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Paeonol Promotes Reendothelialization After Vascular Injury Through Activation of c-Myc/VEGFR2 Signaling Pathway
Authors Wang Y, Wang Z, Wu X, Zhu S, Guo Q, Jin Z, Chen Z, Zhang D, Hu W, Xu H, Shi L, Yang L, Wang Y
Received 19 January 2023
Accepted for publication 2 May 2023
Published 24 May 2023 Volume 2023:17 Pages 1567—1582
DOI https://doi.org/10.2147/DDDT.S403134
Checked for plagiarism Yes
Review by Single anonymous peer review
Peer reviewer comments 2
Editor who approved publication: Prof. Dr. Georgios Panos
Yang Wang,1,* Zheng Wang,1,* Xiao Wu,1,* Song Zhu,2,* Qiru Guo,1 Zhong Jin,1 Zixian Chen,3 Delai Zhang,2 Wangming Hu,1 Huan Xu,1 Liangqin Shi,1 Lan Yang,1 Yong Wang1
1College of Basic Medicine, Chengdu University of Traditional Chinese Medicine, Chengdu, People’s Republic of China; 2Hospital of Chengdu University of Traditional Chinese Medicine, Chengdu, People’s Republic of China; 3School of Ethnic Medicine, Chengdu University of Traditional Chinese Medicine, Chengdu, People’s Republic of China
*These authors contributed equally to this work
Correspondence: Yong Wang, College of Basic Medicine, Chengdu University of Traditional Chinese Medicine, Chengdu, Sichuan, People’s Republic of China, Tel +86 18280350393, Email [email protected]; [email protected]
Purpose: Dysfunction of endothelium is associated with multiple pathological vascular diseases. However, how to regulate reendothelialization after vascular injury is not well defined. This study aims to determine whether and how Paeonol controls reendothelialization following artery injury.
Methods: The endothelium of murine carotid artery was denuded by catheter guide wires injury. H&E staining and IF staining were performed to determine whether Paeonol is critical for reendothelialization. BRDU Incorporation Assay, Boyden Chamber Migration Assay, Tube Formation Assay, and Spheroid Sprouting Assay were used to investigate whether Paeonol is involved in regulating proliferation and migration of endothelial cells. The underlying mechanism of how Paeonol regulates reendothelialization was determined by Molecular docking simulation and CO-IP Assay.
Results: Paeonol treatment significantly inhibits neointima formation in carotid artery ligation model by promoting proliferation and migration of endothelial cells. Mechanistically, Paeonol enhances c-Myc expression, consequently interacts with VEGFR2 results in activating VEGF signaling pathway, and eventually promotes reendothelialization after vascular injury.
Conclusion: Our data demonstrated that Paeonol plays a critical role in regulating vascular reendothelialization, which may be therapeutically used for treatment of pathological vascular diseases.
Keywords: Paeonol, c-Myc, VEGFR2, vascular injury, reendothelialization
Graphical Abstract:
Introduction
Maintenance of endothelium integrity and function plays a pivotal role during ontogeny of organisms. Endothelium lining inside of heart and vessels not only forms an interface between circulating blood, vascular, and lymph wall, but also forms a barrier between vascular and tissues. The integrity of endothelium plays a pivotal role in regulating communication between circulating blood and tissues.1 Endothelial cells can synthesize and secrete multiple substances, which are crucial in regulating vascular contraction and relaxation, and synthesize and secrete a variety of enzymes, which are critical in controlling blood clotting and platelet adhesion.2
Endothelial dysfunction can be induced by vascular injury, such as stent implantation. Preexisting vascular diseases, especially atherosclerosis,3 hypertension,4 diabetes,5 and some other conditions, including cigarette smoking,6 alcohol,7 high fat diet,8 and aging,9 which can accelerate endothelial dysfunction. Dysfunction of endothelium is characterized by not only alternation of morphology and motility but also changes in endothelial behaviors, including an imbalance in the relative contribution of endothelium-derived relaxing and contracting factors,10 disrupted vascular tone,11 increased vascular permeability-induced inflammatory reactions,3 which contributes to regulate development of thrombus formation,12 atherosclerosis,3 vascular restenosis,13 arterial aneurysm,14 and arterial stiffness.15
The endothelium can be repaired by resident endothelial cells, circulating endothelial progenitor cells and marrow release of endogenous progenitor cells, which mediates homing and arrangement in arterial denuded sites or intravascular stent surfaces.16,17 Endothelial cell-specific growth factor, including VEGF, promotes reendothelialization.18 Studies have demonstrated that Neurotrophin-3 promotes reendothelialization by promoting endothelial progenitor cell mobilization and homing.19 Pattern recognition receptors (PRRs) promote reendothelialization through increased inflammasome activation.20 Mitochondrial oxidation caused by SIRT3/SOD2 signaling deficiency contributes to decline of reendothelialization.21 Insulin and Bone marrow-derived Krüppel-like factor 10 accelerates reendothelialization following arterial endothelial injury.22,23 Erythropoietin-mobilized endothelial progenitors induce reendothelialization via Akt-mediated nitric oxide synthase activation.24 Eva-1 homologue 1 (Eva1a) ameliorates atherosclerosis by promoting reendothelialization via Rac1 signaling pathway.25
Numerous studies have demonstrated that Traditional Chinese Medicine could be used for cardiovascular disease treatment. Paeonol is a natural ingredient isolated from Paeonia Suffruticosa and Paeonol lactiflora pall.26 Our previous studies have demonstrated that Paeonol suppresses SMC phenotypic switching associated with neointima formation by inhibiting SMC proliferation and mobility. However, whether inhibition of neointima formation is due to regulating reendothelialization is unknown. Our previous study also indicates that Paeonol treatment dramatically induces endothelial cell c-Myc expression. c-Myc is an early molecular marker of cell cycle activity.27 Research has found that c-Myc could directly promote SMC growth and motility28,29 and suppress vascular inflammation,30 which is critical for the development of occlusive vascular disease.27 However, whether c-Myc regulates reendothelialization is not well defined. This study aimed to investigate the potential role of Paeonol in regulating reendothelialization.
Materials and Methods
Ethics Approval and Consent to Participate
Animal care and treatment refer to the National Institutes of Health “Guide for the Care and Experimentation of Laboratory Animals”. The experimental protocols and operating procedures were reviewed and approved by the Animal Welfare and Use Committee of Chengdu University of Traditional Chinese Medicine (ethical approval number: 2019–04).
Chemicals
Paeonol is an effective ingredient of Paeonia suffruticosa Andr. Paeonol (C9H10O3) was purchased from Sigma. Ki8751 (C24H18F3N3O4) was purchased from Selleck.
Animal Model
Murine carotid artery catheter guide wires injury performed as in a previous publication.31 Briefly, 2-month-old male ApoE−/− mice were pretreated with Paeonol (30 mg/kg) by intraperitoneal injection for 7 days. Mice were anesthetized and placed on a temperature-controlled heating pad. Separated internal carotid artery and external artery under microscope. Endothelium of common carotid artery was denuded by catheter guide wires (0.014 inch). Mice were continuously treated with Paeonol until sacrificed. The carotid arteries were harvested and paraffin-embedded for further analysis. The mice were anesthetized by intraperitoneal injection of ketamine 80 mg/kg and xylazine 5 mg/kg.
Hematoxylin and Eosin (H&E), Immunohistochemistry (IHC), and Immunofluorescence (IF) Staining
Harvested murine common carotid arteries, paraffin embedded, and collected slides of 5 μm thickness. H&E staining was performed as in our previous study.32 For IHC staining, the slides were dealt with unmasking solution for antigen retrieval, followed by incubation with primary antibody. After being incubated with a biotinylated secondary antibody, ABC and DAB solutions (Vector Laboratories) were used to visualize targets. For IF staining, the slides were immersed in citric acid solution for antigen retrieval. Blocked and incubated with primary antibody. A fluorophore-conjugated secondary antibody was used. Images were captured using confocal microscopy (LS510, Zeiss).
Cell Culture
Human primary umbilical vein endothelial cell (HUVEC) and human umbilical vein/vascular endothelial cell line (HUVEC-C) were purchased from ATCC (USA). HUVEC cells were cultured in vascular cell basal medium (ATCC, USA) and supplemented with endothelial Cell Growth Kit (ATCC, USA), and the HUVEC-C cells cultured in basal medium (ATCC, USA) containing 10% FBS (Gibco, USA).
CCK-8 Assay
HUVECs were trypsinized and seeded in a 96-well culture plate (3×103/well), following Paeonol (10 μM) treatment for 24 h. After incubated of CCK-8 solution, the absorbance at 450 nm was measured.
BRDU Incorporation Assay
Suspended HUVEC in the medium containing Paeonol (10 μM), then labeled with BRDU labeling reagent for 12 h. IF staining was performed to visualize BRDU-incorporated cells.
Cell Cycle Analysis
Treated HUVEC with Paeonol (10 μM), trypsinized, and fixed with 70% ethanol. Cell cycle was analysed by flow cytometry analysis after propidium iodide staining (BD Biosciences).
Boyden Chamber Migration Assay
Cells seeded in serum-free medium that was settled into a culture plate containing 10% FBS and Paeonol (10 μM). Migrated cells were counted after crystal staining.
Spheroid Sprouting Assay
More details of spheroid sprouting assay described in our previous publication.33 Mixed cell suspension and methylcellulose solution in a ratio of 1:4. The mixture was added in a 96-well culture plate to form “cell sphere”. Neutralized liquid collagen solution and solidified at 37°C. Calcein staining was used to visualize cells. Images of “cell spheres” were captured under microscope (Leica Microsystem CMS GmbH). Image J was used to quantify the length of spheroid sprouting.
Matrigel-Based Tube Formation Assay
Solidified neutralized collagen solution and suspended HUVEC-Cs with medium contained Paeonol (10 μM). The endothelial tubule formation was monitored under microscope and images were captured after Calcein staining. Cumulative tube numbers were quantified using Image J.
Quantitative Real Time PCR Analysis
Total RNA was extracted from HUVEC or HUVEC-C using the Trizol reagent (Thermo Invitrogen). Reverse transcription was performed using iScript cDNA synthesis kit (Vazyme). Quantification was calculated using the 2−ΔΔCT method against β-actin. The primer sequences are exhibited in primer list (Supplementary Figure 1).
Western Blot Analysis
Proteins from HUVEC or HUVEC-C were extracted using RIPA lysis buffer. Protein concentration was evaluated using BCA kit (Biosharp). Protein is denatured at 98°C for 10 min and separated by SDS-PAGE. It is incubated with specific antibodies. Visualization was performed using a chemiluminescence Western blotting detection kit, and images were captured by a chemiluminescence detection system.
Protein and Protein Interaction (PPI) Network Analysis
The String (Version: 11.5) database (http://string-db.org/) was used to obtain the protein–protein interactions (PPI). The organism was selected as Homo sapiens, interaction score ≥0.4 was set, and disconnected nodes were hidden in the network.
Molecular Docking
The molecular docking performed by Autodock Vina 1.5.6 was used to evaluate the binding energy. The mol2 format for the structure of Paeonol was downloaded through TCMSP (https://old.tcmsp-e.com/). The three-dimensional structures of c-Myc (Homo, ID: 5G1X) and VEGFR2 (Homo, ID: 1VR2) were downloaded from PDB database (http://www.rcsb.org/). Before molecular docking, we removed the organic and H2O molecules of the macromolecular protein and added hydrogens before molecular docking. Then, the Grid Box was prepared. Finally, the value of binding energy was measured.
Co-Immunoprecipitation Assay
Cell lysate is extracted from HUVEC cells. Cleared Protein A/G agarose beads (TransGen Biotech, Beijing, China). Mixed beads and cell lysate and incubated with c-Myc (Abcam) and VEGFR2 (Cell Signaling Technology). The CO-immunoprecipitation protein targets were evaluated using Western blotting.
Protein Docking Prediction
The protein docking prediction is based on a previous publication.34 Briefly, the crystal structures of c-Myc (ID: 5G1X) and VEGFR2 (ID: 1VR2) were obtained from the RSCB PDB and the IDs of both were input into ZDOCK SERVER (http://zdock.umassmed.edu/), in which we obtained the complexes. Then, the complexes ranked top five were analyzed by PDBePISA (https://www.ebi.ac.uk/msd-srv/prot_int/). Finally, the complex ranked top was visualized by Pymol Version 2.5.2.
Statistical Analysis
Quantitative data was presented as mean ± SEM. GraphPad prism software was used for statistical analysis. The difference in significance between two groups was analyzed using unpaired Student’s t-test. One-way ANOVA followed by Tukey’s-b test and repeated measures ANOVA followed by S-N-K (Student-Newman-Keuls) test were used to compare the differences in cell viabilities after different doses of paeonol treatment and at different time points, respectively. Normal Q–Q plots are used to assess data distribution. * P < 0.05 was considered statistically significant.
Results
Paeonol Alleviates Vascular Stenosis Induced by Endothelial Injury
Various vascular diseases lead to vascular stenosis after endothelial injury. To assess whether Paeonol involves in regulating vascular stenosis responding to vascular injury, catheter guide wires injury was performed. The male ApoE−/− mice were pretreated with Paeonol (30 mg/kg) for consecutive 7 days by intraperitoneal injection. After catheter guide wires injury, those animals were continuously treated with Paeonol until tissues were harvested (Figure 1A). H&E was performed to observe vascular pathological changes. At the third day after surgery, most endothelial cells were denuded by catheter guide wires. Paeonol treatment did not change the thickness of the vascular wall, as well as lumen areas (Supplementary Figure 2A and B). However, at the seventh day after catheter guide wires, Paeonol treatment significantly suppressed vascular neointima formation characterized by decreased neointima areas, media layer areas, and ratio of neointima and media layer areas (Figure 1B–1D). Similar results were observed at the 10th day after injury, when Paeonol treatment dramatically suppressed neointima areas, media layer areas, and the ratio of neointima and media layer areas (Figure 1E–1G). Our IF staining against the CD31 antibody further indicated that a higher expression level of CD31 was exhibited around the inner neointima after Paeonol treatment (Figure 1H; Supplementary Figure 3). Our data showed that Paeonol attenuates vascular stenosis, possibly through vascular reendothelialization.
Paeonol Promotes Vascular Endothelial Cell Proliferation
HUVEC was treated with Paeonol (10 μM) for 24 h, and our CCK-8 assay results indicated that Paeonol treatment enhanced HUVEC viability (Figure 2A). The number of HUVEC-Cs was counted, and we observed that Paeonol treatment significantly increased cell numbers following 24 h, 48 h and 72-h treatment (Figure 2B). Paeonol treatment regulated the transcription level of cell cycle-related genes characterized by suppressing cell cycle negative related genes as P14arf, P18ink4c, and P19arf, whereas increasing cell cycle positive related genes CCND1, which was determined by Real-Time PCR (Figure 2C). Based on the flow cytometry analysis after PI staining, we found that Paeonol treatment induced HUVEC-C to enter the synthesis phase during cell cycle (Figure 2D; Supplementary Figure 4). BRDU assay showed that Paeonol significantly increased the percentage of BRDU-positive HUVEC cells (Figure 2E and Figure 2F). We next sought to determine whether Paeonol induced endothelial cell proliferation in our animal studies. At the third day after vascular injury, the endothelial was undetectable due to catheter guide wires injury. However, at the seventh day after catheter guide wires injury, the endothelial cells mainly exhibited around the inner part of neointima and more proliferating endothelial cells displayed after Paeonol treatment, which was determined by using IF staining against CD31 and PCNA antibodies (Figure 2G). Similar results were also exhibited at the 10th day after vascular injury. Within the endothelial layer of neointima, Paeonol treatment induced PCNA and Ki67 expression, which was evaluated using IHC staining (Supplementary Figure 5). These data indicated that Paeonol induced endothelial cell proliferation response to vascular injury.
Paeonol Promotes Vascular Endothelial Cell Motility
We performed Boyden migration assay and observed that Paeonol significantly induced HUVEC migration, and the number of HUVECs that passed through Boyden’s chamber was dramatically increased (Figure 3A and Figure 3B). Matrigel-based Tube Formation Assay was performed to evaluate whether Paeonol promotes endothelial cell regulated tube formation. After Paeonol treatment, more tube-like phenotypes, including tube number and partially tube-like branches, were exhibited comparing vehicle groups (Figure 3C and Figure 3D). We also performed Spheroid Sprouting Assay, which turned out that Paeonol observably enhanced both the number of sprouts and sprouts lengths (Figure 3E–3G). The metabolism of extracellular matrix plays a pivotal role in regulating cell motility. After Paeonol treatment, we evaluated transcription levels of extracellular matrix-related genes using Real-Time PCR, and the results indicated that transcription levels of Collagen 1, Fibronectin, VE-Cadherin, and MMP9 dramatically increased (Figure 3H). Protein level of VE-Cadherin was also evaluated, and we observed that Paeonol observably induced VE-Cadherin expression in HUVEC(Figure 3I and Figure 3J). Our data indicated that Paeonol can significantly induce the motility of endothelial cells.
Paeonol Induces Endothelial Cell c-Myc Expression After Vascular Injury
Based on our previous studies of Paeonol regulated pathological vascular remodeling by monitoring vascular smooth muscle cell phenotypic switching,26 we hypothesized that Paeonol may contribute to reendothelialization, which is involved in pathological vascular remodeling. We treated HUVEC with Paeonol and performed Real-Time PCR to evaluate vasculogenic signaling pathways. Our results indicated that Paeonol could observably induce c-Myc, as well as VEGF signaling pathway expression (Supplementary Figure 6). We first sought to determine whether Paeonol directly regulates the expression level of c-Myc in endothelial cells. Paeonol treatment promoted c-Myc transcription levels in both HUVEC-C and HUVEC (Supplementary Figure 7A). We treated HUVEC-C with different doses of Paeonol, including 1 μM, 5 μM, 10 μM, 15 μM, and 20 μM. Proteins were harvested, and Western blot was performed. Our results indicated that 5 μM, 10 μM, 15 μM, and 20 μM Paeonol treatment observably induced c-Myc expression in HUVEC-C (Figure 4A and Figure 4B). After 10 μM of Paeonol treatment, c-Myc protein levels in HUVEC-C were evaluated at different time points, including 6 h, 12 h, 24 h, 36 h, and 48 h. Our Western blot data indicated that Paeonol treatment for 6 h significantly induced c-Myc expression in HUVEC-C, and a high expression of c-Myc could be detected after 48-h treatment (Figure 4C and Figure 4D). The expression of c-Myc in HUVEC-C also increased following Paeonol treatment (Supplementary Figure 7B). We further determined the expression pattern of c-Myc and observed that c-Myc was specifically expressed in nucleus, which can be enhanced following Paeonol treatment (Figure 4E and Figure 4F). We next sought to determine whether Paeonol induced c-Myc expression in our animal studies. At the third day after the catheter guide wires injury, lower expression of c-Myc was exhibited in the media smooth muscle layer, as well as in adventitia layer. Whereas no distinguishable difference was displayed between the Paeonol group and the vehicle group (Supplementary Figure 7C). At the seventh day after catheter guide wires injury, higher expression of c-Myc was exhibited within the media smooth muscle cell layer, neointima layer, and inner endothelial monolayer. Endothelial c-Myc dramatically increased after Paeonol treatment (Figure 4G and Figure 4H). Our data indicated that Paeonol induces endothelial cell c-Myc expression after vascular injury.
Paeonol Actives Endothelial Cell VEGF Signaling Pathway After Vascular Injury
To confirm whether VEGF signaling pathway is involved in reendothelialization, we performed Real-Time PCR to evaluate targets of VEGF signaling pathway. Our results indicated that Paeonol treatment observably induced VEGFA121, VEGFA165, VEGFA189, VEGFR1, and VEGFR2 expression (Figure 5A). After Paeonol treatment, protein was harvested after 6 h, 12 h, 24 h, 36 h, and 48 h. Our Western blot results indicated that Paeonol treatment dramatically induced VEGFR2 expression after 6 h, and high expression levels of VEGFR2 were detectable from 6 h to 48 h (Figure 5B and Figure 5C). VEGFR2 ubiquitin is expressed in HUVEC and could be significantly enhanced after Paeonol treatment (Figure 5D and Figure 5E). We further evaluated whether Paeonol treatment induced VEGFR2 expression in our animal studies. For catheter guide wires injury model, Paeonol treatment dramatically induced VEGFR2 expression, and high expression of VEGFR2 was exhibited in the inner layer of neointima, which was determined by IHC staining (Figure 5F and Figure 5G). The skeletal injury induced angiogenesis model was also used in our studies. Our IF staining against CD31 and VEGFR2 antibodies indicated that Paeonol could induce endothelial cell VEGFR2 expression during skeletal muscle injury induced angiogenesis (Supplementary Figure 8). Our data indicated that Paeonol activates endothelial cell VEGF signaling pathway after vascular injury.
Paeonol Induces Reendothelialization by Regulating the Interaction Between c-Myc and VEGFR2 After Vascular Injury
Both c-Myc and VEGFR2 contributed to reendothelialization. However, whether c-Myc interacts with VEGFR2 is largely unknown. We first analyzed protein–protein interaction using the STRING database (https://www.string-db.org/), including c-Myc, VEGFA, VEGFR1, VEGFR2, and VEGFR3. Our analysis of data suggested that c-Myc can interact with VEGFA, VEGFR1, and VEGFR2 (Figure 6A). To next seek to evaluate the interaction between Paeonol and c-Myc, VEGFR2, we conducted Molecular docking and measured the binding energy of Paeonol with c-Myc and VEGFR2. Multiple potential binding sites within c-Myc and VEGFR2 have been displayed (Figure 6B and Figure 6C). When the value of binding energy is less than zero, those binding sites are considered spontaneously binding and interacting with paeonol. −3.6 of binding energy exhibited between Paeonol and c-Myc, and −3.8 of binding energy exhibited between Paeonol and VEGFR2 (Figure 6D). We further tried to predict the potential binding sites between c-Myc and VEGFR2 using ZDOCK (Figure 6E). 3D structures of c-Myc and VEGFR2 were obtained from RCSB database (https://www.rcsb.org). c-Myc served as ligand and VEGFR2 served as acceptor. The potential binding sites identified using ZDOCK database (https://zdock.umassmed.edu/). The potential binding sites between c-Myc and VEGFR2 can form a complex that was determined by binding energy and interface area using PDBePISA database (https://www.ebi.ac.uk/msd-srv/prot_int/). Our data indicated that five complexes exhibited which likely the potential binding sites between c-Myc and VEGFR2 (Supplementary Figure 9). We also performed a CO-immunoprecipitation Assay to evaluate the interaction between c-Myc and VEGFR2. Total proteins prepared from HUVEC, and after antibodies immunoprecipitation, we observed that c-Myc could bind to VEGFR2 (Figure 6F). We next sought to determine expression patterns c-Myc and VEGFR2 in HUVEC. Our IF staining against c-Myc and VEGFR2 antibodies indicated that c-Myc and VEGFR2 CO-expressed in the nucleus (Figure 6G). Those data demonstrated that endothelial cell c-Myc interacts with VEGFR2 to promote reendothelialization after vascular injury.
Inhibition of the VEGF Signaling Pathway Attenuates Paeonol Associated Reendothelialization, Which is Essential in Suppressing Pathological Vascular Remodeling
To identify whether Paeonol regulates reendothelialization specifically through c-Myc/VEGF Pathway, we inhibited VEGF signaling pathway by Ki8751 treatment, a VEGFR2 inhibitor, to suppress VEGFR2. Paeonol treatment promoted HUVEC-C viability, whereas VEGFR2 inhibition can attenuate Paeonol treatment induced HUVEC-C viability (Figure 7A). After inhibition of the VEGF signaling pathway following Paeonol treatment, we used Real-Time PCR to evaluate cell cycle-related genes and observed that transcription levels of P14arf, P18ink4c were reduced, whereas CCND1 increased (Figure 7B). After inhibition of the VEGF signaling pathway following Paeonol treatment, BRDU incorporation assay data indicated that inhibition of the VEGF signaling pathway could attenuate Paeonol treatment induced BRDU-positive cells (Figure 7C and Figure 7D). Inhibition of the VEGF signaling pathway can also reduce Paeonol treatment induced cell motility (Figure 7E and Figure 7F).
Discussion
This study provides evidence that Paeonol promotes reendothelialization following artery injury. Paeonol induces c-Myc expression, which is associated with VEGFR2, to accelerate reendothelialization and eventually suppress pathological vascular remodeling (Figure 7G).
Vascular endothelial cell exhibits high plasticity.35,36 High plasticity is critical not only for vascular development but also important for endothelium repair. Repair of endothelium is mediated by proliferation, differentiation and arrangement of resident endothelial cells, circulating endothelial progenitor cells and marrow release of endogenous progenitor cells.16,17 In this study, we demonstrated that Paeonol could induce reendothelialization after endothelial denuded by catheter guide wires injury, and our in vitro studies on HUVEC also indicated that Paeonol can promote cell proliferation and motility. However, whether existent resident endothelial cells or circulating endothelial progenitor cells and marrow release of endogenous progenitor cells are regulated by Paeonol is not clearly elucidated. Further studies will focus on identifying the major cell source that controls reendothelialization after artery endothelial injury.
Some other cell types, including SMC, fibroblast, and adipocyte, contribute to reendothelialization after artery injury. Our previous study demonstrated that Paeonol suppressed pathological vascular remodeling by regulating SMC phenotypic switching.26 Dysfunction of endothelium leads to enhanced vascular permeability-induced vascular inflammatory response. However, it is hard to convince the relationship between inflammatory stress and pathological vascular remodeling due to the different stages of vascular diseases. More studies combined with clinical observation are required to investigate the function of crosstalk between endothelial cells and SMCs.
Normal primary human endothelial cells (HUVEC) and human endothelial cell line (HUVEC-C) were used in this study. However, our data indicated that HUVEC is more sensitive in responding to Paeonol treatment than HUVEC-C. Different doses of Paeonol treatment dramatically increased the viability of HUVEC, whereas no difference was exhibited in HUVEC-C after Paeonol treatment (Supplementary Figure 10A–D). Both vascular catheter guide wire injury and skeletal muscle injury models were used. Difference in morphology, functions, and behaviors of endothelial cells was exhibited between arteries and developing endothelial cells.
Conclusion
In summary, our data suggested that Paeonol could significantly accelerate reendothelialization after vascular injury through activating c-Myc-mediated VEGFR2 signaling pathway at least partially, which provides a potential strategy for endothelial repair.
Author Contributions
All authors contributed to data analysis, drafting or revising the article, have agreed on the journal to which the article will be submitted, gave final approval for the version to be published, and agree to be accountable for all aspects of the work.
Funding
This work was supported by the National Natural Science Foundation of China [grant number 81741007, 81870363]; the science & technology departments of Sichuan province [grant number 2020JDTD0025]; and the Chengdu University of Traditional Chinese Medicine [grant number 008066, 030038199, BJRC2018001/030041023, 030041224, ZKYY2004/030055180, and 242030016].
Disclosure
The authors report no conflicts of interest in this work.
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