Abstract
Background
Long noncoding RNAs (lncRNAs) are dysregulated in periodontitis development and involved in osteogenesis. The current study was aimed at investigating the function of lncRNA ANRIL in periodontal ligament cells (PDLCs) and potential molecular mechanisms.
Methods
Firstly, the level of ANRIL was tested by qPCR. Then, PDLCs were treated with a mineralizing solution to induce osteogenic differentiation. ALP activity was measured, and protein levels of BMP2, Osterix, and OCN were measured by Western blot. A target of ANRIL was verified using dual-luciferase reporter assay. miR-7 level was measured by qPCR, and the signals of the NF-κB pathway were tested by Western blot.
Results
ANRIL expression was downregulated in PDL tissues. Next, ALP activity and protein levels of BMP2, Osterix, and OCN were increased to show that PDLCs were differentiated. ANRIL level was increased in differential PDLCs, in which knockdown inhibited osteogenic differentiation. Then, miR-7 was found as a target of ANRIL. The miR-7 level was upregulated in PDL tissues and reduced in differential PDLCs. Inhibition of miR-7 suppressed ALP activity and BMP2, Osterix, and OCN expression. Moreover, inhibition of miR-7 reversed the effects on the osteogenic differentiation induced by knockdown of ANRIL. Besides, the levels of p-P65 and p-IκBα were elevated by ANRIL downregulation and were rescued by suppressing miR-7.
Conclusions
Knockdown of ANRIL inhibited osteogenic differentiation via sponging miR-7 through the NF-κB pathway, suggesting that ANRIL might be a therapeutic target for periodontitis.
1. Background
Periodontitis is a chronic, nonspecific, and multifactorial inflammatory disease associated with periodontal support tissue. It will cause pathological loss of the periodontal ligament and alveolar bone, leading to teeth loss ultimately [1]. Diabetes, obesity, and aging are associated with the pathogenic factors of periodontitis [2–4]. Periodontitis may be a potential risk factor for other human diseases like Alzheimer's disease and stroke, which affect human systemic health [5, 6]. The periodontal ligament (PDL), made up of collagen fiber bundles and cells, has many functions, including tooth support, tooth nutrition, alveolar bone remodeling, and damage tissue repair [7]. Periodontal ligament cells (PDLCs) play essential roles in maintaining the homeostasis of periodontal tissue and repairing periodontal ligament. Unfortunately, periodontitis injures the osteogenic differentiation of PDLCs [8]. The treatment of periodontitis is complex, and there is still a lack of early screening biomarkers and therapeutic targets.
Long noncoding RNAs (lncRNAs) are a class of more than 200 nt noncoding transcripts. Recently, with the gradual deepening of lncRNA's biological and functional roles, we found that lncRNA acts as miRNA sponges and then regulates mRNA effects [9]. An increasing body of evidence has suggested that lncRNAs are involved in human diseases, such as cardiovascular diseases [10], malignant tumors [11], and inflammation-related diseases [12]. As important inflammatory regulators, lncRNAs are often abnormally expressed in the progression of periodontitis [13] and associated with osteogenesis [14]. An antisense lncRNA, antisense noncoding RNA in the INK4 locus (ANRIL), is located at the CDKN2A/B genomic locus, consisting of at least 21 exons and a large number of reported isoforms [15]. ANRIL is reported as an immune response-related lncRNA, in which expression is reduced in the peripheral blood of patients with periodontitis [16]. However, biological functions are still largely unknown.
In the present study, the effects of ANRIL on the osteogenic differentiation of PDCLs were explored. Moreover, ANRIL was found to be sponging to miR-7. Notably, the mechanism of ANRIL sponged to miR-7 to regulate the osteogenic differentiation of PDLCs was investigated.
2. Methods
2.1. PDL Tissue Collection
A total of 30 patients with periodontitis and 30 healthy controls participated in the study. This study protocol was approved by the Ethics Committee of Beihua University Affiliated Hospital.
Written informed consent was provided before the study. All participators were diagnosed with periodontitis or not by Beihua University Affiliated Hospital. None of them had infectious diseases, a history of smoking, and orthognathic surgery. At routine premolar or third molar extractions, the PDL tissues were separated from the middle 1/3 of the dental roots. Partial tissues were stored at -80°C until further use.
2.2. Cell Culture and Osteogenic Induction
Other tissues were cut into 1 mm3 pieces and digested by 3 mg/ml of collagenase type I (Sigma-Aldrich, USA) and 4 mg/ml of dispase (Corning, USA) at 37°C. The cell suspension was maintained in DMEM (Hyclone, USA) supplemented with 10% FBS (Solarbio, China) and 1% penicillin/streptomycin (Solarbio, China) at 37°C with 5% CO2. The medium was changed every 2-3 days until cell passage to the fifth generation. For osteogenic induction, PDLCs were seeded into 6-well plates until the confluency researched exceed 70%. DMEM supplemented with 10% FBS, 10 mM β-glycerophosphate (Sigma-Aldrich, USA), 50 μg/ml vitamin C (Aladdin, China), and 10 nM dexamethasone (Aladdin, China) was used as an osteogenic-induced medium. Two weeks postincubation, PDLCs were harvested for testing osteogenic differentiation.
2.3. Alkaline Phosphatase (ALP) Activity Analysis
ALP activity was assessed by the ALP Assay Kit (Beyotime, China). Briefly, PDLCs were lysed by a lysis buffer and seeded into 96-well plates. The test buffer was added and incubated with cells at 37°C for 10 min. After stopping the reaction, the absorbance was measured at 405 nm.
2.4. Dual-Luciferase Reporter Assay
The sequences of ANRIL containing the miR-7 potential binding sites were amplified and inserted into pGL3 vectors (Promega, USA) as the ANRIL-WT group. The ANRIL-MUT group was obtained by targeted mutation. miR-7 mimic and mimic negative control (NC) were purchased from GenePharma (Shanghai, China). HEK293T cells were seeded into 24-well plates and cotransfected with ANRIL-WT or ANRIL-MUT and miR-7 mimic or mimic NC using Lipofectamine 2000 (Invitrogen, USA). After 24 h, the relative luciferase activity (firefly activity normalized to Renilla activity) was measured by Dual-Luciferase Reporter Assay Kit (Promega, USA).
2.5. Cell Transfection
shRNA-NC, shRNA-ANRIL, miR-7 inhibitor, and inhibitor-NC were all acquired from GenePharma (Shanghai, China). PDLCs in the logarithmic growth phase were seeded into 6-well plates, and the transfection process used Lipofectamine 2000 (Invitrogen, USA). After 48 h, transfection efficiency was detected.
2.6. qPCR
Total RNA was isolated from PDLCs by TRIzol reagent (Sigma-Aldrich, USA). After concentration and purity testing, RNA was reverse transcribed into cDNA using LnRcute lncRNA cDNA First Chain Synthetic Kit (Tiangen, China), and miRNA reverse transcription was conducted by miScript II RT Kit (Qiagen, Germany). INRcute lncRNA qCPR Detection Kit (SYBR Green) (Tiangen, China) was performed for qPCR of lncRNA with the following conditions: 95°C for 3 min, 40 cycles of 95°C for 5 sec, and 60°C for 15 sec. qPCR was used to measure miR-7 level by microRNA qPCR kit (SYBR Green Method) (Sango, China) with the conditions as 95°C for 30 sec, 95°C for 5 sec, and 60°C for 30 sec (40 cycles). The level of mRNA was detected by Real-Time One-Step RT-qPCR (Tiangen, China) for reverse transcription and qPCR, and the conditions were 50°C for 30 min, 95°C for 3 min, 40 cycles of 95°C for 15 sec, and 60°C for 30 sec. The reaction instrument was an ABI PRISM 7500 system (Applied Biosystems, USA). β-Actin level was performed as the loading control. The results of relative expression were assessed by the 2 − ΔΔCt.
2.7. Western Blot
The transfected cells were collected, and precooled RIPA lysate (Beyotime, China) was added to extract the total protein. After 10% SDS-PAGE, the protein was transferred to PVDF membranes (Millipore, USA) and blocked with 5% skim milk. Primary antibodies including anti-BMP2, anti-Osterix, anti-osteocalcin (OCN), anti-P65, anti-p-P65, anti-IκBα, and anti-p-IκBα were added and incubated with the membranes at 4°C overnight. After washing the membranes, the secondary antibody was added to incubate at room temperature for 1 h. The protein bands were developed by ECL Western Blotting Substrate (Pierce, USA) and then photographed. The gray analysis was performed by ImageJ software 1.48U (Bethesda, USA).
2.8. Statistical Analysis
The results in this study were analyzed by GraphPad Prism 6.0 (GraphPad Software, USA) and presented as mean ± standard deviation (SD). Student's t-test was used for multiple comparisons between two groups, and one-way ANOVA was used between three or more groups. P < 0.05 was deemed to have significant differences.
3. Results
3.1. The Level of ANRIL Was Downregulated in Periodontitis
Firstly, the PDL tissues were obtained from periodontitis patients and healthy people, and the expression of ANRIL was measured. According to the results of qPCR, the ANRIL level was reduced in PDL tissues of patients with periodontitis, compared with the healthy control group (Figure 1).
Figure 1.
The expression of ANRIL was decreased in PDL tissues of periodontitis patients. PDL tissues from 30 patients with periodontitis and 30 healthy people were collected, and then, ANRIL level was detected by qPCR. ∗∗P < 0.01.
3.2. Identification of the Osteogenic Differentiation of PDLCs
To investigate the osteogenic differentiation capability, PDLCs derived from PDL tissues were cultured in DMEM with β-glycerophosphate, vitamin C, and dexamethasone. Subsequently, some of the specific markers associated with osteogenesis were evaluated. As illustrated in Figure 2(a), ALP activity was elevated in osteogenic differentiated PDLCs. The protein levels of BMP2, Osterix, and OCN were all upregulated in PDLCs after treatment (Figures 2(b)–2(e)). Moreover, the expression of ANRIL was upregulated in differentiated PDLCs, compared with undifferentiated PDLCs (Figure 2(f)).
Figure 2.
Identification of osteogenic differentiation model. (a) ALP activity was detected in undifferentiated and differentiated PDLCs. The relative protein expression normalized to GAPDH was calculated, including (b) BMP2, (c) Osterix, and (d) OCN. (e) The protein levels of osteogenic-related markers as BMP2, Osterix, and OCN were tested by Western blot. GAPDH was performed as the housekeeping control. (f) The expression of ANRIL was measured in undifferentiated and differentiated PDLCs by qPCR. ∗P < 0.05.
3.3. Knockdown of ANRIL Inhibited Osteogenic Differentiation of PDLCs
To explore the biological functions of ANRIL in PDLCs, inhibition of ANRIL expression was conducted by transfection of shRNA-ANRIL-1 and shRNA-ANRIL-2. To examine the transfection efficiency, qPCR was conducted. Compared with the shRNA-NC group, the level of ANRIL was downregulated in the shRNA-ANRIL-1 and shRNA-ANRIL-2 groups, especially in the shRNA-ANRIL-2 group (Figure 3(a)). To evaluate the effects of ANRIL on osteogenic differentiation, ALP activity was measured. As shown in Figure 3(b), shRNA-ANRIL-2 suppressed the ALP activity, compared with shRNA-NC (Figure 3(b)). Additionally, the protein expression of BMP2, Osterix, and OCN was tested by Western blot, and the results demonstrated that knockdown of ANRIL repressed BMP2, Osterix, and OCN levels (Figures 3(c)–3(f)).
Figure 3.
(a) The transfection efficiency was measured by qPCR with PDLC transfection of shRNA-ANRIL-1, shRNA-ANRIL-2, and shRNA-NC. (b) ALP activity was detected posttransfection. The protein levels of (c) BMP2, (d) Osterix, and (e) OCN were quantified. (f) The proteins were detected by Western blot posttransfection. GAPDH was used as an internal control. ∗P < 0.05.
3.4. miR-7 Was Identified as a Target of ANRIL
The binding sites between ANRIL and miR-7 are shown in Figure 4(a). To verify the targeted relationship, a dual-luciferase reporter assay was conducted. The results demonstrated that the relative luciferase activity was decreased in HEK293T cells cotransfected with ANRIL-WT and miR-7 mimic, compared with cotransfection of ANRIL-WT and mimic NC. However, in the ANRIL-MUT group, there was no difference between the miR-7 mimic and the mimic NC (Figure 4(b)).
Figure 4.
ANRIL sponged to miR-7. (a) The binding sites between ANRIL and miR-7 are shown. The mutant sequences of ANRIL are also shown. (b) HEK293T cells were cotransfected with ANRIL-WT or ANRIL-MUT together with miR-7 mimic or mimic NC, and the relative luciferase activity was detected. ∗P < 0.05.
3.5. The Expression of miR-7 Was Evaluated in PDL Tissues and PDLCs
Subsequently, the expression of miR-7 was measured. As compared to healthy control tissues, the miR-7 level was upregulated in PDL tissues (Figure 5(a)). Additionally, the miR-7 level was decreased in differentiated PDLCs, compared with undifferentiated PDLCs (Figure 5(b)). After knockdown of ANRIL, the expression of miR-7 was elevated, compared with the shRNA-NC group (Figure 5(c)).
Figure 5.
miR-7 expression in PDL tissues and PDLCs. (a) The level of miR-7 was tested in PDL tissues from periodontitis patients and healthy control by qPCR. (b) miR-7 level was detected by qPCR in undifferentiated and differentiated PDLCs. (c) The expression of miR-7 was measured by qPCR after PDLCs were transfected with shRNA-NC and shRNA-ANRIL-2. ∗P < 0.05; ∗∗P < 0.01.
3.6. Downregulation of miR-7 Promoted Osteogenic Differentiation of PDLCs
For downregulation of miR-7, miR-7 inhibitor and inhibitor-NC were transfected into differentiated PDLCs. The data of transfection efficiency illustrated that the miR-7 level was reduced in the miR-7 inhibitor group, compared with the inhibitor-NC group (Figure 6(a)). Then, inhibition of miR-7 enhanced ALP activity and BMP2, Osterix, and OCN levels, compared with inhibitor-NC (Figures 6(b)–6(f)).
Figure 6.
miR-7 downregulation facilitated PDLC osteogenic differentiation. (a) The transfection efficiency was measured by qPCR in PDLC transfection of miR-7 inhibitor and inhibitor-NC. (b) After transfection, ALP activity was evaluated. The protein levels of (c) BMP2, (d) Osterix, and (e) OCN were quantified. (f) The proteins were assessed by Western blot. ∗P < 0.05; ∗∗P < 0.01.
3.7. Knockdown of ANRIL Inhibited Osteogenic Differentiation through Sponging miR-7
ALP activity declined in the shRNA-ANRIL-2 group, which was not affected by inhibitor-NC but further abolished by miR-7 inhibitor (Figure 7(a)). Through the results of Western blot, knockdown of ANRIL inhibited BMP2, Osterix, and OCN levels. However, their levels were reversed by miR-7 downregulation (Figures 7(b) and 7(c)).
Figure 7.
ANRIL knockdown suppresses osteogenic differentiation of PDLCs via regulating miR-7. (a) ALP activity was tested in PDLCs after transfection of shRNA-ANRIL-2 and miR-7 inhibitor. Gray analysis for Western blot of (b) BMP2, (c) Osterix, and (d) OCN protein levels. (e) The protein levels were assessed by Western blot. ∗P < 0.05.
3.8. Knockdown of ANRIL Regulated NF-κB Pathway by Mediating miR-7
The protein expression of p-P65, P65, p-IκBα, and IκBα was measured by Western blot. The data demonstrated that knockdown of ANRIL enhanced the levels of p-P65 and p-IκBα, which were rescued by inhibition of miR-7. However, both ANRIL and miR-7 did not affect P65 and IκBα levels (Figures 8(a) and 8(b)).
Figure 8.
ANRIL activated NF-κB pathway by inhibiting miR-7. (a) The relative protein expression of p-P65, P65, p-IκBα, and IκBα was quantified by normalizing to GAPDH level. (b) The protein of p-P65, P65, p-IκBα, and IκBα was examined by Western blot. ∗P < 0.05.
4. Discussion
In the present study, we aimed to explore the biological functions of lncRNA ANRIL in osteogenic differentiation in PDLCs. We found that the level of ANRIL was downregulated in PDL tissues and upregulated in differential PDLCs. Knockdown of ANRIL inhibited ALP activity and BMP2, Osterix, and OCN levels, suggesting that downregulation of ANRIL inhibited osteogenic differentiation of PDLCs.
Recently, lots of researches revealed the role of ANRIL. Polymorphisms at the ANRIL gene are associated with the risks of many human diseases, including malignancy, cardiovascular disease, bone mass, obesity, and type 2 diabetes [15]. Generally, ANRIL is a prognostic biomarker and an oncomiR in human cancers, such as lung cancer, gastric cancer, and esophageal squamous cell carcinoma [17]. In addition, dysregulation of ANRIL promotes the development of atherosclerosis and leads to coronary heart disease through mediating single nucleotide polymorphisms and injuring the endothelial cell [18, 19]. Furthermore, ANRIL mediates VEGF which has an effect on diabetic retinopathy [20]. Osteogenesis is complex and plays a crucial role in periodontitis. Several lncRNAs have been reported to be involved in osteogenic differentiation, such as PCAT1 [21], MEG3 [22], TWIST1 [23], and MSC-AS1 [24]. lncRNA HOTAIR, controlled by the dental material methacrylate, can induce the HOXC11 gene to regulate osteoblast expression [25, 26]. Depletion of lncRNA MEG3 inhibits osteogenesis of PDLCs in periodontitis [27]. However, the roles of ANRIL in osteogenic differentiation, especially in PDLCs, are still unknown. The results of this study indicated that ANRIL downregulation had inhibited effects on the osteogenic differentiation of PDLCs.
Besides, the molecular mechanism of the differentiation induced by ANRIL was further investigated. miR-7 was regarded as a sponge of ANRIL. Zhao et al. have suggested that miR-7 abolishes the attenuation of oxidative injury of human trabecular meshwork cells induced by ANRIL [28]. Shu et al. have reported that silence of ANRIL exacerbates H9c2 cell injury induced by hypoxia by miR-7-5p/SIRT1 axis [29]. Li et al. have revealed that ANRIL mediates the migration and invasion of T-cell acute lymphoblastic leukemia via miR-7-5p/TCF4 axis [30]. In our study, we also verified the ANRIL sponge to miR-7 through the dual-luciferase reporter assay.
Accumulating evidence shows that miR-7 is involved in human diseases. For example, miR-7 may function as a tumor suppressor and regulate cellular processes, including growth, metastasis, differentiation, and apoptosis [31]. Besides cancers, abnormal expression of miR-7 is a potential biomarker for type 2 diabetes, acute pancreatitis, and Alzheimer's disease [32–34]. Moreover, miR-7 plays functional roles in osteoarthritis through regulating proliferation, apoptosis, and inflammation [35]. In periodontitis, miR-7 level was reduced during osteogenic differentiation, mediated by circular RNA ADR1as to repress osteoblastic differentiation of PDLCs [36]. In the present study, the results demonstrated that the expression of miR-7 was increased in PDL tissues and reduced in differential PDLCs. Downregulation of miR-7 promoted osteogenic differentiation of PDLCs. Moreover, knockdown of ANRIL inhibited osteogenic differentiation via sponging miR-7.
The noncanonical NF-κB pathway is related to immune deficiencies, and abnormal activation of the pathway leads to the pathogenesis of a variety of autoimmune and inflammatory diseases [37]. Moreover, the NF-κB pathway is also involved in osteogenic differentiation [38, 39]. Several studies have revealed that ANRIL and miR-7 mediate NF-κB signaling. Overexpression of ANRIL facilitates angiogenesis of diabetes mellitus via activation of the NF-κB pathway [40]. miR-7 suppresses pancreatic cancer progression through inactivation of the NF-κB pathway [41]. In the present study, we found that knockdown of ANRIL enhanced the levels of p-P65 and p-IκBα, which were rescued by inhibition of miR-7. These results suggested that downregulation of ANRIL activation inhibited osteogenic differentiation of PDLCs through the NF-κB pathway by sponging miR-7.
5. Conclusions
The expression of ANRIL was decreased in PDL tissues, while the miR-7 level was increased. miR-7 was identified as a sponge of ANRIL. The level of ANRIL was elevated, and miR-7 was reduced in differentiated PDLCs. Importantly, knockdown of ANRIL inhibited osteogenic differentiation by sponging miR-7 through activating the NF-κB signaling pathway, suggesting that ANRIL contributes to periodontitis.
Acknowledgments
This work was supported by the Science and Technology Research Project of the Education Department of Jilin Province (No. JJKH20200074KJ).
Abbreviations
- ALP:
Alkaline phosphatase
- DMEM:
Dulbecco's modified Eagle's medium
- lncRNA:
Long noncoding RNA
- miRNA:
MicroRNA
- PDL:
Periodontal ligament
- mut:
Mutant
- NC:
Negative control
- PDLCs:
Periodontal ligament cells
- qPCR:
Quantitative polymerase chain reaction
- WT:
Wild type.
Data Availability
The data used to support the findings of this study are available from the corresponding author upon request.
Ethical Approval
This study protocol was approved by the Ethics Committee of Beihua University Affiliated Hospital.
Consent
Written informed consent was provided prior to the study.
Disclosure
This paper is already published in the preprint given in the link “https://www.researchsquare.com/article/rs-199858/v1”.
Conflicts of Interest
The authors declare no conflict of interest.
Authors' Contributions
XL and YZ designed the work and collected the data. XL did the experiments and conducted statistical analysis. XL contributed to writing the manuscript. Review and editing of the manuscript was done by YZ. The authors have read the approved the final manuscript.
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Associated Data
This section collects any data citations, data availability statements, or supplementary materials included in this article.
Data Availability Statement
The data used to support the findings of this study are available from the corresponding author upon request.