The cardiac lymphatic system stimulates resolution of inflammation following myocardial infarction

Myocardial infarction (MI) arising from obstruction of the coronary circulation engenders massive cardiomyocyte loss and replacement by non-contractile scar tissue, leading to pathological remodeling, dysfunction, and ultimately heart failure. This is presently a global health problem for which there is no effective cure. Following MI, the innate immune system directs the phagocytosis of dead cell debris in an effort to stimulate cell repopulation and tissue renewal. In the mammalian adult heart, however, the persistent influx of immune cells, coupled with the lack of an inherent regenerative capacity, results in cardiac fibrosis. Here, we reveal that stimulation of cardiac lymphangiogenesis with VEGF-C improves clearance of the acute inflammatory response after MI by trafficking immune cells to draining mediastinal lymph nodes (MLNs) in a process dependent on lymphatic vessel endothelial hyaluronan receptor 1 (LYVE-1). Deletion of Lyve1 in mice, preventing docking and transit of leukocytes through the lymphatic endothelium, results in exacerbation of chronic inflammation and long-term deterioration of cardiac function. Our findings support targeting of the lymphatic/immune cell axis as a therapeutic paradigm to promote immune modulation and heart repair.


Introduction
The lymphatic system is a network of vessels that pervades the entire body, complementary to the blood cardiocirculatory system. It comprises blind-ended capillaries that collect extravasated interstitial fluid, macromolecules, and leukocytes from the periphery of the body, preventing their accumulation in tissues, and transports them via lymph through larger collecting afferent vessels toward draining lymph nodes (1). These are secondary lymphoid organs, enriched for naive lymphocytes, that filter the lymph to detect foreign particles (antigens), triggering lymphocyte activation and an adaptive immune response (1,2). Lymph then flows from the nodes via efferent lymphatic vessels into larger lymphatic ducts, eventually being returned to the blood circulation, at the level of the subclavian veins. The systemic lymphatic network thus plays a critical role in tissue fluid regulation and immune surveillance during homeostasis (1).
Lymphatic vessel growth, or lymphangiogenesis, begins early during embryogenesis and is promoted by VEGF-C and VEGF-D signaling through their cognate receptor, VEGFR-3, which is expressed in both blood and lymphatic endothelium and becomes specified to the latter toward the end of development (1,3). Postnatally, lymphatic expansion is associated with wound healing and chronic inflammation (4). Previously, the majority of the studies have focused on peripheral tissue injury (for example, skin wounding; ref. 5), whereby following initiation of the inflammatory process, lymphatic endothelial cells (LECs) proliferate in response to VEGF-C and VEGF-D, leading to network expansion (reviewed in ref. 4). In this setting, activated LECs also secrete chemokines, including CCL21, to attract antigen-charged leukocytes and promote their trafficking via lymph, leading to amplification of the immune response (6). As inflammation resolves, anti-lymphangiogenic factors accumulate (e.g., T lymphocytes [ref. 7] and TGF-β [ref. 8]), and the newly expanded lymphatic vasculature regresses.
The mammalian heart has an extensive lymphatic capillary network that drains lymph to periaortic and paratracheal mediastinal lymph nodes (MLNs) via subepicardial pre-collector vessels (9). This vascular network ensures optimal heart function, as an increase in tissue fluid content by as little as 2.5% can lead to 30%-40% reduction in cardiac output (10,11). Cardiac lymphangiogenesis has been described during heart development and in response to injury (myocardial infarction [MI]), whereby induced lymphatic sprouting resulted in improved prognosis (12)(13)(14) via an uncharacterized mechanism. MI triggers a stereotypical reaction of the innate immune system, involving an initial influx to the injury site of a substantial number of neutrophils attracted by apoptotic signals released by dying cells (e.g., IL-1α; ref. 15), cell debris, and cytokines from neighboring cells (16). This acute response is critical to avoiding the undesirable consequences of accumulating damage signals in situ and to restoring tissue homeostasis. However, neutrophils generate high levels of ROS, secrete matrix-Myocardial infarction (MI) arising from obstruction of the coronary circulation engenders massive cardiomyocyte loss and replacement by non-contractile scar tissue, leading to pathological remodeling, dysfunction, and ultimately heart failure. This is presently a global health problem for which there is no effective cure. Following MI, the innate immune system directs the phagocytosis of dead cell debris in an effort to stimulate cell repopulation and tissue renewal. In the mammalian adult heart, however, the persistent influx of immune cells, coupled with the lack of an inherent regenerative capacity, results in cardiac fibrosis. Here, we reveal that stimulation of cardiac lymphangiogenesis with VEGF-C improves clearance of the acute inflammatory response after MI by trafficking immune cells to draining mediastinal lymph nodes (MLNs) in a process dependent on lymphatic vessel endothelial hyaluronan receptor 1 (LYVE-1). Deletion of Lyve1 in mice, preventing docking and transit of leukocytes through the lymphatic endothelium, results in exacerbation of chronic inflammation and long-term deterioration of cardiac function. Our findings support targeting of the lymphatic/immune cell axis as a therapeutic paradigm to promote immune modulation and heart repair. The cardiac lymphatic system stimulates resolution of inflammation following myocardial infarction jci.org Volume 128 Number 8 August 2018 clearance to MLNs are blocked, resulting in a loss of viable myocardium, enhanced scarring, and significantly reduced cardiac output. These findings are of widespread interest in terms of understanding how to optimize immune cell clearance from the site of cardiac injury and to offset the chronic progression to pathological remodeling, functional impairment, and ultimately heart failure.

VEGF-C-driven cardiac lymphangiogenesis increases clearance of immune cells after MI.
Initially we determined the source of VEGF-C that acts to drive the inherent lymphangiogenic response after injury. In the developing heart, the epicardium is a site of VEGF-C expression (20), and in dermal wounding studies CD11b + macrophages act as a source of VEGF-C and VEGF-D in response to inflammatory stimuli (5). In the adult heart, while we found no expression of VEGF-C in the quiescent podoplaninexpressing (PDPN-expressing) epicardium or CD68 + tissue macrophages residing in the intact myocardium (Supplemental Figure 1, A and B; supplemental material available online with this article; https://doi.org/10.1172/JCI97192DS1), expression of VEGF-C was increased in both cell types following MI (Supplemental Figure 1, C and D), leading to substantial lymphangiogenesis and remodeling of the subepicardial lymphatic network ( Figure 1A). Moreover, this response was considerably enhanced in mice treated with 100 ng/g body weight of recombinant selective VEGFR-3 agonist VEGF-C-Cys(156)Ser (21) [henceforth, VEGF-C(C156S)] on days 0, 2, 3, 4, and 6 after MI ( Figure 1B) (14) and resulted in increased LYVE-1 + vessel area percentage (vehicle, 26.43 ± 1.82; VEGF-C, 35.28 ± 1.17; P ≤ 0.001) and junction number (vehicle, 378.6 ± 60.49; VEGF-C, 660.6 ± 77.31; P ≤ degrading proteases, and undergo apoptosis following phagocytosis. Consequently, neutrophils within the injured milieu require timely suppression and spatial confinement to prevent exacerbation of tissue damage, most notably the death of viable cardiomyocytes and enhanced extracellular matrix degradation, that results in chamber dilatation, remodeling, and fibrotic scarring (16). Circulating monocytes and activated macrophages represent the second wave of innate immune cells. These proinflammatory (so-called M1) monocytes/macrophages participate in clearance of cell debris, including apoptotic neutrophils and cardiomyocytes, by essential efferocytosis (17) and also secrete ROS, proteases, and cytokines, leading to pathological remodeling of the infarcted tissue (16). Subsequently M1 macrophages adopt an antiinflammatory, pro-reparative M2 phenotype and contribute to ECM remodeling and fibrosis by signaling to myofibroblasts to patch the area of injury and prevent wall rupture after MI (16,18). Given the physiological role of the lymphatics in immune surveillance and their response to inflammation at sites of skin wounding (5,6,19), we sought to investigate the mechanism by which VEGF-C-induced lymphangiogenesis improves functional outcome after MI and, for the first time to our knowledge, translate findings from peripheral wound healing to organ-based repair. Specifically, we demonstrate that the expanded lymphatic network, draining the injury area, enables active trafficking of innate immune cells (neutrophils, macrophages, and dendritic cells) via lymph to regional MLNs, in a process dependent on the lymphatic endothelial receptor lymphatic vessel endothelial hyaluronan (HA) receptor 1 (LYVE-1). Critically, a global reduction in immune cell load within the infarcted milieu is sufficient to favor optimal heart repair, whereas in Lyve1 -/mutant mice immune cell trafficking and of circulating monocytes and activated macrophages undertake extensive phagocytic activity to clear neutrophils (23). Following this early acute inflammatory phase, CD68 + phagocytes persisted within the injured myocardium at 7 days after MI ( Figure 2, E and F) -a phenomenon known to contribute to chronic inflammation (23). By contrast, in VEGF-C(C156S)-treated hearts on day 7, in which we observed enhanced lymphangiogenesis ( Figure  1), we detected significantly decreased numbers of CD45 + leukocytes (vehicle, 7.80 ± 0.61; VEGF-C, 5.46 ± 0.67; P ≤ 0.05), specifically myeloid cells (CD45 + CD11b + : vehicle, 5.11 ± 0.45; VEGF-C, 3.12 ± 0.44; P ≤ 0.05) and myeloid subtypes such as CD45 + CD11b + Ly6G -F4/80 + macrophages (vehicle, 3.76 ± 0.40; VEGF-C, 2.24 ± 0.34; P ≤ 0.05) and CD45 + CD11b + Ly6G -F4/80 -CD11c + dendritic cells (vehicle, 0.078 ± 0.012; VEGF-C, 0.048 ± 0.005; P ≤ 0.05), as determined by multi-marker flow cytometry ( Figure  2, G-K, and Supplemental Figure 2, A-H). Importantly, TUNEL staining revealed scarce apoptotic CD68 + immune cells (ranging from 0 to 2 CD68 + TUNEL + cells per tissue section) in both vehi-0.05; Figure 1, C and D). Moreover, VEGF-C(C156S) treatment led to augmented expression of the leukocyte chemoattractant CCL21 by LYVE-1-expressing capillaries, indicative of an inflamed lymphatic endothelium ( Figure 1, E-J). Treatment with VEGF-C(C156S) has been reported to reduce myocardial edema and pathological remodeling, leading to improved cardiac function (14,22). However, the effect on tissue fluid constitutes an acute and relatively minor function of the responding lymphatic vasculature; consequently, we investigated whether lymphangiogenesis acts on the immune response and associated inflammation in the setting of cardiac injury. We first probed a potential colocalization of immune cells with the expanding lymphatic plexus after MI and observed that CD68 + macrophages were closely associated with LYVE-1 + cardiac lymphatic capillaries throughout the myocardium of intact ( Figure  2, A and B) and injured hearts (Figure 2, C-F). This colocalization was especially evident within the infarcted area at 4 days after MI (arrowheads in Figure 2D), the time point when a significant influx To address the possibility that the reduced immune cell content was independent of lymphangiogenesis, we performed flow cytometry (Supplemental Figure 2, A-H) on tissue derived from vehicle-and VEGF-C(C156S)-treated hearts collected on days 1 and 4 after MI, before any notable evidence of lymphatic sprouting (Supplemental Figure 3). No significant differences in immune cell numbers were observed between vehicle-and VEGF-C(C156S)treated hearts on day 1 (Supplemental Figure 3, A-E) or day 4 (Supplemental Figure 3, F-J) after MI, suggesting that there was no substantial early effect of VEGF-C(C156S) treatment on cardiac lymphatic vessel permeability to enable clearance of leukocytes from the injured heart. Instead, clearance was only evident by day 7 after MI following the establishment of an extensive lymphatic network draining the infarcted area (Figure 1), supporting the hypothesis that lymphangiogenesis augments the resolution of inflammation after injury.
To determine whether increasing lymphangiogenesis may rescue the phenotype observed in Lyve1 -/animals, we treated KO animals with VEGF-C(C156S) (Supplemental Figure 9). No signif-icant differences in immune cell numbers were observed between vehicle-and VEGF-C(C156S)-treated Lyve1 -/hearts (Supplemental Figure 9, A-E) or MLNs (Supplemental Figure 9, F-J) on day 7 after MI, suggesting that VEGF-C treatment does not alter trafficking in the mutants as it does in control hearts ( Figure 2). These findings reinforce the idea that Lyve1 -/cardiac lymphatics have impaired immune cell uptake, which prevents trafficking, irrespective of lymphangiogenesis. Together, these data support clearance of immune cells via lymph into draining MLNs, a process enhanced by VEGF-C-induced cardiac lymphangiogenesis and dependent on LYVE-1.

Disruption of LYVE-1-dependent clearance of immune cells by lymphatics is detrimental to cardiac function after MI.
To investigate whether immune cell accumulation (failed clearance) in Lyve1deficient mice is detrimental to cardiac function, we performed a longitudinal cine MRI study with mice scanned on days 7 and 21 after MI (Figure 7, A-G, Supplemental Table 1, and Supplemental Videos 1 and 2). These time points were selected based on our observations of active lymphangiogenesis and immune cell trafficking to regional MLNs by day 7 (Figures 1-6) and functional improvement, as previously determined in VEGF-C(C156S)treated hearts, by day 21 (14). MRI revealed that both percentage LV ejection fraction (EF) and stroke volume (SV), calculated as the difference between end-diastolic volume (EDV) and end-systolic volume (ESV) (31), were significantly reduced in Lyve1 -/mice compared with controls (Figure 7, A   function. We reveal that stimulation of lymphangiogenesis by VEGF-C treatment after heart injury leads to early resolution of inflammation through enhanced immune cell clearance, in a process dependent on the lymphatic receptor LYVE-1 (Figures 1-3). While we report direct effects on innate immune cell clearance, the improved outcome may also be mediated, at least in part, via the adaptive immune response and the recruitment of lymphocyte subpopulations that act as negative regulators of inflammation (32). Tregs infiltrate the infarcted tissue as a third wave of (adaptive) immune cells, and promote differentiation of macrophages to an antiinflammatory phenotype and modulate protease synthesis by cardiac fibroblasts to aid wound healing and repair (33,34). It is feasible that the increased clearance of dendritic cells we observed following VEGF-C treatment ( Figure 2K) enhances the programing of remote naive T cells (35) residing in draining lymph nodes to Tregs, which when mobilized into the injured heart alter macrophage polarization to favor a more antiinflammatory/ pro-reparative M2 state (reviewed in ref. 27). However, our expression analyses revealed no evidence of alterations in macrophage polarization, M1/M2 marker ratios, cytokine profiles, or selection of specific macrophage subtypes in the infarcted milieu at 7 days after MI (Supplemental Figure 4), arguing against an indirect pro-reparative effect via the adaptive immune system. control, 30.93% ± 1.15%, Lyve1 -/-, 25.52% ± 1.84%; P ≤ 0.05 [day 7 vs. 21 control] and P ≤ 0.05 [day 21 control vs. day 21 Lyve1 -/-]). Moreover, the ESV in Lyve1-mutant hearts was significantly increased (Figure 7, C-G, and Supplemental Table 1; day 7 control, 36.47% ± 8.26%, Lyve1 -/-, 34.34% ± 6.17%; day 21 control, 43.33% ± 9.00%, Lyve-1 -/-, 47.18% ± 7.92%; P ≤ 0.05; day 7 vs. 21 Lyve1 -/-), and there was evidence of LV wall thinning (Supplemental Videos 1 and 2), which is known to contribute to a decline in cardiac function after MI. Histological analyses by Masson's trichrome and Picrosirius red staining revealed extensive collagen deposition and scarring in Lyve1 -/hearts on day 21 after MI compared with controls (Picrosirius signal/area ratio quantification: control, 2.28 × 10 -10 ± 1.79 × 10 -11 ; Lyve1 -/-, 5.22 × 10 -10 ± 6.99 × 10 -11 ; P ≤ 0.05; Figure 7, H-N). Thus, in the absence of any gross lymphatic vessel defects at baseline or abnormal lymphangiogenic response after MI, these data collectively suggest that impaired immune cell uptake and clearance in Lyve1 mutants resulted in a progressive deterioration in heart function, accompanied by elevated pathological remodeling and fibrosis.

Discussion
Taken together, our results demonstrate an essential immunomodulatory role for lymphangiogenesis in regulating heart extraction, post-MI hearts were dissected into infarct and remote regions before snap freezing. Assessment of area at risk. Following LAD ligation of C57BL/6 WT and Lyve1 -/mice, Evans Blue dye (1 ml of 2% Evans Blue in distilled water) was perfused through the jugular vein to demarcate the area of non-perfused myocardium due to occlusion of the coronary artery (blue, perfused; pink/red, non-perfused). Hearts were rapidly extracted and frozen at -20°C for 2 hours to facilitate manual slicing of 6 transverse slices of approximately 1-mm thickness from apex to the base of the ventricles. Heart slices were briefly incubated in 2% formaldehyde solution at room temperature, washed in PBS, blotted dry, weighed, and imaged using a Zeiss Axio Imager Z1 microscope with an AxioCam MRm camera attachment running AxioVision software release 4.8 (Zeiss). Quantifications were performed on transverse slices of the LV using Fiji software (NIH Image), and area at risk (AAR) was expressed as a fraction of LV area (AAR/LV %).
Immunodetection methods. Whole-mount hearts or cryosections (hearts and MLNs) were processed for indirect immunofluorescence using standard methods. Primary antibodies are listed in Supplemental Table 2. Alexa Fluor secondary antibodies (Invitrogen, 1:200) were used in all cases. Imaging was performed using a Zeiss Z1 Light sheet microscope (whole-mount tissue) or an Olympus FV1000 confocal microscope (tissue sections/whole-mount tissues). Images were digitally captured and processed using Fiji software. Analysis of lymphatic vessel area and junction number calculations were performed using AngioTool software (37).
Single-cell isolation of cardiac cells. Post-MI hearts harvested for flow cytometry studies were isolated, placed in cold HBSS (Life Technologies), finely minced into small pieces, and digested with collagenase type II (Worthington Biochemical Corp.) solution (containing 500 U/ml HBSS) at 37°C for 30 minutes with agitation. Supernatant was removed and 10% heat-inactivated FBS (Sigma-Aldrich) added. The remaining tissue was digested with a fresh collagenase solution for a total of 3 times. Cell suspensions were combined and filtered through a 40-μm cell strainer (BD Falcon). Cells were centrifuged and washed with PBS, and Red Cell Lysis buffer (BioLegend) was used according to the manufacturer's instructions to remove red blood cells. Isolated single cardiac cells were stained and subjected to flow cytometric analyses.
Adoptive cell transfer. Monocytes were isolated from the spleen of hCD68-EGFP + adult mice. Following Schedule 1 killing, the spleen was removed by dissection and the tissue disrupted with the blunt end of a sterile syringe. The disrupted spleen tissue was washed through a 70-μm cell strainer into red cell lysis buffer and incubated at room temperature for 10 minutes. Cells were then spun down, and red cell lysis buffer was removed by aspiration. Monocytes were then puri-Our study suggests that macrophage load correlates directly with effective cardiac repair and improved functional outcome. This is consistent with the fact that splenectomized or monocytedepleted mice and human patients on steroids adversely lowering monocyte numbers (36,37) -as well as patients with elevated monocytosis (increased monocyte load) and apoE-null mice with increased monocytes (38,39) -have impaired peripheral wound healing. Thus, achieving the optimal monocyte/macrophage loading after injury in general terms represents a therapeutic opportunity (reviewed in ref. 40) that in the heart may be achieved by targeting the cardiac lymphatic system to spatiotemporally constrain the innate immune response. By efficiently clearing immune cells away from the injury site to MLNs, the lymphatic network dampens the acute immune response, preventing its long-term escalation to a more chronic inflammatory setting, which in turn favors more optimal tissue repair and a beneficial outcome after MI. Therefore, therapeutic strategies to invoke lymphangiogenesis may prevent the inflammation-dependent progression to heart failure in acute MI patients with ischemic heart disease.

Methods
Animal models. Mice were housed and maintained in a controlled environment by University of Oxford Biomedical Services. Lyve1 -/-, hCD68-EGFP, and R26R tdTomato mice were kept on a C57BL/6J inbred background and have been described previously (25,36,41). Myh6-Cre/Esr1 mice were purchased from the Jackson Laboratory and kept on a C57BL/6J inbred background. For experiments where WT mice were required, C57BL/6J animals were used (Charles River Laboratories). For tamoxifen-dependent tissue-specific gene activation using the Myh6-Cre/Esr1 driver, 2 mg tamoxifen (Sigma-Aldrich) was administered daily (for 5 days) to 8-to 10-week-old Myh6-Cre/Esr1;tdTomato mice by i.p. injection. There was a 2-week waiting period between the last i.p. injection of tamoxifen and the surgical procedure to induce MI.
MI. All surgical and pharmacological procedures were performed in accordance with the Animals (Scientific Procedures) Act 1986 (Home Office, United Kingdom). C57BL/6 WT, Lyve1 -/-, and tamoxifentreated Myh6-Cre/Esr1;R26R tdTomato adult mice (10-14 weeks old; 25-30 g body weight) were used in MI experiments. MI was induced in isoflurane-anesthetized mice by permanent ligation of the left anterior descending coronary artery (LAD). For sham controls, a suture was passed under the LAD but not ligated. Upon recovery (day 0), C57BL/6 WT animals were administered 100 ng/g body weight of recombinant VEGF-C-Cys(156)Ser (R&D Systems) or vehicle (PBS) i.p. on days 0, 2, 3, 4, and 6 after MI. Hearts were harvested at 7 days following LAD ligation (day 7 after MI). For the day 1 after MI experimental group, a single i.p. injection of vehicle (PBS) or recombinant VEGF-C(C156S) was given at recovery from surgery (day 0), and hearts were collected at 1 day following ligation. For the day 4 after MI experimental group, animals received i.p. injections of vehicle (PBS) or recombinant VEGF-C(C156S) on days 0, 2, and 3 after MI, and hearts were harvested at 4 days following ligation. Hearts and MLNs collected for immunostaining were washed in ice-cold PBS prior to overnight fixation in a 4% formaldehyde solution at 4°C. Hearts for flow cytometry were washed in ice-cold HBSS (Life Technologies) prior to tissue digestion. Hearts for subsequent RNA extraction were removed and immediately placed in a CryoTube (Nunc, Thermo Fisher Scientific), which was submerged in liquid nitrogen. For RNA jci.org Volume 128 Number 8 August 2018 outcome. For MI studies, hearts showing no morphological signs of infarct (e.g., tissue blanching around the ligating suture) at the stage of sample collection were excluded from further analysis. No randomization criteria were used. Statistics were calculated using GraphPad Prism 7 software. The statistical significance between 2 groups was determined using an unpaired 2-tailed Student's t test; these included an F test to confirm the 2 groups had equal variances, and the data were reported as mean ± SEM. Among 3 or more groups (e.g., data shown in Figure 6I), 1-way ANOVA followed by Tukey's multiple comparisons test was used for comparisons. Statistical significance of data generated by the longitudinal cardiac cine MRI approach was determined using 2-way ANOVA with repeated measures. P ≤ 0.05 was considered statistically significant. Study approval. All animal experiments were carried out according to United Kingdom Home Office project License PPL30/2987 compliant with the United Kingdom Animals (Scientific Procedures) Act 1986 and approved by the University of Oxford Central Committee on Animal Care and Ethical Review (ACER).

Author contributions
JMV, SN, and CVdC carried out all experiments (except MI surgeries and flow cytometry), analyzed the data, and contributed figures for the manuscript. TJC, DNB, and JMV performed the flow cytometry studies and analyzed the data generated. MGR performed all MI surgeries. DNB performed histology. CAC performed blinded MRI scanning, and CAC, MGR, and JMV analyzed the MRI data blinded to the genotype of experimental specimen. LAJ and DGJ provided the Lyve1 -/mice, advice and technical assistance with MLN dissection, and helped edit the manuscript. DRG provided the hCD68-EGFP transgenic mice. JMV and PRR established the hypotheses, supervised the studies, and cowrote the manuscript. fied from the cell pellet using an EasySep Mouse Monocyte Enrichment Kit (STEMCELL Technologies) according to the manufacturer's instructions. Prior to surgery, i.e., permanent ligation of the LAD, cells were counted and resuspended in sterile PBS. Each recipient animal received 100,000 cells by intramyocardial injection (using a 30G insulin syringe) at the time of MI surgery.
TUNEL staining. Apoptotic cells were detected by TUNEL staining in cryosections of infarcted hearts collected on day 7 after MI using the In-Situ Cell Death Detection Kit (Roche) and fluorescence detection, based on the manufacturer's protocol.
RNA isolation and gene expression profile by qRT-PCR. Total RNA was isolated from post-MI heart samples using Trizol reagent (Invitrogen), according to the manufacturer's instructions. Total RNA was reverse transcribed using oligo-dT primers and Superscript III RT (Invitrogen). qRT-PCR analysis was performed on a ViiA 7 Real-Time PCR System (Thermo Fisher Scientific) using Fast SYBR Green Master Mix (Thermo Fisher Scientific). Data were normalized to 18s, Hprt, and Gapdh housekeeping gene expression. Fold change in gene expression was determined by the 2 −ΔΔCT method (42). Primer sequences are listed in Supplemental Table 3. Statistical differences were detected using an unpaired, 2-tailed Student's t test.
Cardiac cine MRI. Cardiac cine MRI was performed after LAD ligation as described previously (43), with the operator blinded to the experimental group genotype. Briefly, mice were anesthetized with 2% isoflurane in O 2 and positioned supine in a purpose-built cradle. ECG electrodes were inserted into the forepaws, and a respiration loop was taped across the chest. The cradle was lowered into a vertical-bore, 11.7 T MR System (Magnex Scientific) with a 40-mm birdcage coil (RAPID Biomedical) and a Bruker console running Paravision 2.1.1 (Bruker Medical). A stack of contiguous 1-mm-thick true short-axis ECG-gated cine FLASH images were acquired to cover the entire LV (TE/TR, 1.43/4.6 ms; 17.5° pulse; field of view, 25.6 × 25.6 mm; matrix size, 128 × 128 zero filled to 256 × 256, giving a voxel size of 100 × 100 × 1000 μm; 20-30 frames per cardiac cycle). Long-axis 2-chamber and 4-chamber images were also acquired. Blinded-image analysis was performed using ImageJ (NIH). LV volumes, SV, and EF were calculated as described previously (31).
Histology. Upon completion of MRI scanning on day 21 after MI, hearts were harvested and processed for paraffin embedding, cut into Superfrost slides, and deparaffinized using standard methods. For Masson's trichrome staining (Abcam), sections were stained according to the manufacturer's instructions. For Picrosirius red staining, sections were stained using the Picro Sirius Red Stain Kit (Abcam) for 60 minutes according to the manufacturer's protocol and imaged on a Nikon TE2000 microscope under transmission and polarized light. Quantification of fibrotic scarring based on (Picrosirius) yelloworange birefringence signal was performed using Fiji software.
Statistics. Animal numbers and sample sizes reflected the minimal number needed for statistical significance based on prior experience and power analysis calculations to reflect at least a 15% difference in