week 3 after the induction of hypertension [58]. Additionally, this hypertensive model showed a dramatic decrease in proliferating CD68+ cells at week 4. Since proliferating CD68+ cells have not been previously reported in the MCAO model of rhesus monkey, this expression pattern could be valuable information.

The present study provides evidence for a novel approach to treating stroke after the subacute stage (2 weeks~20 months). Specifically, because the activity of CD206+ M2-type microglia/ macrophages decreased during this time frame, activated TGFβ-secreting CD68 cells may exert anti-inflammatory effects. Furthermore, because almost all neurogenesis-promoting chemicals have poor blood-brain barrier permeability, regulation of the endogenous CD68+ cells may be an effective alternative treatment strategy. For instance, intranasal treatment with TGFβ increases the density of doublecortin-positive migrating neuroblasts and NeuN+ mature neuronal cells in the subventricular zone (SVZ) and the striatum in the MCAO mouse model [33]. This treatment also significantly reduces the infarct volume and improves functional outcomes, as measured with the modified Neurological Severity Scores test. Therefore, additional investigation of anti-inflammatory activity in the infarct area will further our understanding of the role of TGFβ-secreting CD68 cells in the brain after ischemic damage.

There were several limitations in our study. First, only two experimental animals were present in each group, for analysis, at the respective time points after stroke. Secondly, CD68 may not be representative of all macrophages. A recent report summarized various M1/M2 (or M0) type markers based on the microenvironments [59], suggesting 12 markers (CX3CR1, CD11b, CD45hi, CD45low, MERTK, MHC class IIhi, MHC class IIlow, TMEM119, P2RY12, SALL1, CD206, and CD163) that can be used to distinguish between 4 cell types (meningeal macrophages, perivascular macrophages, parenchymal endogenous microglia, and choroid plexus macrophages). Thirdly, each animal was induced different occlusion time, since it was dependent on plateaued ADC-derived volume of the focal ischemia from our previous MRI study [15]. For instance, the infarct volume of animal R326 was significantly larger than in others animals, potentially resulting in greater induction of anti-inflammatory processes. Additionally, duration of recovered infarct volume or behavioral function could be different from other reports [60, 61]. However, since our stroke model is supposed to be diffusion-perfusion matched, it is worth reducing the overestimation of the infarct core by including part of the penumbra.

The present study revealed the presence of TGFβ-secreting CD68 cells after subacute ischemic brain damage. Our findings suggest that TGFβ-secreting CD68 cells may be used as a potential therapeutic target, instead of CD206+ cells. However, further in vivo studies are needed to illustrate the beneficial effects of TGFβ expressed by CD68-expressing cells. Moreover, pre-clinical experiments, including behavioral assessments for hemiplegia, determination of infarct volume reductions, and examinations of the promotion of neurogenesis by CD68+ cells in the non-human primate MCAO model of stroke, are required.