Circ-ABCA1 promotes oxidized low-density lipoprotein-induced inflammation and phenotypic switch in vascular smooth muscle cells

Yu, Fang; Liu, JiWei; Wei, Xiao

doi:10.1016/j.clinsp.2024.100343

Abstract

Objectives

Atherosclerosis (AS) is a chronic inflammatory disease of the arterial wall, in which Human Vascular Smooth Muscle Cells (HVSMCs) are involved. Nevertheless, the functions and mechanisms of circRNAs in oxidized Low-Density Lipoprotein (ox-LDL)-induced vascular smooth muscle cells remain unclear.

Methods

Circ-ABCA1 expression was measured in the models of AS. Then, in the vitro model, oligonucleotide transfection was performed, followed by an analysis of VSMC proliferation, migration, inflammation, and phenotypic switch. Also, in the in vivo model, mice were injected with shRNA lentivirus, followed by histological examination of aortic tissues. Finally, the interaction of circ-ABCA1, miR-885–5p, and ROCK2 was identified.

Results

Circ-ABCA1, was confirmed to be overexpressed in ox-LDL-induced VSMCs and mouse models of AS. Functionally, silencing circ-ABCA1 via oligonucleotide transfection suppressed VSMC proliferation, migration, inflammation, and phenotypic switch in vitro and prevented AS development in mice in vivo. Mechanistically, circ-ABCA1 absorbed miR-885–5p, which targeted ROCK2.

Conclusion

Taken together, the data from this study suggest that circ-ABCA1 mediates cellular inflammation and phenotype switching through the miR-885–5p/ROCK2 axis in ox-LDL-induced VSMCs, and the circ-ABCA1/miR-885–5p/ROCK2 axis is a new potential biomarker for the treatment of AS.

HIGHLIGHTS

Si-circABCA1 inhibits VMSC malignant proliferation, inflammation, and phenotypic switch.

miR-885–5p blocks the promoting effects of circABCA1 on VMSCs.

CircABCA1 regulates the miR-885–5p/ROCK2 axis in VMSCs.

Knockdown of circABCA1 reduces arterial plaque size and improves inflammation in AS mice.

Introduction

Atherosclerosis (AS), originating from the intima, is a chronic inflammatory disease of the arterial wall and a major cause of cardiovascular disease, characterized by lipid metabolism disorders.²³23 Saigusa R, Winkels H, Ley K. T-cell subsets and functions in atherosclerosis. Nature rev Cardiol 2020;17(7):387–401. Vascular Smooth Muscle Cells (VSMCs) have been believed to be key players in early and advanced AS.⁸8 Grootaert M, Bennett M. Vascular smooth muscle cells in atherosclerosis: time for a reassessment. Cardiovasc Res 2021;117(11):2326–39. VSMCs are the main cells that make up the arterial media and are essential for maintaining the integrity of the arterial wall. Indeed, VSMCs participate in arterial wall remodeling, and cellular viability, migration, and phenotypic switch are of significance in the progression of AS.¹³13 Hu D, Yin C, Luo S, Habenicht A, Mohanta S. Vascular smooth muscle cells contribute to atherosclerosis immunity. Front Immunol. 2019;10:1101.,⁶6 Ding Y, Tang T, Lu J, Wang J. Circ_UBR4 Knockdown alleviates oxidized low-density lipoprotein-provoked growth and migration of human vascular smooth muscle cells by acting on the miR-637/FOXO4 Pathway. J Cardiovasc Pharmacol 2021;78(4):534–43. Therefore, exploring the action of VSMCs in AS is crucial for understanding the pathogenesis of AS and developing new therapeutic measures.

Circular RNA (circRNA) is a kind of endogenous non-coding RNA that is covalently closed and highly stable.³¹31 Vo J, Cieslik M, Zhang Y, Shukla S, Xiao L, Zhang Y, et al. The landscape of circular RNA in cancer. Cell 2019;176(4):869–81. e813. Computational analysis of RNA sequencing has discovered thousands of circRNAs expressed in the cardiovascular system.²2 Aufiero S, Reckman Y, Pinto Y, Creemers E. Circular RNAs open a new chapter in cardiovascular biology. Nat Rev Cardiol 2019;16(8):503–14. Many circRNAs regulate gene expression by absorbing microRNA (miR) in the physiological and pathological processes of various diseases, including cardiovascular diseases.¹⁵15 Kristensen L, Andersen M, Stagsted L, Ebbesen K, Hansen T, Kjems J. The biogenesis, biology and characterization of circular RNAs. Nat Rev Genet 2019;20(11):675–91. Circ-ABCA1 has been currently identified to be up-regulated after Spinal Cord Injury (SCI) and it exerts neurosuppressive effects when being silenced.³⁵35 Yue S, Su X, Teng J, Wang J, Guo M. Cryptotanshinone interferes with chondrocyte apoptosis in osteoarthritis by inhibiting the expression of miR-574-5p. Mol Med Rep 2021;23(6):424. However, whether circ-ABCA1 mediates AS has not been elucidated. miRs are capable of regulating a variety of physiological and molecular signaling pathways and mediating pathological and physiological changes in VSMC function.²⁴24 Shoeibi S. Diagnostic and theranostic microRNAs in the pathogenesis of atherosclerosis. Acta Physiol (Oxf) 2020;228(1):e13353. For example, miR-141–5p protects against AS in part by inhibiting VSMC inflammation, proliferation, and migration,¹⁹19 Li Y, Li H, Chen B, Yang F, Hao Z. miR-141-5p suppresses vascular smooth muscle cell inflammation, proliferation, and migration via inhibiting the HMGB1/NF-κB pathway. J Biochem Mol Toxicol 2021;35(8):e22828. and miR-33a-5p prevents VSMCs from ox-LDL-induced calcification.¹⁰10 Han R, Luo J, Wang L, Li L, Zheng H. miR-33a-5p suppresses ox-LDL-stimulated calcification of vascular smooth muscle cells by targeting METTL3. Cardiovasc Toxicol 2021;21(9):737–46. miR-885–5p has been confirmed to be abnormally expressed in elderly patients with cardiovascular disease and may prevent and treat cardiovascular disease.²⁵25 Streese L, Demougin P, Iborra P, Kanitz A, Deiseroth A, Kroöpfl J, et al. Untargeted sequencing of circulating microRNAs in a healthy and diseased older population. Sci Rep 2022;12(1):2991.,²⁹29 Tang J, Chen L, Qin Z, Sheng R. Structure, regulation, and biological functions of TIGAR and its role in diseases. Acta Pharmacol Sinica 2021;42 (10):1547–55. In addition, miR-885–5p has also been revealed to be involved in fat/lipid metabolism.²¹21 Raitoharju E, Seppäaläa I, Lyytikäainen L, Viikari J, Ala-Korpela M, Soininen P, et al. Blood hsa-miR-122-5p and hsa-miR-885-5p levels associate with fatty liver and related lipoprotein metabolism-The Young Finns Study. Sci Rep 2016;6:38262.

The study targeted to explore the interrelationships of circ-ABCA1, miR-885–5p, and ROCK2 in AS by establishing AS cell models and animal models using human VSMCs and ApoE knockout mice. Ultimately, a novel molecular reference targeting AS may be developed based on the axis of circ-ABCA1/miR-885–5p/ROCK2.

Materials and methods

Clinical samples

Forty-six AS patients and 15 healthy subjects were recruited from Yantaishan Hospital between March 2017 and June 2019. All patients were diagnosed with carotid AS by angiography, and those with cancer and autoimmune or inflammatory diseases were excluded. The patient’s blood samples were collected, and sera were obtained by centrifugation at 1000 × g and stored at –80 °C for RNA extraction. For human study, written informed consent and approval documents from the Ethics Committee of Yantaishan Hospital were obtained.

Cell culture

Human VSMCs (ATCC, USA) were grown in Ham’s F-12 K medium (Gibco/BRL life Technologies, Germany) containing 10 % fetal bovine serum (Hyclone, USA), 100 U/mL penicillin, and 100 mg/mL streptomycin, and placed under humidified conditions of 37 °C, 5% CO₂. VSMCs were treated with 50 μg/mL Ox-LDL (Peking Union Biology Company, China) for 6 h, 12 h, and 24 h to establish an in vitro AS model.¹⁴14 Huang S, Luo W, Wu G, Shen Q, Zhuang Z, Yang D, et al. Inhibition of CDK9 attenuates atherosclerosis by inhibiting inflammation and phenotypic switching of vascular smooth muscle cells. Aging 2021;13(11):14892–909.

Actinomycin D and RNase R treatment

The ring structure of circABCA1 was determined by actinomycin D and RNaseR treatment. Total RNA from VSMCs was incubated with 3 U/ μg RNase R (Geneseed, China) or diethylpyrocarbonate-treated water (Sigma) at 37 °C.

To test for genetic stability, transfected VSMCs were treated with 4 μM actinomycin D for 0 h, 2 h, 4 h and 6 h, and analyzed by quantitative PCR to determine circABCA1 or GAPDH levels.

Cell transfection

All transfection oligonucleotides/plasmids were obtained from Gene-Pharma (Shanghai, China), including small interfering RNAs targeting circABCA1 and ROCK1 (si-circABCA1: ATGAATGGAGGAGGGAGAGC, si-ROCK2: GTCCTTGATTTAGATTTTCCTGC), overexpression vectors (oe-circABCA1, oe-ROCK2), miR-885–5p mimic/inhibitor, and the corresponding negative controls. Oligonucleotides (30 nM) or plasmids (100 ng) were transfected into VMSCs using Lipofectamine 2000 (Invitrogen). Quantitative PCR or immunoblotting was required to examine the transfection efficacy at 48 h post-transfection.

CCK-8 analysis

VMSCs were allowed to grow in 96-well plates containing DMEM (100 μL/well) at 2 × 10³ cells/well for 0 h, 24 h, 48 h, and 72 h. At each time point, 10 μL of CCK-8 solution (Dojindo, Japan) was co-cultured for 2 h avoiding light at 37 °C. Absorbance was measured by a microplate reader (Bio-Rad, Hercules, CA) at 450 nm.

ELISA

To evaluate the inflammatory response of VMSC, VMSCs were lysed and the supernatants were collected to measure IL-1β, IL-6, and TNF-α using commercial assay kits (Thermo Fisher Scientific, USA).

Wound healing assay

Wound-healing assay was used to assess VSMC migration. VSMCs were seeded to generate confluent monolayers in 6-well plates and wounds were created by scraping cells with a 200 μL sterile pipette and were conditioned to recovery for 48 h. At that time, images of wounds were captured with a microscope.

RT-qPCR

Total RNA from sera, mouse aortic tissue, and VMSCs was extracted by TRIzol reagent and reverse transcribed using the PrimeScript RT Master Mix kit (Takara). In the PCR system, SYBR® Green PCR Master Mix (Vazyme Biotech) was utilized, and the reaction volume was 10 µL using 5 µL 2 × PCR master mix (SYBR Premix Ex Taq), 0.5 µL PCR Primer, and 2 µL cDNA diluted to 20 µL ddH₂O. Gene expression was calculated using the 2^–ΔΔCt method and normalized to GAPDH. Primers are shown in Table 1.

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Table 1
PCR primer sequence.

Western blot

Mouse aortic tissue and VMSCs were lysed with RIPA lysis buffer (Beyotime, China), and the products were analyzed by a BCA kit (Cowbiotech, China). After gel-separation by SDS-PAGE, 30 μg of protein was loaded onto a polyvinylidene fluoride membrane (Millipore, USA), followed by addition of 5 % bovine serum albumin and incubation with primary antibodies overnight at 4 °C including p65 (sc-8008, Santa Cruz Biotechnology), p-p65 (3033, Cell Signaling Technology), Ki-67 (ab15580, Abcam), α-SMA (A5228, MilliporeSigma), OPN (ab8448, Abcam). Afterward, Horseradish Peroxidase (HRP)-conjugated secondary antibody (ab6721; Abcam) was added to develop bands which were then scanned using Image Lab software (Bio-Rad).

Dual-luciferase reporter assay

Fragments of Wild-Type (WT) or Mutant (MUT) circABCA1 and ROCK2 3′UTR containing the miR-885–5p binding site were synthesized and cloned into pmirGLO vector (Promega, USA) to generate recombinant luciferase vector (WT/MUT-circACBA1, WT-MUT-ROCK2). After co-transfection with miR-885–5p mimic or mimic NC in VSMCs according to Lipofectamine 2000, the luciferase activity of the recombinant luciferase reporter was determined using a dual-luciferase reporter assay system (Promega). The relative firefly luciferase activity was calculated by normalizing to renilla luciferase activity.

RIP experiment

RIP analysis was performed by EZ-Magna RIP kit (Millipore, USA). VSMCs were made into lysates using RIP lysis buffer and combined with protein A/G magnetic beads and antibodies against IgG (Millipore) or AGO2 (Abcam). Then, purified RNA was obtained from a bead binding complex for quantitative PCR to measure RNA abundance.

Animal experiment

Animals underwent treatment with the approval of the Animal Ethics Committee of Yantaishan Hospital. Twenty male ApoE^–/ mice (5–6 weeks old, SJA Animal Experiment Co., Ltd., China) were randomized into 4 groups (n = 5): 1 normal diet group (10 % fat, 20 % protein, 70 % carbohydrate) and 3 high-fat diet groups (60 % fat, 20 % protein, 20 % carbohydrate). All mice were fed for 12-weeks at 20-25 °C with a 12/12 light-dark cycle in the SPF environment. shRNA lentivirus targeting circABCA1 (sh-circABCA1, Gene-Pharma) or the negative control were injected via tail vein (1 × 10⁹ PFU) into mice fed a high-fat diet every 3-weeks. Atorvastatin (AVT, 10 mg/kg) was administrated daily as a positive control. Finally, the mice were exposed to excess CO₂, and the mouse aortic tissues were collected, some were fixed with 4% paraformaldehyde, and the rest were placed at –80 °C.

HE staining

Aortic pathology was assessed as previously described.¹¹11 Hao Y, Lu C, Zhang B, Xu Z, Guo H, Zhang G. CircPVT1 up-regulation attenuates steroid-induced osteonecrosis of the femoral head through regulating miR-21-5p-mediated Smad7/TGFβ signalling pathway. J Cell Mol Med 2021;25(10):4608–22. The tissue was embedded in paraffin, cut into 5 μm sections, and stained with HE staining solution.

IHC staining

Aortic tissues were dewaxed in xylene, blocked with 3% H₂O₂, and added with 5% BSA for 15 min. Primary antibodies α-SMA (A5228, MilliporeSigma) and OPN (ab8448, Abcam) were supplemented to the tissues at 4 °C overnight, followed by HRP-labeled IgG secondary antibody for 1 h. Finally, DAB development was implemented for 10 min.³³33 Wu S, Zhou P, Chen J, Lei J, Hua L, Dong Y, et al. circ-PTK2 (hsa_circ_0008305) regulates the pathogenic processes of ovarian cancer via miR-639 and FOXC1 regulatory cascade. Cancer Cell Inter 2021;21(1):277.

Data analysis

Statistical analysis was performed using GraphPad Prism 9.0 and data collected from at least three independent experiments were shown as mean ± Standard Deviation (SD). Two sets of data were compared by Student’s t-test, and multiple sets were by one-way ANOVA; p < 0.05 was considered a significant difference.

Results

CircABCA1 expression at a high level in AS

Firstly, the expression of circABCA1 in AS was examined. CircABCA1 levels were higher in sera of AS patients than in healthy subjects (Fig. 1A). Since the formation of atherosclerotic plaques has an important relationship with the malignant proliferation of VMSCs, abnormally expressed circABCA1 is considered to relate to the malignant proliferation of VMSCs. Therefore, ox-LDL was used to induce the proliferation of VMSC, and the changes of circABCA1 were examined by quantitative PCR. Fig. 1B demonstrates the increase in circABCA1 levels after 12 h and 24 h of ox-LDL treatment. The ring structure of circABCA1 was examined by actinomycin D and RNase R experiments. As the results suggested, circABCA1 had a longer half-life than linear GAPDH mRNA, and RNsae R degraded linear GAPDH mRNA, but had no effect on circABCA1 expression (Fig. 1C D). In summary, circABCA1 has a ring structure and is highly expressed in AS.

Fig. 1.
CircABCA1 expression maintains a high level in AS. CircABCA1 expression in patients’ sera (A) and VMSCs treated with ox-LDL for 0 h, 6 h, 12 h, and 24 h (B); The stability of circABCA1 (C) and the ring structure of circABCA1 (D); data are expressed as mean ± SD (n = 3); *p < 0.05.

Si-circABCA1 inhibits vmsc malignant proliferation, inflammation, and phenotypic switch

Subsequently, circABCA1-targeting siRNA was transfected into ox-LDL-treated VMSC to investigate the biological function of circABCA1. Transfection of si-circABCA1 reduced circABCA1 levels in VMSCs (Fig. 2A). CCK-8 assay showed that ox-LDL treatment significantly promoted the proliferation of VMSC, but circABCA1 knockdown inhibited the proliferation of VMSC (Fig. 2B). In addition, the promoting effect of ox-LDL on the proliferation protein Ki-67 was alleviated by knockdown of circABCA1 (Fig. 2C). Subsequently, wound healing experiments indicated that ox-LDL enhanced the migration ability of VMSCs, but this effect was inhibited when si-circABCA1 was introduced (Fig. 2D). NF-κB pathway regulates inflammation and mediates the development of AS.¹⁶16 Lawrence T. The nuclear factor NF-kappaB pathway in inflammation. Cold Spring Harb Perspect Biol 2009;1(6):a001651. This research, therefore, assessed inflammation by ELISA and immunoblotting. In fact, ox-LDL treatment induced increased levels of inflammatory factors and promoted the phosphorylation of NF-κB in VMSCs, while silencing circABCA1 reduced the inflammation in VMSCs (Fig. 2E F). During AS development, contractile VMSCs transform into secretory VMSCs and VMSCs acquire the ability to proliferate and migrate. Marker proteins for both phenotypes were subsequently assessed by immunoblotting. As measured, ox-LDL resulted in a decrease in α-SMA expression and an increase in OPN expression, but downregulating circVMSC rescued the changes in both proteins.

Fig. 2.
Si-circABCA1 inhibits VMSC malignant proliferation, inflammation, and phenotypic switch. si-circABCA1 was transfected into ox-LDL-treated VMSCs. Changes in circABCA1 expression (A), proliferation (B), Ki-67 protein expression (C), migration ability (D), levels of inflammatory factors (E), p-NF-κB protein expression (F), α-SMA and OPN protein expression (G); data are expressed as mean ± SD (n = 3); *p < 0.05.

CircABCA1 competitively binds miR-885–5p

Through the bioinformatics website https://circinteractome.nia.nih.gov/, 10 miRNAs were found to share potential binding sites with circABCA1. RIP screening further targeted miR-885–5p as the study object because of its enrichment with circABCA1 in Ago2 magnetic beads (Fig. 3A B). Subsequently, the targeting relationship was further verified, as the results showed that WT-circABCA1 had a decreased luciferase activity when co-transfected with miR-885–5p mimic (Fig. 3C). Actually, miR-885–5p levels were lower in both AS patients and ox-LDL-treated VMSCs, but circABCA1 silencing restored miR-885–5p expression (Fig. 3D E).

Fig. 3.
CircABCA1 competitively binds to miR-885–5p. Potential binding sites of circABCA1 and miR-885–5p on the https://circinteractome.nia.nih.gov/ (A), verification of circABCA1 and miR-885–5p targeting relationship (B‒C); miR-885–5p expression in patients’ sera (D) and VMSCs after knockdown of circABCA1 (E); data are expressed as mean ± SD (n = 3); *p < 0.05.

miR-885–5p blocks the promoting effects of circABCA1 on VMSCs

Based on a co-transfection design, ox-LDL-treated VMSCs were intervened with oe-circABCA1 and miR-885–5p mimic. As measured, oe-circABCA1 promoted circABCA1 and down-regulated miR-885–5p levels, while miR-885–5p mimic did not affect circABCA1 but restored miR-885–5p levels (Fig. 4A). Functional assays discovered the promoting effects of oe-circABCA1 on the proliferative, migratory, and inflammatory abilities of VMSCs, but concurrent induction of miR-885–5p reduced the changes in VMSC malignant proliferation, inflammation, and phenotypic switch (Fig. 4B C D E F G).

Fig. 4.
miR-885–5p blocks the promoting effects of circABCA1 on VMSCs. oe-circABCA1 and miR-885–5p mimic were co-transfected into ox-LDL-treated VMSCs. Changes in circABCA1 and miR-885–5p expression (A), proliferation (B), Ki-67 protein expression (C), migration ability (D), levels of inflammatory factors (E), p-NF-κB protein expression (F), α-SMA and OPN protein expression (G); data are expressed as mean ± SD (n = 3); *p < 0.05.

ROCK2 is a target gene of miR-885-5p

Bioinformatics website found 10 target genes with potential binding sites to miR-885–5p, and ROCK2 and miR-885–5p were enriched in Ago2 magnetic beads by RIP screening (Fig. 5A B). The dual luciferase reporter assays further confirmed their targeting relationship as evidenced by miR-885–5p mimic-induced impairment of luciferase activity of WT-ROCK2 (Fig. 5C). Furthermore, oe-LDL induced ROCK2 expression, but this increase was prevented in the presence of miR-885–5p mimic in VMSCs (Fig. 5D).

Fig. 5.
ROCK2 is a target gene of miR-885-5p. Potential binding sites of ROCK2 and miR-885–5p on the https://starbase.sysu.edu.cn (A), verification of ROCK2 and miR-885–5p targeting relationship (B-C); ROCK2 expression in VMSCs after overexpression of miR-885–5p (D); data are expressed as mean ± SD (n = 3); *p < 0.05.

CircABCA1 regulates the miR-885–5p/ROCK2 axis in VMSCs

Subsequently, a co-transfection plan was implemented with si-circABCA1 and oe-ROCK2 into VMSCs. Fig. 6A and 6B checked the elevation of miR-885-5p and reduction of ROCK2 levels in VMSCs after sicircABCA1 introduction, while oe-ROCK2 did not affect miR-885-5p but restored ROCK2 levels. Functional experiments discovered that the effects of si-circABCA1 on VMSCs were reduced by oe-ROCK2, mainly manifested in the proliferation ability, Ki-67 protein expression, migration ability, inflammatory factor levels, NF-κB phosphorylation, and secretory transformation (Fig. 6C D E F G H).

Fig. 6.
CircABCA1 regulates the miR-885–5p/ROCK2 axis in VMSCs. si-circABCA1 and oe-ROCK2 were co-transfected into ox-LDL-treated VMSCs. Changes in miR-885–5p and ROCK2 protein expression (A, B), proliferation (C), Ki-67 protein expression (D), migration ability (E), levels of inflammatory factors (F), p-NF-κB protein expression (G), α-SMA and OPN protein expression (H); data are expressed as mean ± SD (n = 3); *p < 0.05.

Knockdown of circABCA1 reduces arterial plaque size and improves inflammation in AS mice

To further support the in vitro results, in vivo experiments were next performed. AS mice were injected with sh-circABCA1, causing the decline of circABCA1 and ROCK2 levels in the aortic tissues. HE staining depicted that sh-circABCA1 reduced plaque size, and the treatment effect was close to that of atorvastatin treatment (Fig. 7C). IHC staining showed that sh-circABCA1 reduced the positive rate of OPN and promoted that of α-SMA in the aortic tissues (Fig. 7D). In addition, sh-circABCA1 also reduced Ki-67 and p-NF-κB expression in the aortic tissues (Fig. 7E).

Fig. 7.
Knockdown of circABCA1 reduces arterial plaque size and improves inflammation in AS mice. circABCA1 and ROCK2 expression in aortic tissue (A‒B); HE staining to detect aortic pathological damage (C); IHC staining to assess the number of positive cells for OPN and α-SMA in the aorta (D); Ki-67 and P-NF-κB protein expression in the aorta (E); data are expressed as mean ± SD (n = 5); *p < 0.05.

Discussion

Dysfunction of VSMCs has been accepted to be associated with the formation of AS.¹²12 He L, Zhou Q, Huang Z, Xu J, Zhou H, Lv D, et al. PINK1/Parkin-mediated mitophagy promotes apelin-13-induced vascular smooth muscle cell proliferation by AMPKα and exacerbates atherosclerotic lesions. J Cell Physiol 2019;234(6):8668–82. CircRNAs are a special class of regulators in various diseases including AS.³⁴34 Yang Y, Mao W, Wang L, Lu L, Pang Y. Circular RNA circLMF1 regulates PDGF-BBinduced proliferation and migration of human aortic smooth muscle cells by regulating the miR-125a-3p/VEGFA or FGF1 axis. Clin Hemorheol Microcirc 2022;80 (2):167–83. Based on previous studies, this study treated VSMCs with ox-LDL to establish a cellular model of AS.²⁷27 Sun C, Li J, Li Y, Li L, Huang G. Circular RNA circUBR4 regulates ox-LDL-induced proliferation and migration of vascular smooth muscle cells through miR-185-5p/FRS2 axis. Mol Cell Biochem 2021;476(11):3899–910.,⁵5 Ding P, Ding Y, Tian Y, Lei X. Circular RNA circ_0010283 regulates the viability and migration of oxidized low-density lipoprotein-induced vascular smooth muscle cells via an miR-370-3p/HMGB1 axis in atherosclerosis. Inter J Mol Med 2020;46 (4):1399–408. The research discovered that circABCA1 was upregulated in AS patients, and moreover, circABCA1 was induced by ox-LDL in VSMCs in a time-dependent manner. Furthermore, the knockdown of circABCA1 suppressed AS progression in vitro and in vivo by suppressing VMSC malignant proliferation, inflammation, and phenotypic transformation through the miR-885–5p/ROCK2 axis.

CircRNAs are important regulators of VSMC proliferation, migration and inflammation, such as circ_GRN,¹⁷17 Li X, Li L, Dong X, Ding J, Ma H, Han W. Circ_GRN promotes the proliferation, migration, and inflammation of vascular smooth muscle cells in atherosclerosis through miR-214-3p/FOXO1 Axis. J Cardiovasc Pharmacol 2021;77(4):470–9. circ_CHFR³⁹39 Zhuang J, Li T, Hu X, Ning M, Gao W, Lang Y, et al. Circ_CHFR expedites cell growth, migration and inflammation in ox-LDL-treated human vascular smooth muscle cells via the miR-214-3p/Wnt3/β-catenin pathway. Eur Rev Med Pharmacol Sci 2020;24 (6):3282–92. and circMAPK1.⁷7 Fu X, Niu T, Yang T, Li X. CircMAPK1 promotes the proliferation and migration of vascular smooth muscle cells through miR-22-3p/methyl-CpG binding protein 2 axis. Nutr Metab Cardiovasc Dis 2021;31(7):2189–98. Abnormal proliferation of VSMCs can promote plaque formation in the early stage, but benefit in the late stage, such as preventing the rupture of the fibrous cap.³3 Bennett M, Sinha S, Owens G. Vascular smooth muscle cells in atherosclerosis. Circ Res 2016;118(4):692–702. VSMC phenotype switching has historically been considered a two-way process, with cells either adopting a physiological contractile phenotype or an alternative “synthetic” phenotype in response to injury.³⁶36 Zhang F, Guo X, Xia Y, Mao L. An update on the phenotypic switching of vascular smooth muscle cells in the pathogenesis of atherosclerosis. Cell Mol Life Sci 2021;79 (1):6. However, recent studies have believed that VSMC phenotype switching results in poorly differentiated forms lacking VSMC markers, including macrophage-like cells, responsible for the regulation of proliferation and chemotaxis-induced production of proinflammatory mediators, directly promoting AS.⁴4 Chistiakov D, Orekhov A, Bobryshev Y. Vascular smooth muscle cell in atherosclerosis. Acta Physiol (Oxf) 2015;214(1):33–50.,¹1 Allahverdian S, Chaabane C, Boukais K, Francis G, Bochaton-Piallat M. Smooth muscle cell fate and plasticity in atherosclerosis. Cardiovasc Res 2018;114(4):540–50. Therefore, modulating the phenotype of VSMCs in a direction favorable to alleviating disease progression is a promising therapeutic approach for AS. Here, circABCA1 was demonstrated as a novel regulator of VSMC phenotype switching and inflammation. The in vitro results showed that silencing circABCA1 inhibited the ability of VMSCs to proliferate and migrate and suppressed inflammatory response. Meanwhile, the present in vivo experimental results revealed that silencing circABCA1 inhibited the development of AS in vivo, similar to the therapeutic effect of atorvastatin.

Regarding the molecular mechanism of circRNAs in human pathogenesis, the most typical way for circRNAs is to absorb miR to regulate mRNA expression.³⁸38 Zhu Y, Li J, Liu H, Song Z, Yang Q, Lu C, et al. Circular RNA, hsa_circRNA_102049, promotes colorectal cancer cell migration and invasion via binding and suppressing miRNA-455-3p. Exp Ther Med 2022;23(3):244. The study indicated that miR-885–5p was a target of circABCA1. miR-885–5p is involved in various human diseases, especially different types of cancer,²⁶26 Su M, Qin B, Liu F, Chen Y, Zhang R. miR-885-5p upregulation promotes colorectal cancer cell proliferation and migration by targeting suppressor of cytokine signaling. Oncol Lett 2018;16(1):65–72. and is associated with chronic thromboembolic pulmonary hypertension²⁰20 Miao R, Dong X, Gong J, Li J, Pang W, Liu Y, et al. Analysis of significant microRNA associated with chronic thromboembolic pulmonary hypertension. Zhonghua Yi Xue Za Zhi 2018;98(18):1397–402. and embryonic development.²²22 Rodosthenous R, Burris H, Sanders A, Just A, Dereix A, Svensson K, et al. Second trimester extracellular microRNAs in maternal blood and fetal growth: an exploratory study. Epigenetics 2017;12(9):804–10. In the present study, miR-885–5p was downregulated in ox-LDL-induced VSMCs and was negatively regulated by circABCA1. Functional experiments showed that miR-885–5p prevented the promoting effects of overexpressed circABCA1 on VMSC proliferation, inflammation, and phenotypic transformation. To our knowledge, this is the first report that miR-885–5p mediates VMSC function in AS, based on the study by Streete L et al.²⁵25 Streese L, Demougin P, Iborra P, Kanitz A, Deiseroth A, Kroöpfl J, et al. Untargeted sequencing of circulating microRNAs in a healthy and diseased older population. Sci Rep 2022;12(1):2991.

To deeply understand the regulatory mechanism of miR-885–5p in AS, its target genes were predicted, and ROCK2 was identified. ROCK2 is a major regulator of central nervous system damage, and inhibition of ROCK2 can inhibit the activation of the NF-κB pathway and exert antiapoptotic and anti-inflammatory roles.¹⁸18 Li X, Tong J, Liu J, Wang Y. Down-regulation of ROCK2 alleviates ethanol-induced cerebral nerve injury partly by the suppression of the NF-κB signaling pathway. Bioengineered 2020;11(1):779–90. ROCK2 is also a key driver of cell migration⁴⁰40 Zucchini C, Manara M, Cristalli C, Carrabotta M, Greco S, Pinca R, et al. ROCK2 deprivation leads to the inhibition of tumor growth and metastatic potential in osteosarcoma cells through the modulation of YAP activity. J Exp Clin Cancer Res 2019;38 (1):503. and endothelial inflammation.²⁸28 Takeda Y, Matoba K, Kawanami D, Nagai Y, Akamine T, Ishizawa S, et al. ROCK2 regulates monocyte migration and cell to cell adhesion in vascular endothelial cells. Inter J Mol Sci 2019;20(6):1331. Therefore, ROCK2 inhibition may be a potential therapeutic strategy for AS. The study measured that ROCK2 was up-regulated in ox-LDL-induced VSMCs, which was consistent with a previous study.⁹9 Guo H, Lu Z, Zhao B, Jiang W, Xiong Y, Wang K. Effects of Bunao-Fuyuan decoction serum on proliferation and migration of vascular smooth muscle cells in atherosclerotic. Chin J Nat Med 2021;19(1):36–45. Furthermore, ROCK2 suppressed circABCA1 up-regulation-induced protection against proliferation, migration, and inflammation of VSMCs.

Previous documents have elucidated that ROCK2 affects VSMC development by regulating multiple gene expression and signaling pathways, such as MLCP,³²32 Wang Y, Zheng X, Riddick N, Bryden M, Baur W, Zhang X, et al. ROCK isoform regulation of myosin phosphatase and contractility in vascular smooth muscle cells. Circ. Res. 2009;104(4):531–40. JNK pathway,³⁰30 Tang L, Dai F, Liu Y, Yu X, Huang C, Wang Y, et al. RhoA/ROCK signaling regulates smooth muscle phenotypic modulation and vascular remodeling via the JNK pathway and vimentin cytoskeleton. Pharmacol Res 2018;133:201–12. ERK, cyclin D1 and PCNA,³⁷37 Zhao Y, Lv M, Lin H, Cui Y, Wei X, Qin Y, et al. Rho-associated protein kinase isoforms stimulate proliferation of vascular smooth muscle cells through ERK and induction of cyclin D1 and PCNA. Biochem Biophys Res Commun 2013;432 (3):488–93. whether circABCA1/miR-885–5p/ROCK2 axis regulates AS progression through these pathways requires further exploration. In addition, the mechanism by which ox-LDL induces circABCA1 upregulation in VSMCs is unclear.

Conclusion

In conclusion, circABCA1 is stably expressed in VMSC as a circRNA, which upregulates ROCK2 expression by acting as a ceRNA for miR-885–5p. Knockdown of circABCA1 can inhibit malignant proliferation, inflammation and secretory phenotype transformation of VMSCs. However, circABCA1 mainly regulates miR-885–6p/ROCK2 axis to achieve this effect. These data provide strong data support for understanding the biological role of circRNA in the pathogenesis of AS and provide potential molecular targets for the treatment of AS.

Funding

Not applicable.
Data available

Data is available from the corresponding author on request.
Ethics approval

For human study, written informed consent and approval documents from the Ethics Committee of Yantaishan Hospital were obtained. Written informed consent was obtained from all patients. Animals underwent treatment with the approval of the Animal Ethics Committee of Yantaishan Hospital.

Acknowledgments

Not applicable.

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Data availability

Data is available from the corresponding author on request.

Publication Dates

Publication in this collection
24 May 2024
Date of issue
2024

History

Received
27 Dec 2023
Accepted
03 Mar 2024

This is an Open Access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

[1] Funding

Not applicable.

[2] Data available

Data is available from the corresponding author on request.

[3] Ethics approval

For human study, written informed consent and approval documents from the Ethics Committee of Yantaishan Hospital were obtained. Written informed consent was obtained from all patients. Animals underwent treatment with the approval of the Animal Ethics Committee of Yantaishan Hospital.

	Primer sequence (5′‒3′)
hsa_circ_0137614	Forward: 5′- TGAAGCCAATCCTGTTAATGACC-3′ Reserse: 5′-GGGTAACGGAAACAGGGGTT-3′
mmu_circ_0011675	Forward: 5′- CCAGTTGTGTTAATGACCAGCC-3′ Reserse: 5′- TTCGTAGGGTGGGTAGCTCA-3′
miR-885-5p	Forward: 5′- TCCATTACACTACCCTGCCTCT -3′ Reserse: 5′- TGGTGTCGTGGAGTCG-3′
ROCK2	Forward: 5′-GGCTTGTATGAAGCCCCTGT-3′ Reserse: 5′-ACCCACTTCTGCTGCTCTTC-3′
Human GAPDH	Forward: 5′- CACCCACTCCTCCACCTTTG-3′ Reserse: 5′- CCACCACCCTGTTGCTGTAG-3′
mouse GAPDH	Forward: 5′- CATCAACGGGAAGCCCATC-3′ Reserse: 5′- CTCGTGGTTCACACCCATC-3′
U6	Forward: 5′-CTCGCTTCGGCAGCACA-3′ Reserse: 5′-AACGCTTCACGAATTTGCGT-3′

Brasil

Brasil

Circ-ABCA1 promotes oxidized low-density lipoprotein-induced inflammation and phenotypic switch in vascular smooth muscle cells

Abstract

Objectives

Methods

Results

Conclusion

HIGHLIGHTS

Introduction

Materials and methods

Clinical samples

Cell culture

Actinomycin D and RNase R treatment

Cell transfection

CCK-8 analysis

ELISA

Wound healing assay

RT-qPCR

Western blot

Dual-luciferase reporter assay

RIP experiment

Animal experiment

HE staining

IHC staining

Data analysis

Results

CircABCA1 expression at a high level in AS

Si-circABCA1 inhibits vmsc malignant proliferation, inflammation, and phenotypic switch

CircABCA1 competitively binds miR-885–5p

miR-885–5p blocks the promoting effects of circABCA1 on VMSCs

ROCK2 is a target gene of miR-885-5p

CircABCA1 regulates the miR-885–5p/ROCK2 axis in VMSCs

Knockdown of circABCA1 reduces arterial plaque size and improves inflammation in AS mice

Discussion

Conclusion

Funding

Data available

Ethics approval

Acknowledgments

References

Data availability

Publication Dates

History