Dear Editor,
Vascular endothelial growth factor-A (VEGFA, also known as VEGF) is a critical angiogenic factor that regulates the physiological and pathological blood vessel growth.1 Increased abundance of VEGF in the eye underlies many forms of aberrant ocular angiogenesis and resultant vision loss, including in neovascular age-related macular degeneration (nvAMD), proliferative diabetic retinopathy (PDR), ischemic retinal vein occlusion, and retinopathy of prematurity (ROP). Multiple VEGF inhibitors are approved for such ocular angiogenic diseases. Despite the initial, and often dramatic, efficacy of anti-VEGF therapy, real-world and long-term studies are more sobering.2,3 Thus, enhanced understanding about the regulation of ocular VEGF can further elucidate the underlying pathological mechanisms and aid in developing new therapeutic strategies.
N6-methyladenosine (m6A), the most abundant post-transcriptional modification of eukaryotic mRNA, plays fundamental roles in regulating biological processes and diseases.4 The m6A modification is dynamic, being “written” by methyltransferase complex components, and “erased” by demethylases, including Fat mass and Obesity-associated protein (FTO) and AlkB Homolog 5, RNA Demethylase (ALKBH5). The best studied effect of the m6A modification is promotion of mRNA instability, thereby affecting target mRNA transcript abundance. Accordingly, m6A RNA modifications are essential for macrophage activation,5 which was found to be crucial for the development of experimental nvAMD in our prior studies.6 However, whether m6A modification of macrophage genes plays a role in nvAMD is unknown.
We studied the role of the m6A methyltranscriptome in laser photocoagulation-induced choroidal neovascularization. We observed an increased abundance of Vegfa mRNA in angiogenic choroid, accompanied by enhanced levels of Fto mRNA (Fig. 1a) and modestly decreased levels of Rbm15 and Wtap mRNAs (Supplementary Fig. S1a). However, there were no significant changes in Metttl3, Mettl14, and Alkbh5 mRNA abundance (Fig. 1a and Supplementary Fig. S1a). At 3 days after laser injury, coinciding with macrophage infiltration and the onset of neovascularization,7 we observed a dramatic increase in FTO-expressing cells within the area of neovascularization, some but not all of which were F4/80+ (Fig. 1b, c, d, e and Supplementary Fig. S1b, c). Inhibiting FTO activity in vivo using a selective inhibitor resulted in a significant reduction in neovascularization but, interestingly, not in F4/80+ macrophage recruitment (Fig. 1f, g, h). In addition, inhibition of FTO suppressed VEGFA protein levels in laser treated RPE-choroid tissue (Fig. 1i) and suppressed the VEGFA release in human ARPE-19 cells (Supplementary Fig. S1d). In primary mouse bone marrow derived macrophages, knockdown of FTO expression by specific small interfering RNA (siRNA) significantly dampened macrophage-mediated VEGFA release (Supplementary Fig. S1e, f, g).
FTO in macrophage VEGFA release and choroidal neovascularization. a Quantification of Vegfa, m6A methyltransferase (Mettl3, Mettl4), demethylase (Fto) mRNA levels in pooled eye tissues (n = 3) of control, naive (no laser treated) mice (Ctrl) or mice following laser injury (choroidal neovascularization, CNV, day 3 after laser injury). b, c Immunofluorescent staining of FTO in flat-mounted RPE-choroid tissues (b) and cryosections of eyes (c) at 3 days after laser injury. F4/80 immunostaining indicates macrophage infiltration following laser injury. d, e Immunoblotting and quantification of FTO and F4/80 protein levels in RPE-choroid tissues isolated from mice eyes at 3 days after laser injury (n = 2 eyes). f Immunofluorescent staining of neovascularization using isolectin B4 (green) and of macrophages by F4/80 (red) in RPE-choroid tissues of mice treated with FTO inhibitor (FTOi) or vehicle, at 7 days after laser injury. g, h Quantification of CNV and F4/80 volumes based on isolectin B4 and F4/80 staining in RPE-choroid tissues of mice treated with FTO inhibitor (FTOi) or vehicle, at 7 days after laser injury (n = 24 laser spots for Ctrl, and n = 25 spots for FTOi). i Quantification of VEGFA levels in the RPE/choroid tissues of mice treated with FTO inhibitor (FTOi) or vehicle, at 3 days after laser injury (n = 5 eyes). j Quantification of methylated Vegfa mRNA levels in mouse BMDMs treated with FTO inhibitor (FTOi) or vehicle for 24 h by using MeRIP-qPCR (n = 2). k Determination of Vegfa mRNA stability in BMDMs pretreated with FTO inhibitor (FTOi) or vehicle, followed with Actinomycin D inhibition (10 µg/ml). mRNA abundance was measured by RT-qPCR at the indicated time points and Vegfa mRNA half-lives (t1/2) determined by fitting the data to a nonlinear one phase decay model (mean ± SEM, n = 3). l Schematic diagram showing FTO regulates VEGFA release and choroidal neovascularization in AMD. Retinal pigment epithelium RPE, BM Bruch’s membrane, Mφ macrophages. Data are shown as mean ± SEM, *p < 0.05; ** p < 0.01; ***p < 0.001; ****p < 0.0001; ns not significant. Two-way ANOVA with Sidak’s multiple comparisons (a, c); One-way analysis of variance (ANOVA) with Dunnett’s multiple comparisons (g); unpaired two-tailed t-test (e, j, g, k)
Next, we used Methylated RNA ImmunoPrecipitation PCR (MeRIP-PCR) to determine whether FTO demethylated macrophage Vegfa mRNA. Consistent with previous studies,8 we found Vegfa mRNA is abundantly methylated in basal conditions (Fig. 1j). Inhibition of FTO significantly increased the abundance of m6A methylated Vegfa mRNA; this was accompanied by a reduction in mouse VEGFA release (Fig. 1i and Supplementary Fig. S2a to c). In contrast, targeting m6A methylase with a METTL3 inhibitor resulted in a dose-dependent increase in VEGFA release (Supplementary Fig. S2d). FTO regulates gene expression via maintaining mRNA stability.9 After blocking new mRNA synthesis, we found that macrophage Vegfa mRNA half-life was significantly shorter in the presence of an FTO inhibitor (Fig. 1k and Supplementary Fig. S2e). However, FTO inhibition did not significantly alter the mRNA abundance of other pro-angiogenic factors, such as placental growth factor (Plgf) and platelet-derived growth factors (Pdgfa), suggesting the preferential effect of FTO-mediated m6A demethylation on maintaining macrophage Vegfa mRNA stability and VEGFA release (Supplementary Fig. S2f).
Although we found Vegfa mRNA was the principal pro-angiogenic RNA substrate regulated by FTO in murine macrophages, other genes could also be impacted by FTO inhibition during neovascularization. For example, FTO regulates focal adhesion kinase (FAK) expression in corneal neovascularization.10 Our study suggests FTO inhibition has minimal adverse effects on cell viability, and we did not observe in vivo retinal toxicity with FTO inhibition in our studies. However, more detailed toxicity studies remain to be performed. Additionally, macrophage- targeted delivery systems could be a promising approach for targeting FTO in ocular angiogenic disorders.
Collectively, our study identifies a previously undescribed role of FTO regulation of VEGFA expression and choroidal neovascularization in vivo (Fig. 1l). This work reveals a new mechanism of Vegfa mRNA modification that is regulated by the m6A methyltranscriptome. The discovery that inhibition of FTO suppresses VEGFA release and choroidal neovascularization opens the possibility of therapeutic targeting of FTO for angiogenic eye diseases.
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All materials are available in the main text or supplementary materials. Further information and requests for resources and reagents are available from the corresponding authors on reasonable request.
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Acknowledgements
J.A. has received support from the UVA Strategic Investment Fund, National Institutes of Health (NIH) grants (R01EY028027, R01EY029799, R01EY031039, R01AG082108), DuPont Guerry, III, Professorship, and a gift from Mr. and Mrs. Eli W. Tullis; S.B.W has received support from Annette Lightner Fund (Annette Lightner Research Award); B.D.G. has received support from NIH grants (R01EY028027, R01EY031039, R01EY032512, R01AG082108), BrightFocus Foundation Award M2020114, and the Owens Family Foundation.
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S.B.W. and J.A. designed research; S.B.W., Y.N., D.A., A.N., and P.Y. performed research; S.B.W., Y.N., B.D.G., and J.A. analyzed data; S.B.W., B.D.G., and J.A. wrote the manuscript. All authors have read and approved the submission of manuscript.
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J.A. is a cofounder of iVeena Holdings, iVeena Delivery Systems, and Inflammasome Therapeutics and has been a consultant for Allergan, Boehringer-Ingelheim, Olix Pharmaceuticals, Retinal Solutions, and Saksin LifeSciences unrelated to this work. J.A. and B.D.G. are cofounders of DiceRx. J.A., B.D.G., and S.B.W. are named as inventors on patent applications filed by their university. P.Y.: none; A.N.: none, D.A.: none; Y.N.: none.
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The mouse study protocol was approved by the University of Virginia’s Institutional Animal Care and Use Committee (IACUC, approval number: 4138).
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Wang, Sb., Nagasaka, Y., Argyle, D. et al. Targeting the m6A mRNA demethylase FTO suppresses vascular endothelial growth factor release and choroidal neovascularization. Sig Transduct Target Ther 8, 72 (2023). https://doi.org/10.1038/s41392-022-01277-4
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DOI: https://doi.org/10.1038/s41392-022-01277-4
