Abstract Background: Oxygen supplementation in myocardial infarction (MI) remains controversial. Inflammation is widely believed to play a central role in myocardial repair. A better understanding of these processes may lead to the design of novel strategies complementary to MI treatment. Methods: To investigate the role of hypoxia in inflammation and myocardial repair after acute MI, we placed MI mice in a tolerable mild hypoxia (10% O[2]) chamber for 7 days and then transferred the mice to ambient air for another 3 weeks. Results: We found that the cumulative survival rate of the MI mice under hypoxia was significantly higher than that under oxygen supplementation. Hypoxia promoted postinfarction myocardial repair. Importantly, we found that hypoxia modulated the phenotypic transition of blood monocytes from pro-inflammatory to pro-reparative in a timely manner, leading to the subsequent discontinuation of inflammation in myocardial tissues and promotion of myocardial repair post-MI. Specifically, cultured bone marrow-derived macrophages (BMDMs) primed by hypoxia in vitro exhibited improved reparative capacities and differed from M[1] and M[2] macrophages through the AMPKα2 signaling pathway. The deletion of AMPKα2 in monocytes/macrophages prevented the phenotypic transition induced by hypoxia and could not promote myocardial repair after MI when transplanted into the myocardium. Conclusions: Taken together, our work demonstrates that hypoxia promotes postinfarction myocardial repair by modulating the blood monocyte/macrophage phenotypic transition from pro-inflammatory to pro-reparative in a timely manner through the AMPKα2 signaling pathway. Hypoxia priming might be an attractive translational strategy for MI treatment by amplifying immune cells during early inflammation and subsequent resolution and repair. Keywords: hypoxia, myocardial infarction, monocytes/macrophages, phenotypic transition, AMPKα2 Introduction A large population of inflammatory cells, including neutrophils and monocytes, are mobilized to the myocardium during acute myocardial infarction (AMI) [41]^1. This process occurs in a time-dependent manner, and the rapid infiltration of neutrophils is followed by an influx of monocytes [42]^2. Monocytes/macrophages play different roles during early inflammatory and late repair processes [43]^3^, [44]^4. However, the specific environmental cues that induce monocyte/macrophage polarization and promote cardiac repair after AMI remain unclear [45]^5. Oxygen supplementation has been a cornerstone of supportive care in patients suspected of having AMI for more than a century and is widely endorsed by international guidelines [46]^6^, [47]^7. However, clinical studies have increasingly confirmed that oxygen supplementation has no beneficial effects when administered to ST-elevation myocardial infarction (STEMI) patients with no hypoxemia [48]^8^, [49]^9. Moreover, some studies proposed that the administration of oxygen supplementation therapy to acutely ill patients could be toxic and increase mortality and morbidity [50]^10. Recently, studies have confirmed that hypoxia is a major regulatory factor responsible for maintaining the proliferative capacity of cardiomyocytes in neonatal mice and inducing the regeneration of cardiomyocytes in adult mice [51]^11^-[52]^13. Hypoxia can promote macrophage phenotypic transition to a specific type or the M[2] phenotype in solid tumors [53]^14. Therefore, the role of hypoxia in heart recovery after MI seems to be protective, and further studies are needed to confirm this phenomenon. Adenosine 5'-monophosphate (AMP)-activated protein kinase (AMPK) is a highly conserved, key regulator of intracellular energy homeostasis. The catalytic α subunit has the following two isoforms: α1 is localized to the cytosol, while α2 can translocate to the nucleus [54]^15. AMPKα2 has been shown to regulate the stability of hypoxia-inducible factor-1α (HIF-1α) and neutrophil survival, thereby determining further myeloid cell recruitment and repair potential after hindlimb ischemia [55]^16. AMPK is upregulated under hypoxic conditions and promotes cardiomyocyte adaptation to chronic hypoxia [56]^17. However, the role of AMPK in modulating the functions of monocytes/macrophages under AMI is still largely unknown. In the present study, we investigated the role of hypoxia in cardiac repair after MI and the mechanism involved. Methods Study Approval The Institutional Animal Care and Use Committee of Army Medical University (Shapingba District, Chongqing, China) approved all animal care and experimental procedures prior to the commencement of this study (AMUWEC2020666). The authors declare that all supporting data are available within the article. Experimental Protocols, Animals, and Surgical Procedures Eight- to twelve-week-old male C57BL/6 mice from Charles River Laboratories (Stock No: 219) were used for the in vivo and in vitro experimental protocols. The mice were subjected to general anesthesia with isoflurane, and then, a thoracotomy was performed. A 7-0 silk suture was used to permanently ligate the LAD. The animals were allowed to recover under aseptic conditions and received analgesic medication (buprenorphine, 0.1 mg/kg s.c.) to reduce postoperative pain. CX3CR1-GFP BM-derived macrophages were isolated from CX3CR-1^GFP knock-in mice from The Jackson Laboratory (Stock No: 005582). CX3CR1-GFP BM-derived macrophages (1×10^6) or phosphate buffered saline (PBS) were injected at 3 different sites along the infarct border zone at a final volume of 10 µL in each site. Clodronate liposomes (dichloroethylene diphosphonate [Cl2MDP]) were injected through the caudal vein to deplete systemic macrophages. All operated mice were anesthetized with an intraperitoneal injection of sodium pentobarbital (80 mg/kg) and then euthanized by cervical dislocation. Cardiac Functional Measurements The mice were anesthetized by isoflurane. Transthoracic echocardiography was performed to evaluate the cardiac function. The measurements of the LV end-systolic dimension and LV end-diastolic dimension were obtained through two-dimensional short and long axes. The ejection fraction and fraction shortening were calculated ([57]Table S1, S2). After measuring the heart function by echocardiography, the mice were immediately euthanized by cervical dislocation, and the hearts were collected and randomly divided for different assays in further experiments. Tissue Harvesting Heparin (10 IU/g) was administered through an intraperitoneal (i.p.) injection 30 min before anesthesia. Then, the mice were deeply anesthetized with isoflurane. The abdominal cavity was opened, and the inferior vena cava was separated. Then, 500 μL of saturated potassium chloride solution (KCl) were injected through the inferior vena cava to induce heart arrest in the diastolic phase. Next, the heart was excised and washed with PBS on ice, and the connective tissue was quickly removed. The heart was fixed in 4% paraformaldehyde for paraffin-cut sectioning or embedded in OCT compound and stored at -80 °C until sectioning. Sectioning commenced from the apical part, and each heart slice was cut at a 6 μm thickness. Serial slices were obtained from 12 equally distant (300 μm) regions originating from the heart apex. Histology, Immunohistochemistry, and Immunocytochemistry Masson's trichrome staining. Paraffin-cut sections were stained according to the manufacturer's protocol and imaged under a microscope. Morphometric analyses of the infarcted tissue were performed using ImageJ software. Infarct size measurements were performed with the assistance of MI Quant software. Picrosirius red staining and polarized light microscopy. Paraffin-cut heart sections were stained according to the manufacturer's protocol (Abcam). The sections were digitized using an Olympus slide scanner. Fibrosis was quantified as a picrosirius red-positive area. The red-orange collagen area was compared with the green area in fibrosis. Immunohistochemistry. Frozen slices were fixed with 4% PFA and blocked with bovine serum albumin (BSA). The primary antibodies are listed in [58]Table S3. To detect apoptotic cardiomyocytes, a TdT dUDP nick-end labeling assay (TUNEL, Roche) was performed according to the manufacturer's protocol, and the samples were stained with cTnT and DAPI. Bone Marrow-derived Monocyte (BMDM) Isolation and Macrophage Differentiation Femurs were isolated from 8- to 12-week-old C57BL/6 mice. The bone marrow (BM) was isolated, flushed with PBS, and filtered through a 70-μm mesh. A red blood cell (RBC) lysate was used to remove RBC. The bone marrow cells were washed, centrifuged and resuspended for plating. After 3 days, the media were exchanged. The BMDMs were incubated overnight between days 7 and 8 to polarize toward normoxic macrophages. On day 3 after the media change, for the hypoxia treatment, the macrophages were induced in a 1% O[2] and 5% CO[2] cell incubator. The positive control for the hypoxic macrophages was stimulated with CoCl[2]. On day 7, the medium was changed. New growth medium containing 10% FBS and 100 ng/mL LPS with 50 ng/mL IFN-γ was used for the M[1] activation, while a medium containing 10% FBS with 10 ng/mL IL-4 and 10 ng/mL IL-13 was used for the M[2] activation. Polarized activated macrophages were harvested for the gene expression examination after 24 h of stimulation. A flow cytometry analysis of these cells was performed 48 h after the stimulation. Macrophage Migration Assay Migration of macrophages through 8-μm pores were assessed using a Transwell® Cell Culture chamber (Corning Costar, NY, USA). New medium supplemented with 15% fetal bovine serum (FBS) was added to the lower chamber and 1 × 10^4 cells in 100 μL of serum-free medium were added to the upper chamber and incubated for 24 h at 37 °C. After removing the non-migrated cells from the upper surface of the membrane, the cells that moved through the pores were fixed in 4% paraformaldehyde and stained with 1% Giemsa blue (Sigma-Aldrich). The membranes were photographed and cells were counted. Cell Isolation and Flow Cytometry The hearts were perfused with 4 °C PBS buffer. The infarct zone and border zone were separated and gently minced into 1-mm^3 granules and digested using Collagenase II. The digested material was filtered through a 200-mesh screen filter and centrifuged at 1000 rpm for 5 min at 4 °C. The red blood cells were lysed and then resuspended in FACS buffer. The suspended cells were incubated with conjugated antibodies ([59]Table S4) for 30 min at 4 °C protected from light. Peripheral blood was collected through the abdominal aorta. Leukocytes were washed and resuspended in FACS buffer. All conjugated antibodies used in this study are listed in [60]Table S4. The analysis was performed using a BD FACS Verse flow cytometer and FlowJo 10.0 software. Protein and RNA Isolation Protein. At the appropriate time point, the macrophages were harvested and rinsed with PBS. Cell lysis buffer was used to lyse the macrophages on ice for 30 min. It was necessary to scrape the culture plates on ice. The lysates were centrifuged, and the supernatant containing the sample protein was collected. The concentrations were measured using a BCA assay. RNA. The infarct zone and border zone were separated from the heart and gridded in liquid nitrogen. TRIzol was added to the mouse heart tissue, which was stored for a long time until use at -80 °C. The macrophages were washed twice and collected for the RNA isolation using TRIzol (1×10^6 cells). The following steps were performed according to the manufacturer's protocol. Quantitative RT-PCR SYBR Green was used to compare the gene profile levels under different processing conditions following normoxia and hypoxia. cDNA was first synthesized from mRNA using a PrimeScript^TM RT reagent kit according to the manufacturer's protocol. The resulting cDNA was standardized across the samples depending on the sample concentration. Then, the gene profile was amplified over the course of 30 cycles and analyzed by the ∆∆CT method. Primer sets predesigned for the following genes were purchased from Invitrogen. The sequences are listed in [61]Table S5 and S6. Macrophage Gene Array Library construction and sequencing. The total RNA was extracted from the cells/tissues using TRIzol according to the manufacturer's protocol, and ribosomal RNA was removed using a Ribo-Zero™ kit. Fragmented RNA was subjected to first- and second-strand cDNA synthesis, followed by adaptor ligation and enrichment with a low cycle according to the instructions of the NEBNext® Ultra™ RNA Library Prep Kit for Illumina. The purified library products were evaluated using an Agilent 2200 TapeStation and Qubit®2.0 (Life Technologies, USA). The libraries were paired-end sequenced (PE150, sequencing reads were 150 bp) at Guangzhou RiboBio Co., Ltd. (Guangzhou, China) using an Illumina HiSeq 3000 platform. Western Blot Analysis Equal amounts of protein samples were loaded for gel electrophoresis according to the manufacturer's protocol. Briefly, the proteins were separated through SDS-PAGE and then transferred to polyvinylidene fluoride membranes. The membranes were incubated overnight with primary antibodies, followed immediately by secondary antibody incubation. A Western blot imaging system was used to show chemiluminescence to reveal immunoreactivity. The gray value was analyzed by ImageJ software. Statistical Analysis The data are expressed as the mean ± standard deviation (SD) or number (percentage) and were analyzed by GraphPad Prism 8.0 software and SPSS 26.0 software. Unpaired t-test, Mann-Whitney test, analysis of variance (ANOVA) followed by Sidak's multiple comparisons or Kruskal-Wallis test followed by Dunn's posttest for correction were used to evaluate the differences between the groups. The sample capacity estimation was performed using SPSS 26.0 software. The Kaplan-Meier method was used to estimate the survival curves, and the log-rank test was performed to examine the comparisons between the groups. The differences were considered statistically significant only when the P-value was less than 0.05. Results Hypoxia Promotes Murine Cardiac Repair and Survival after MI We first evaluated whether mice could tolerate 10% O[2] conditions for a long period. We found that the survival rate of the MI mice under long-term hypoxia conditions was significantly lower than that of the mice under ambient air conditions ([62]Figure S1A). The heart weight did not significantly differ between the two groups of mice ([63]Figure S1B), but the lung weight was increased under hypoxia ([64]Figure S1C). Meanwhile, the tibia length and food intake were reduced in the MI mice under the hypoxic condition ([65]Figure S1D-E). Even though we provided equivalent food to the MI mice that received ambient air and the MI mice that underwent hypoxia, the reductions in body weight were more obvious in the hypoxic MI mice 28 days after MI ([66]Figure S1F). Thus, we chose to expose mice to 10% O[2] for 7 days immediately after MI (Figure [67]1A). The body weights and food intake were comparable between the MI mice exposed to hypoxia and those exposed to ambient air ([68]Figure S2A-B). To study the toxic effect of hyperoxemia on postinfarction myocardial repair, we subjected another group of mice to 33% O[2] to mimic hyperoxia for 7 days and then transferred these mice to ambient air for another 21 days (Figure [69]1A). On day 28, the survival rate of the hypoxia-treated mice (approximately 80%) was significantly higher than that of the ambient air-treated mice (approximately 53%, p < 0.05), while the survival rate of the hyperoxia-treated mice (approximately 33%) was significantly lower (Figure [70]1B, p < 0.01) than that of the normoxia-treated MI mice. Four weeks after MI, 11 of 30 ambient air-treated mice (36.67%), 4 of 30 hypoxia-treated mice (13.33%), and 13 of 30 hyperoxia-treated mice (43.33%) had died with signs of heart failure ([71]Figure S2C). Rupture deaths were observed less frequently in our results and were not significantly affected by different conditions ([72]Figure S2D). Moreover, the hypoxia-treated mice demonstrated significantly less cardiac compensatory hypertrophy, which was measured as the heart weight-to-body weight ratio, than the ambient air-treated mice (Figure [73]1C-D). The heart dimensions and function were evaluated, and compared to the normoxic MI mice, the left ventricular (LV) dimension was smaller, and heart function was better in the hypoxic MI mice (Figure [74]1E and [75]Table S1). Sequential heart sections from the apex to the ligation point showed that the thickness of the LV free wall was less reduced in the hypoxia-treated mice compared with that in the ambient air-treated mice. The scar size and LV compensatory hypertrophy were changed in the same manner as the thickness of the LV free wall (Figure [76]1F-G and [77]Figure S3A-B). Collagen deposition was measured by picrosirius red under polarized light microscopy, and the tightly packed versus loosely packed fiber ratio (red-orange: green) in the infarcts and border zones in the hypoxic MI mice was significantly lower than that in the normoxic MI mice (Figure [78]1H-I and [79]Figure S4A-C). Figure 1. [80]Figure 1 [81]Open in a new tab Hypoxia promotes postinfarction myocardial repair in mice. (A) Mice were exposed to 10% O[2] after LAD ligation-induced MI, which was then maintained for 7 days, and then, the mice were subjected to normoxia (21% O[2]) for 21 days. Hearts were harvested 28 days after MI. (B) Cumulative survival curve (Kaplan-Meier survival plot) of MI mice under hypoxia, normoxia and hyperoxia and sham-operated mice (n = 30 for the MI + hypoxia group, n = 30 for the MI + normoxia mice group, n = 30 for the MI + hyperoxia group, and n = 10 for the sham-operated group). (C) Representative results of trichrome staining of longitudinal heart sections after MI. Scale bar: 1 mm. (D) Heart weight-to-body weight (HW/BW) ratio in sham, MI + normoxic, MI + hypoxic and MI + hyperoxic mice. (E) Left ventricular ejection fraction (LVEF), fractional shortening (LVFS), left ventricular internal diameter at end-systole (LVID, s) and left ventricular volume at end-systole (LV Vol; s) were measured by echocardiography and are presented. (F) Schematic representation of left ventricle (LV) sampling 8 mm from the apical region to the section. Trichrome staining of the transverse section is presented. (n = at least 3 per group). Scale bar: 1 mm. (G) Quantification of the fibrotic area relative to the myocardium in transverse sections. (H) Representative images of infarct areas stained with picrosirius red and visualized under polarized light. Scale bar: 100 μm. (I) Quantification of picrosirius red polarized light analysis in the infarct areas of MI mice. Dot-plots represent data from individual mice. Statistical significance was determined by log-rank test (B), ANOVA followed by Sidak's multiple comparisons test (D, E) or Kruskal-Wallis test followed by Dunn's posttest to correct for multiple comparisons (G, I). *P < 0.05, **P < 0.01 and ***P < 0.001 compared to the corresponding control. Hypoxia Mitigates Cardiomyocyte Apoptosis and Promotes Myocardial Repair after MI We further examined cell death in the border zone at different time points after MI. There was no significant difference in the number of TUNEL-positive cardiomyocytes at the border zone during the first 5 days after MI between the hypoxic and normoxic mice. The number of TUNEL-positive cardiomyocytes was strikingly reduced in the MI mice treated with hypoxia on the 7th day after MI (Figure [82]2A-B). The cardiomyocyte size, which was determined by wheat germ agglutinin (WGA) staining, in the hypoxic group was significantly smaller than that in the normoxic or hyperoxic group after MI (Figure [83]2C-D). The vessel density in the border zone in the MI mice subjected to hypoxia was also higher than that in the MI mice subjected to normoxia or hyperoxia (Figure [84]2E-F and [85]Figure S5A-B). There was a significant trend toward decreased fibroblast proliferation in the infarct area in the hypoxic group compared to the normoxic or hyperoxic group after MI (Figure [86]2G-H and [87]Figure S4D). As hypoxia promotes cardiomyocyte re-entry into the proliferation cycle in adult mice, we measured the expression of phosphorylated histone H3 Ser10 (pH3), which is a mitosis marker in the heart, on day 28 after MI. The number of pH3-positive cardiomyocytes was increased in the MI mice under hypoxia conditions (Figure [88]2I-J and [89]Figure S5C). Aurora B kinase-positive cardiomyocytes, which are markers of cytokinesis, were also increased in the hypoxia-treated mice (Figure [90]2K-L and [91]Figure S5D). Figure 2. [92]Figure 2 [93]Open in a new tab Hypoxia mitigated cardiomyocyte apoptosis, induced angiogenesis and promoted cardiomyocyte proliferation. (A) Representative immunofluorescence images of TUNEL-stained heart tissue from the border zones of normoxia- and hypoxia-treated MI mouse hearts. (B) Quantitative assessment of cardiomyocytes in A and similar images revealed reduced TUNEL positivity in the hypoxia-treated MI mouse hearts at different time points (n = 3 at each time point). (C) Representative immunofluorescence images of wheat germ agglutinin (WGA)-stained heart tissue in the border zone. (D) Pooled analyses of the cardiomyocyte size. (E) Representative immunofluorescence images of CD31-stained heart tissue in the border zone. (F) Quantification of CD31 positivity surrounding cardiomyocytes. (G) Representative images of coimmunofluorescent staining of proliferating cardiac fibroblasts in the infarct area of mice under normoxia, hypoxia and hyperoxia 7 days postinfarction (MI). (H) Quantification of proliferating cardiac fibroblasts in the infarct area of mice. (I) Representative immunofluorescence images of coimmunostaining with anti-pH3 and anti-cTnT antibodies in the border zones of MI hearts. (J) Quantification of pH3+ cardiomyocytes after MI in the hypoxia and normoxia groups. (K) Representative immunofluorescence images of coimmunostaining with anti-Aurora B and anti-cTnT antibodies in the border zones of MI hearts. (L) Quantification of Aurora B+ cardiomyocytes after MI in the hypoxia and normoxia groups. Dot-plots represent data from individual mice. Statistical significance was determined by ANOVA followed by Sidak's multiple comparisons test. *P < 0.05, **P < 0.01 and ***P < 0.001 compared to the corresponding MI+normoxia. Scale bar: 50 μm. Hypoxia Modulates the Ratio of Pro-inflammatory to Pro-reparative Monocytes/Macrophages in Blood and Injured Myocardial Tissue To determine whether the systemic inflammatory reaction of monocytes was upregulated under hypoxia in our study, we analyzed the inflammatory subtype of monocytes by staining harvested blood cells for lymphocyte antigen 6 complex locus C (Ly6C). The gating strategy for monocyte identification in blood is shown in [94]Figure S6A. Ly6C^high monocytes are generally considered a pro-inflammatory subtype, while Ly6C^low monocytes are considered a subtype associated with the resolution of inflammation and the propagation of repair [95]^14. There was no difference in the ratio of Ly6C^high cells during the first to third days after MI between the mice exposed to ambient air and those exposed to hypoxia. However, the ratio of Ly6C^low cells in the hypoxic group was strikingly higher than that in the ambient air group on the 5th day after MI (Figure [96]3A-B), and representative flow cytometric results at different time points are shown in [97]Figure S6B. Similarly, the ratio of tissue Ly6C^low monocytes/macrophages was also significantly increased on the 5th day after MI in heart tissue from the mice under hypoxia (Figure [98]3C-D). The gating strategy and representative flow cytometric results at different time points are shown in [99]Figure S7A-B. These results are consistent with the apoptosis level measured in injured myocardium as there was no significant difference in the first 5 days, but the apoptosis level was reduced after 7 days of hypoxia (Figure [100]2B). Figure 3. [101]Figure 3 [102]Open in a new tab Systemic hypoxia promoted monocyte/macrophage phenotypic transitions. (A) Representative flow cytometric analysis of blood monocytes 5 days after MI under normoxia or hypoxia. (B) Ratios of Ly6C^high and Ly6C^low blood monocytes among all blood monocytes (n=3 per group at each time point). (C) Representative flow cytometric analysis of tissue monocytes/macrophages 5 days after MI under normoxia or hypoxia. (D) Ratios of Ly6C^high and Ly6C^low tissue monocytes among all monocytes (n=3 per group at each time point). (E) Representative immunofluorescence images of coimmunostaining with anti-CCR2 and anti-F4/80 antibodies within the infarct zone over 14 days in mice after LAD ligation. Scale bar: 50 μm. (F) Cell counts of macrophages in the infarct area in each field at various time points after MI in the normoxia or hypoxia group (n = 3 per group). (G) No difference was observed in the ratio of CCR2-positive macrophages in the MI mouse hearts between the hypoxia and normoxia groups. (H) Pooled flow cytometry data from infarcted mouse tissue revealed no difference in the CCR2+ macrophage population between the normoxia- and hypoxia-treated MI hearts. (I) Protein expression of inflammatory cytokines in the infarct zones of hearts treated with hypoxia 3 days after LAD ligation (n = 3 per group). (J) Protein expression of inflammatory cytokines in the infarct zones of hearts treated with hypoxia 7 days after LAD ligation (n = 3 per group). Dot-plots represent data from individual mice. Statistical significance was determined by a Mann-Whitney test (B, D, F, I, J) or unpaired t-test (H). ^NSP > 0.05, *P < 0.05, **P < 0.01 and ***P < 0.001 compared to the corresponding MI+normoxia group. Furthermore, we found that there was no significant change in the numbers of monocytes in the blood and monocytes/macrophages in heart tissue subjected to hypoxia after MI ([103]Figure S6C and [104]Figure S7C). Meanwhile, the ratio of Ly6C^low splenic monocytes in total blood monocytes in the hypoxic group was higher than that in the ambient air group on the 5th day after MI ([105]Figure S8A-C), which is consistent with the changes we observed in blood (Figure [106]3A-B). Moreover, we detected the effect of hypoxia on myelopoiesis in the spleen and bone marrow and found that systemic hypoxia did not exert a major impact on myelopoiesis in the bone marrow and spleen ([107]Figure S8D-I). F4/80^+ macrophage accumulation peaked at approximately 5 days after MI and then rapidly decreased on approximately the 7th day after MI, and the hypoxia treatment had no impact on this process (Figure [108]3E-F). To further characterize the macrophage population, we detected M[1] and M[2] macrophage infiltration into the myocardium over time after MI. We found that hypoxia had no impact on the number of M[1] and M[2] macrophages in the infarct area ([109]Figure S9A-D). C-C motif chemokine receptor 2 (CCR2) was used to distinguish the monocyte-derived macrophages (CCR2^+) from the resident macrophages (CCR2^-) [110]^18. Laser confocal microscopy and flow cytometry showed that CCR2^+ macrophages were the overwhelming cell type in the early stage after MI (Figure [111]3E-H and [112]Figure S10A). Next, we measured the expression of cytokines associated with inflammation in the ischemic zone in the MI hearts. On the third day after MI, hypoxia significantly inhibited chemokine (C-C motif) ligand 2 (CCL2) expression, which was associated with inflammation (Figure [113]3I) [114]^19. On the 7^th day after MI, interleukin-13 (IL-13), chemokine (C-C motif) ligand 5 (CCL5) and chemokine (C-C motif) ligand 20 (CCL20, also known as MIP-3a) were decreased in the hypoxia-treated MI hearts, while matrix metalloproteinase-8 (MMP8) and chemokine (C-X-C motif) ligand 7 (CXCL7) were upregulated by hypoxia (Figure [115]3J) [116]^20. Accordingly, as higher Ly6C^low content would be consistent with efficacious inflammation resolution, we therefore examined dynamic changes of inflammatory cytokines, like IL-1β, Il-1α, IL-6, IL-4, Nos2, Arg-1 and IL-10. We found the level of IL-1β, Il-1α, IL-6 and Nos2 declined in hypoxia-treated group after MI ([117]Figure S11A). In the contrast, Arg-1 and IL-10, increased in hypoxia-treated group after MI on day 5 and day 7 ([118]Figure S11B). These results confirm that hypoxia modulates the ratio of reparative monocytes/macrophages in both the blood and injured myocardial tissue during the late resolution of inflammation and propagates repair with no significant effects on the pro-inflammatory functions of monocytes/macrophages during the early period. Systemic Depletion of Macrophages Using Clodronate Reduces the Efficacy of Hypoxia after MI We tested whether the systemic depletion of macrophages could recapitulate the benefits of hypoxia-induced cardioprotection to establish the importance of macrophages in mediating hypoxia-induced cardiac protection. We administered clodronate (dichloromethylene diphosphonate [Cl2MDP]) liposomes immediately after MI via the caudal vein. Clodronate effectively reduced the spleen and heart macrophage populations after MI ([119]Figure S12A-B). Clodronate attenuated the benefits of hypoxia after MI as follows: we observed no differences in the morphology of the left ventricle between the normoxia- and hypoxia-treated groups ([120]Figure S12C-D). Echocardiography revealed LV aneurysms and mural thrombi in both groups ([121]Figure S12E). No obvious differences were observed in the left ventricular ejection fraction (LVEF) and left ventricular internal diameter at end-systole (LVID, s) measured using echocardiography ([122]Figure S12F). An even greater scar size was detected in the hypoxia-treated group compared with that in the normoxia-treated group ([123]Figure S12G-H). Hypoxia-Primed Monocytes/Macrophages Promote Postinfarction Myocardial Repair In Vivo To further clarify whether the monocyte/macrophage phenotypic transition was regulated by hypoxia, bone marrow cells were isolated and differentiated into macrophages (Figure [124]4A). The hypoxic macrophages (M[H] macrophages) displayed a circle-like morphology with reduced pseudopodia formation (Figure [125]4B and [126]Figure S13A-B). Meanwhile, hypoxia could enhance the migration ability of MH macrophages relative to MN macrophages ([127]Figure S13C). In the analysis of M[H] macrophages in a wide panel versus M[1] and M[2] macrophages, we found that the M[H] macrophages differed from the M[1] and M[2] macrophages ([128]Figure S1D-F). To trace the macrophages injected into the heart, we isolated and cultured monocytes / macrophages from CX3CR1-GFP mice ([129]Figure S14A-B). M[H] CX3CR1-GFP macrophages were transplanted into the myocardium immediately after left anterior descending coronary artery (LAD) ligation. The location of the CX3CR1-GFP macrophages was determined by co-immunostaining with anti-GFP and anti-F4/80 antibodies in the MI mice ([130]Figure S14C-E). We quantified the number and identified the location (infarct, border and remote) of the transplanted CX3CR1-GFP macrophages relative to all macrophages found in different regions of the heart at various time points to further evaluate the transplantation efficacy ([131]Figure S14F-G). Figure 4. [132]Figure 4 [133]Open in a new tab Hypoxia-primed monocytes/macrophages promote postinfarction myocardial repair in vivo. (A) Schematic protocol of intramyocardial injection. The animals were monitored for 28 days. (B) Representative laser confocal microscopy images of M[N]- and M[H]-polarized macrophages. Scale bar: 50 μm. (C) Cumulative survival curve (Kaplan-Meier survival plot) of MI mice after macrophage transplantation and sham-operated mice (n = 46 for MI followed by M[N] macrophage transfer, n = 36 for MI followed by M[H] macrophage transfer, n = 20 for MI followed by vehicle transfer, and n = 10 for sham-operated mice). (D) The heart weight-to-body weight (HW/BW) ratio was significantly decreased in the MI mice following the M[H] macrophage transfer. (E) Left ventricular ejection fraction (LVEF), fractional shortening (LVFS), left ventricular internal diameter at end-systole (LVID, s) and left ventricular volume at end-systole (LV, Vol, s) were measured by echocardiography and are presented. (F) Trichrome staining of longitudinal sections showed enlarged hearts after MI. Scale bar: 1 mm. (G) Quantification of the fibrotic area and LV thickness relative to the myocardium in transverse sections demonstrated a significant decrease in scar formation in the hypoxia-treated MI mice and an increase in scar formation in the hyperoxia-treated mice. (H) Representative images of infarct areas stained with picrosirius red visualized under polarized light. Scale bar: 100 μm. (I) Quantification of picrosirius red polarized light analysis in the infarct areas of MI mice. Dot-plots represent data from individual mice. Statistical significance was determined by a log-rank test (C), two-way ANOVA followed by Sidak's multiple comparisons test (D, E, G) or Kruskal-Wallis test followed by Dunn's posttest to correct for multiple comparisons (G). *P < 0.05, **P < 0.01 and ***P < 0.001 compared to the corresponding control. Compared with the normal macrophage transplantation, the M[H] macrophage transplantation improved the long-term survival rate after MI (Figure [134]4C). The M[H] macrophage transplantation effectively reduced ventricular remodeling and significantly decreased the heart weight-to-body weight ratio compared with those following normal macrophage transplantation (Figure [135]4D). Additionally, the ejection fraction (EF) and fractional shortening (FS) were preserved following the M[H] macrophage transplantation (Figure [136]4E and [137]Table S2). The LV size and morphology were also well maintained in the M[H] macrophage-transplanted mice compared to those in the normal macrophage-transplanted mice (Figure [138]4F and [139]Figure S15A). Additionally, a reduction in the scar size was observed in the M[H] macrophage-transplanted mouse hearts (Figure [140]4G and [141]Figure S15A). The tightly packed versus loosely packed fiber ratio was significantly lower in the infarcts and border zones in the M[H] macrophage-transplanted mouse hearts (Figure [142]4H-I and [143]Figure S16A-C). Moreover, fibroblast proliferation in the infarct area in the M[H] macrophage-transplanted mouse hearts was lower than that in the other groups ([144]Figure S16D). More capillaries and pH3-positive cardiomyocytes were observed surrounding the border zone in the MI mice transplanted with the M[H] macrophages compared to those in the mice transplanted with normal macrophages ([145]Figure S17A-B). These results strongly suggest that isolated monocytes/macrophages treated with hypoxia exerted a protective effect on postinfarction myocardial repair. Hypoxia Polarizes Unstimulated Bone Marrow-Derived Macrophages to a Pro-reparative Phenotype The M[H] macrophages differed from the M[1] and M[2] macrophages ([146]Figure S13A-E). A gene analysis was performed to distinguish the M[H] macrophages from the M[1] and M[2] macrophages. In total, 583 genes were upregulated, while 469 genes were downregulated in the M[H] macrophages compared to those in the M[1] macrophages. Compared to the M[2] macrophages, 165 genes were upregulated, and 248 genes were downregulated in the M[H] macrophages (Figure [147]5A and [148]Figure S18A-B). We filtered the genes upregulated in the M[H] macrophages compared to the other two subtypes. The heat map shows all upregulated genes (Figure [149]5B). The KEGG pathway enrichment analysis and Gene Oncology analysis indicated that the upregulated genes in the M[H] macrophages were associated with aspects of metabolism and environmental processing, such as hypoxia and nutrition depletion (Figure [150]5C-D). The protein interaction network analysis identified multiple functions of the M[H] macrophages, including metabolic regulation, paracrine regulation, and especially angiogenesis as vascular endothelial growth factor (VEGF) expression was significantly upregulated (Figure [151]5E). Regarding the downregulated genes in the M[H] macrophages, the protein interaction network analysis showed that CCL2, cluster of differentiation 274 (CD274, also known as programmed death-ligand 1 (PD-L1)) and interferon-induced protein 35 (IFI35) might be the core factors ([152]Figure S18C-E). Figure 5. [153]Figure 5 [154]Open in a new tab Hypoxia polarizes isolated macrophages to a reparative phenotype. (A) Volcano plot showing the different gene expression levels between M[1] macrophages and M[H] macrophages (left) or between M[2] macrophages and M[H] macrophages (right). (B) Heat map of upregulated gene expression in M[H] macrophages relative to those in M[1] and M[2] macrophages. (C) KEGG analysis of biological pathways associated with the genes upregulated in the M[H] macrophages relative to those in the M[1] and M[2] macrophages. (D) Functional enrichment analysis of genes upregulated in the M[H] macrophages relative to those in the M[1] and M[2] macrophages. (E) Protein interaction network of genes upregulated in the M[H] macrophages relative to those in the M[1] and M[2] macrophages. (F) Gene expression profiles of macrophages polarized toward the M[1], M[2], and M[H] phenotypes relative to M[N] macrophages. n = 3 per group. Statistical significance was determined by a Kruskal-Wallis test, followed by Dunn's posttest to correct for multiple comparisons. *P < 0.05, **P < 0.01 and ***P < 0.001 compared to corresponding M[N] macrophages. The gene expression of M[N] macrophages was set as the control panel. The expression levels of nitric oxide synthase 2 (Nos2), interleukin-1 alpha (IL-1α), interleukin-1β (IL-1β), interleukin-6 (IL-6) and tumor necrosis factor (TNF) in the M[H] macrophages were all lower than those in the M[1] macrophages but higher than those in the M[2] macrophages (Figure [155]5F). Meanwhile, arginase 1 (Arg-1), peroxisome proliferator-activated receptor gamma (Pparg) and transforming growth factor beta 1 (Tgfβ1) were also changed in the M[H] macrophages, and their expression levels were higher than those in the M[1] macrophages but lower than those in the M[2] macrophages (Figure [156]5F). Importantly, the M[H] macrophages expressed higher levels of IL-10, which is associated with anti-inflammation, than the M[1] and M[2] macrophages [157]^21 ([158]Figure S18F). Thus, these results indicate that hypoxia-primed macrophages transform into a phenotype that prone to promoting tissue repair, and this phenotype differs from that of M[1]and M[2] macrophages. Macrophages Were Modulated by Hypoxia through the AMPKα2 Signaling Pathway As metabolism- and stress-responsive genes were upregulated in the M[H] macrophages, we investigated whether AMPK participates in the development of hypoxia-primed macrophages. AMPKα1, which is a key regulator of macrophage skewing during skeletal muscle regeneration [159]^22, was not changed in the M[H] macrophages; however, AMPKα2 was significantly upregulated at both the gene and protein levels in the macrophages (Figure [160]6A-C and [161]Figure S19A-B). Thus, we postulated that the macrophages primed by hypoxia might be regulated through AMPKα2. As AMPKα2 has transcriptional regulation activity and is one of the most important regulators of hypoxia inducible factor 1α (HIF-1α) [162]^16, we measured the protein level of HIF-1α in the M[H] macrophages. We found that the protein levels of HIF-1α following both the hypoxia exposure and CoCl[2] treatment, which mimics hypoxia, were hardly upregulated when AMPKα2 was abrogated (Figure [163]6D). Then, we isolated bone marrow cells from AMPKα2^-/- mice and cultured and induced these cells to differentiate into M[H] macrophages. We found that AMPKα2^-/- BMDMs exposed to hypoxia still exhibited more pseudopodia formation than normoxic cells (Figure [164]6E), which differed from the effect on wild-type (WT) BMDMs under hypoxia (Figure [165]4B). No significant changes in the gene expression profiles of general M[1] and M[2] macrophage markers were observed in the WT and AMPKα2^-/- BMDMs (Figure [166]6F). Additionally, the AMPKα2^-/- BMDMs showed no obvious phenotypic transition after exposure to hypoxia relative to normoxia (Figure [167]6G). Additionally, the WT BMDMs showed obvious phenotypic transition after exposure to hypoxia relative to the AMPKα2^-/- BMDMs ([168]Figure S20A). Figure 6. [169]Figure 6 [170]Open in a new tab Macrophages were polarized by hypoxia through the AMPKα2 signaling pathway. (A) Gene expression of AMPKα2 in M[N] macrophages and M[H] macrophages (n = 3). (B) Representative immunoblots showing AMPKα2 expression and pooled data. (C) Representative immunoblots showing HIF-1α expression in M[N] macrophages, M[H] macrophages and macrophages induced by CoCl[2]. (D) Representative immunoblots showing HIF-1α expression in M[N] macrophages, M[H] macrophages and CoCl[2]-induced macrophages from wild-type (WT) or AMPKα2-knockout (AMPKα2^-/-) mice. (E) Representative phase-contrast images of AMPKα2^-/- macrophages and pooled data showing the number of pseudopods in macrophages under normoxic and hypoxic conditions. Scale bar: 275 μm. (F) Gene expression profiles of normoxic macrophages from WT and AMPKα2^-/- mice (n = 3). (G) Gene expression profiles of normoxic or hypoxic AMPKα2^-/- macrophages (n = 3). (H) Cumulative survival curve (Kaplan-Meier survival plot) of MI mice following WT and AMPKα2^-/- M[H] macrophage transplantation (n = 14 for MI followed by WT M[H] macrophage transfer, n = 20 for MI followed by AMPKα2^-/- M[H] macrophage transfer). (I) Heart weight-to-body weight (HW/BW) ratio after MI. (J) LVEF, LVFS, LVID, s and LV Vol; s were measured by echocardiography and are presented. (K) The ratio of anti-CD31-positive cells to anti-cTnT-positive cells was significantly decreased in the MI mice following the AMPKα2^-/- macrophage transfer. Scale bar: 50 μm. (L) Coimmunostaining with anti-pH3 and anti-cTnT antibodies showed significantly decreased cardiomyocyte mitosis in the MI mice following the AMPKα2^-/- M[H] macrophage transfer. Scale bar: 50 μm. Dot-plots represent data from individual mice. Statistical significance was determined by a Mann-Whitney test (A, B, F, G), unpaired t-test (E, I, J, K, L) or log-rank test (H). *P < 0.05, **P < 0.01 and ***P < 0.001 compared to the corresponding WT control. After transplanting hypoxia-primed AMPKα2^-/- BMDMs into the myocardium after MI, we observed that after MI, the mice did not benefit from transplantation within 28 days, and the long-term survival rate did not significantly differ from that of the vehicle-transplanted mice, which was much lower than that in the hypoxia-primed WT BMDM transplantation group (Figure [171]6H). LV remodeling, which is indirectly expressed by the ratio of heart weight to body weight, was obvious (Figure [172]6I), and cardiac function remained low (Figure [173]6J). Angiogenesis surrounding the infarct area was crippled due to the AMPKα2^-/- BMDM transplantation (Figure [174]6K and [175]Figure S21A). The number of pH3-positive cardiomyocytes in the AMPKα2^-/- hypoxic BMDM-treated mice was lower than that in the WT BMDM-treated mice (Figure [176]6L). Discussion Since Steele et al first demonstrated that oxygen can alleviate angina pectoris a century ago, oxygen supplementation has become the standard treatment for patients with AMI. It appears quite logical and biologically plausible to give oxygen to patients with AMI to improve oxygenation in ischemic myocardial tissue and decrease ischemic pain. However, several clinical trials have confirmed that oxygen supplementation might be harmful or at least not beneficial for short-term or long-term mortality and increase the rehospitalization rate [177]^8^-[178]^10. Therefore, supplemental oxygen is not recommended for routine use in AMI patients without hypoxemia. However, without considering the possible systemic harmful effect of hypoxemia, whether hypoxemia is beneficial for heart recovery after AMI is unclear. In the present study, we found that systemic hypoxia could reduce the scar size, promote cardiomyocyte proliferation, and most importantly, promote heart function recovery and increase survival. Importantly, mild systemic hypoxia was tolerable in the mice after MI. To the best of our knowledge, this report is the first to show that mild hypoxia during the early period after AMI could promote myocardial infarct repair. Studies have confirmed the close relationship between hypoxia and cardiomyocyte proliferation. The transition to an oxygen-rich postnatal environment is a key factor resulting in the cell cycle arrest of cardiomyocytes [179]^11, which is consistent with the fact that neonatal mice gradually lose cardiomyocyte proliferation capacity in the first postnatal week [180]^12. In adult mice, when treated with a extremely low concentration of oxygen (7% O[2]) for approximately 2 weeks, cardiomyocyte regains proliferative abilities and promotes myocardial repair through cardiomyocyte proliferation [181]^13. These findings provide an interesting therapeutic strategy for AMI by promoting cardiomyocyte proliferation under hypoxia. In the current study, we found evidence of cardiomyocyte proliferation, such as H3 phosphorylation and positive staining for Aurora B kinase, in cardiomyocytes under hypoxia. Myocyte metabolism is a critical factor related to the oxygen supply and is intimately linked to the lack of oxygen supply promoting preferential glucose utilization over fatty acids as a more efficient supply of ATP. Adaptive metabolism promotes fetal gene expression, including GLUT1, to prioritize glucose utilization. A previous study showed that an increase in glucose metabolism promotes cardiac regeneration in the neonatal mouse heart [182]^23. Neonatal mice have been shown to regenerate their hearts during a transient window of time of approximately 1 week after birth [183]^24. A previous study showed that the hypoxic nature of the zebrafish external and circulatory environments prevents the activation of the DNA damage response and cell cycle arrest of myocytes. Mitochondrial ROS-mediated activation of the DNA damage response is an important upstream event that mediates cell cycle arrest in postnatal cardiomyocytes [184]^12. The maintenance of the regenerative capacity may be related to hypoxic conditions. We previously found that hypoxia could prolong the cardiomyocyte regeneration window in neonatal mice [185]^25. Meanwhile, cardiomyocyte proliferation in the cyanotic infant group was also observed to be significantly increased compared with that in the acyanotic infant group [186]^13. Furthermore, decreased mitochondrial content with corresponding changes in metabolites, decreased radical oxygen species (ROS), and decreased DNA damage were observed in hypoxic hearts [187]^26. Hypoxia can induce a switch in energy metabolism from mitochondrial oxidative phosphorylation to glycolysis [188]^27. These results suggest that cardiomyocyte metabolism is hindered under hypoxia, which might be another contributor to the attenuation of remodeling after MI. The inflammatory responses play crucial role in myocardial ischemic injury and repair. Early after MI, tissue necrosis initiates inflammation and dynamically recruits monocytes/macrophages. Infarct myocardial healing begins approximately 4 days after MI in murine models [189]^28. During the processes of myocardial injury and repair, monocytes/macrophages are vital in clearing necrotic tissue and tissue healing [190]^29. Any treatment that impairs or deletes macrophages will damage the process of myocardial repair [191]^30. Modulating the function of monocytes/macrophages in different ways has obtained complex results [192]^31^,[193]^32. In nonreperfusion MI, the early period of inflammation is critical for the clearance of necrotic cells. In the present study, we found that systemic tolerable hypoxia enhanced the monocyte/macrophage transition from the pro-inflammatory to the pro-reparative subtype on approximately the 5th day after MI. Importantly, this tolerable hypoxia promoted the monocyte phenotypic transition without affecting the pro-inflammatory effect in the first 3 days after MI. Therefore, this tolerable hypoxia might be an ideal strategy to promote myocardial infarct repair. A previous study showed that hypobaric hypoxia caused by exposure to altitude results in a significant reduction in the number of circulating peripheral dendritic cells [194]^33. Another study reported that circulating inflammatory monocytes were increased in hypoxic mice. In hypoxic mice, the percentage and number of circulating monocytes, including pro-inflammatory Ly6C^high monocytes, increased at different time points after hypoxic exposure [195]^34. In contrast, we found that under the specific context of MI, hypoxia could halt inflammation in a timely manner and promote cardiac repair. Moreover, hypoxia influences the proliferation and lineage differentiation of bone marrow hematopoietic stem cells. Whether hypoxia might have an impact on myelopoiesis in the spleen or bone marrow is worthy of attention. Myeloid cells were reported to be derived from the bone marrow, and the spleen drove a substantial increase in the number of monocytes in the blood following MI [196]^35. Monocytes are generated through two distinct cellular pathways. The earliest monocytes arise from granulocyte-monocyte progenitors (GMPs) and monocyte-dendritic cell progenitors (MDPs). GMPs and MDPs are proposed to arise from the hierarchical model of a common myeloid progenitor (CMP) [197]^36. In our additional experiments, we found no impact on GMPs and MDPs in either proliferation assays or absolute cell numbers. This finding might be related to the short time (7 days) of hypoxia treatment after MI, proving that relatively short period of hypoxia has few side effects on MI mice. The numbers and phenotypes of macrophages dynamically vary across different heart diseases. According to their functions and locations, different names have been used to distinguish macrophages. The terms “M[1] macrophage” and “M[2] macrophage” were recommended two decades ago to classify the macrophage subtypes. These terms were based on analyses of macrophages from C57BL/6 mice, and M[1] macrophages were induced by LPS and IFN-r via the STAT-1 pathway, while M[2] macrophages were induced by IL-4 via the STAT-6 signaling pathway. Our observations of macrophages revealed that M[H] macrophages were distinct from M[1] and M[2] macrophages. We found that M[H] macrophages possessed improved tissue repair abilities and weak inflammatory responses. Recent research shows that oxygen is immediately reduced after injury and that the phenotypic transition of macrophages occurs simultaneously [198]^37. We propose that hypoxia regulates the inflammatory response in the border zone of MI by altering the release of inflammatory factors, shifting from a pro-inflammatory to an anti-inflammatory environment. We also observed that hypoxia could upregulate genes related to macrophage skewing in myocardial tissue, strongly suggesting that hypoxia-regulated monocytes/macrophages might be critical for cardiac repair after MI. Importantly, we confirmed that this modulation was mainly based on blood monocytes and was not regulated by the tissue microenvironment. This finding offers a great opportunity for clinical translation as we could isolate monocytes/macrophages, stimulate them with hypoxia in vitro and use these hypoxia-primed monocytes/macrophages in vivo. The detailed molecular mechanisms of monocyte/macrophage responses to hypoxia are still largely unknown. We found that M[H] macrophages exhibited a “pooled” change in gene expression, mainly in genes associated with metabolic modulation and hypoxia. This finding is consistent with a previous report suggesting that metabolic modulation is critical for macrophage phenotypic transition [199]^38. Since AMPK is a key regulator of cellular energy metabolism, ROS redox balance and the interaction between HIF-1α and AMPKα have been reported in cancer cells [200]^39. Inhibiting the expression of AMPKα impaired the expression of HIF-1α in the nucleus under hypoxia or low glucose conditions. Studies have shown that AMPKα1 is a key molecule through which macrophages promote angiogenesis and tissue repair under normoxia and that the depletion of AMPKα1 impairs macrophage promotion of arteriogenesis [201]^40. AMPKα1 in fibroblasts was reported to function as a master regulator of cardiac fibrosis and remodeling after MI [202]^41. However, there have only been a few reports on the role of AMPKα2 in macrophages. In contrast to the AMPKα1 subunit, AMPKα2 can modulate gene and protein expression by translocating to the nucleus through many signaling pathways. In neutrophils, AMPKα2 regulates α-ketoglutarate generation, HIF-1α stability, and neutrophil survival, which, in turn, further facilitates myeloid cell recruitment and repair potential. In the present study, we found that AMPKα2, but not AMPKα1, was upregulated in hypoxia-primed monocytes/macrophages and that AMPKα2 was a key regulator of monocyte/macrophage phenotypic transition. The latest results demonstrated that the production of interleukin (IL)-10 by macrophages promotes anti-inflammatory functions and prevents fibrosis after tissue damage, which could lead to new therapeutic perspectives for inflammatory diseases [203]^42. In our study, M[H] macrophages expressed higher levels of IL-10 than M[1] and M[2] macrophages. IL-10 is considered to have a cardioprotective effect on improving the LV function and diminishing pathological remodeling [204]^43. Recombinant IL-10 could preserve cardiac function, attenuate maladaptive remodeling and improve long-term survival in mice [205]^44. IL-10 has been reported to increase the expression of intracellular galectin-3 through the activation of STAT3 in macrophages, which is essential for osteopontin-producing reparative macrophage polarization after myocardial infarction [206]^21. We believe that inflammatory factors, such as IL-10, may be the key mediators secreted by hypoxia-primed macrophages that exert cardioprotective effects. Currently, promising cardioprotective strategies for MI include the combination of ischemic postconditioning and remote ischemic preconditioning [207]^45, which aims to reduce the infarct size and attenuate adverse cardiac remodeling and progression to heart failure [208]^45. Meanwhile, clinical trials have reported that macrophage transplantation could be safe and feasible [209]^46^, [210]^47. These results provide the basis for future prospective randomized clinical trials and hinder the potential clinical applications and future prospects of our results. Conclusion Our data suggest that hypoxia promotes the monocyte/macrophage phenotypic transition from pro-inflammatory to pro-reparative in a timely manner and promotes postinfarction myocardial repair. Hypoxia priming might be an attractive translational strategy for MI treatment by amplifying immune cells during early inflammation and subsequent resolution and repair. Supplementary Material Supplementary figures and tables. [211]Click here for additional data file.^ (9.3MB, pdf) Acknowledgments