Abstract
Objective
Adenosine triphosphate (ATP) is an essential nucleotide that is normally present in both intracellular and extracellular compartments. Extracellular ATP (eATP) has a pivotal role in both physiological and pathological processes of periodontal ligament tissues. Here, this review aimed to explore the various functions of eATP that are involved in the control of behaviours and functions of periodontal ligament cells.
Methods
To identify the included publications for review, the articles were searched in PubMed (MEDLINE) and SCOPUS with the keywords of adenosine triphosphate and periodontal ligament cells. Thirteen publications were used as the main publications for discussion in the present review.
Results
eATP has been implicated as a potent stimulator for inflammation initiation in periodontal tissues. It also plays a role in proliferation, differentiation, remodelling, and immunosuppressive functions of periodontal ligament cells. Yet, eATP has diverse functions in regulating periodontal tissue homeostasis and regeneration.
Conclusion
eATP may provide a new prospect for periodontal tissue healing as well as treatment of periodontal disease especially periodontitis. It may be utilized as a useful therapeutic tool for future periodontal regeneration therapy.
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Introduction
Periodontal ligament cells (PDLCs) possess stem cells that have similar mesenchymal stem cell characteristic features. PDLCs can be differentiated into different cell types like cementoblasts, fibroblasts, and osteoblasts [1, 2]. As PDLCs have the ability to balance between new cell formation by proliferation and cell death, PDLCs have a cell renewal capacity [3]. Therefore, PDLCs may be the main cell source and a promising target approach for periodontal regeneration therapy. But its utilisation alone has some limitations; some conditions, like inflammatory environments, change the characteristic features of resident periodontal ligament cells [2, 4, 5]. Growth factors and molecular activities are required to stimulate resident PDLCs for effective periodontal regeneration. Many factors like VEGF, FGF2, IL1β, and IL12 participate in different periodontal regeneration stages to synergise periodontal regeneration and the regenerative ability [6,7,8]. Despite many factors and molecules involved in the periodontal regeneration process, we targeted adenosine triphosphate and explored its effects on PDLCs functions for this review.
Adenosine triphosphate (ATP) is an essential nucleotide and is normally found intracellularly and extracellularly. Both forms of ATP are involved in the physiological as well as pathological processes of various cell types. The amount of ATP in the extracellular environment during physiological conditions is relatively low [9]. Some conditions like mechanical stress induced the release of ATP into the extracellular environment by PDLCs [10,11,12]. The released ATP has different functions, such as proliferation, differentiation, and inflammatory response on different cell types. eATP induces proliferation through PKC, PI3K/Akt, and MAPK signalling pathways in mouse embryonic stem cells [13]. It also acts as a danger signal by inducing the release of pro-inflammatory cytokines like IL1β in MG-5 microglial cells and IL6 in human thyrocytes [14, 15]. It has immunosuppressive action by stimulating IDO expression in the bone marrow mesenchymal stem cells (BMSCs) [16]. Different functions of PDLCs have been implicated in the periodontal regeneration process. However, the effects of eATP on the functions as well as behavior of PDLCs have not been extensively reviewed. This review aims to evaluate the various impacts of eATP on the functions and properties of PDLCs.
Methods
The articles were searched in PubMed (MEDLINE) and SCOPUS databases using keywords without published period limitation for this review. The keywords used for the search are [adenosine triphosphate AND periodontal ligament cells]. The authors examined and evaluated the title and abstracts of the articles for inclusion and exclusion criteria. The inclusion criteria were as follows; (1) full-text articles published in English or other language articles with available English abstracts, (2) articles demonstrating the effect of extracellular adenosine triphosphate related to functions of PDLCs, including inflammation, differentiation, immunomodulatory functions, and other functions of PDLCs. The exclusion criteria were (1) any study published in other languages, (2) articles related to the effect of adenosine triphosphate on other cell types rather than PDLCs (3) the study evaluating the effect of intracellular adenosine triphosphate.
Results
37 original articles were found in search of the databases by using the described search procedure. According to inclusion and exclusion criteria, 7 non-English studies were removed, and we removed another 17 studies that are not related to extracellular adenosine triphosphate and functions of PDLCs. Final 13 studies were used for this review. We used Preferred Reporting Items for Systematic Reviews and Meta Analyses (PRISMA) for the selection of literature for this review. The flow of information through the different steps involved in the selection of studies for this review (PRISMA) is shown in Fig.1.
Periodontal ligament cells (PDLCs)
The periodontal ligament is one of the tooth’s supporting tissues and is involved in the periodontium together with the cementum and alveolar bone. It is a fibrous tissue rich in vascular supply and connects the tooth cementum on one side and the alveolar bone on either side. As it is a tooth-supporting tissue, it plays a crucial role in maintaining tooth stability and tuning biological functions. One of the periodontal ligament’s major functions is maintaining periodontium homeostasis; for instance, it controls physiologic mechanical force during the masticatory function by transferring force to other supporting tissues of the tooth. The periodontal ligament can also play a key role in periodontal regeneration because it constitutes multiple cell types, such as cementum-forming cells (cementoblasts), bone-forming cells (osteoblasts), nerve cells, fibroblasts, and vascular endothelial cells. Thereby, the periodontal ligament becomes a major cell source for maintaining periodontal tissue homeostasis and regeneration [1, 17]. Periodontal ligament cells (PDLCs) are present in periodontal ligament tissues, which are in periodontal ligament space. PDLCs own stem cells (progenitor cells) and have similar mesenchymal stem cell characteristics and features. They have multiple lineage differentiation abilities that can be transformed into cementoblasts, fibroblasts, osteoblasts, and adipose cells [1, 2, 18, 19]. Beside mesodermal lineages, stem cells isolated from periodontal ligaments can also differentiate into ectodermal and endodermal lineages [20, 21]. PDL fibroblasts are capable of renewal of cells that can be adjusted between new cell formation by proliferation and number of cell loss through cell death and cell migration [3].
Periodontal regeneration
The periodontal tissue regeneration process includes three consecutive phases: inflammation, proliferation, and remodelling. It is similar to other tissue healing processes [22]. However, some pathological and immunocompromised conditions like periodontitis imbalance the normal regeneration process that causes excessive and prolonged inflammatory phase, lack or delayed cell proliferation, and repairing phase leading to periodontal tissue destruction [23]. The final goal of periodontal regeneration is to form new functional periodontal tissue in place of the damaged periodontal tissue [24]. PDLCs may be the main cell source for periodontal regeneration by reason of their similar mesenchymal stem cell features like multilineage differentiation, proliferation, and self-renewal ability. In particular, PDLCs are easily accessible and expanded ex vivo [25]. Nevertheless, PDLCs could be used as a prioritized approach for regenerative treatment in various periodontal diseases. The success of regenerative treatment using PDLCs alone is very restricted because of some restrained conditions such as inflammatory conditions of host PDLCs [2, 4, 5]. Therefore, periodontal therapy needs other factors besides PDLC therapy for effective periodontal regeneration. Additional molecular activities are needed for the periodontal regeneration process by regulating in stages of the regeneration process; some molecules participate in cell proliferation, some in differentiation, some in control of the immune response, and some regulate the release of inflammatory mediators by PDLCs.
As a result of previous studies (as shown in Table 1), many factors participated in the stages of regeneration, in particular inflammation, immunoregulation, proliferation, differentiation, and maturation. Consequently, PDLCs possess stemness, proliferative, immunomodulatory, and differentiation properties; other factors boost the regenerative ability of PDLCs. Among many factors involved in the periodontal regeneration process, we emphasized the role of adenosine triphosphate in the functions of PDLCs in this review.
Adenosine triphosphate (ATP)
ATP is an essential nucleotide that is built up of a purine base (adenine), pentose sugar (ribose) and 3 phosphate groups. Adenine is attached to the carbon atom at 1’place, and 3 phosphate groups are attached at the 5’ place of ribose. The 3 phosphate groups which are attached to the carbon atom at 1’ place, are linked to ATP by high energy bonds. ATP is normally found in both intracellular and extracellular compartments. Intracellular ATP (iATP) functions as the intracellular energy source of the cells. eATP acts as an essential extracellular messenger [9]. Both iATP and eATP take part in physiologic and pathological conditions, involving different functions like inflammatory process, healing process, and immune responses of various cell types.
Functions of intracellular ATP (iATP)
iATP usage promotes skin wound healing resulting in granulation tissue formation, re-epithelialization, and increased VEGF release [26]. iATP promotes wound healing of rabbits’ skin. It attracts the macrophage and inflammatory cells to the wound site and actuates the release of inflammatory cytokines: IL1β and TNFα, along with increases in VEGF expression, without the formation of hypertrophic scar in skin wounds of rabbits. Still, this study has limitations, and the detailed mechanism of the healing process may be specific to the species [27]. Mg-ATP encapsulated lipid vesicles treated at to wound site cause rapid granulation tissue regeneration, and new growth starts in less than 1 day [28]. These previous studies indicate the role of iATP in the wound healing process.
Functions of extracellular ATP (eATP) and its receptors
The amount of eATP is relatively low (400–100 nM) under physiologic conditions [9]. Many situations like mechanical stress, hypoxia, and inflammation cause the release of ATP into the extracellular compartment by various cell types such as PDLCs, cardiomyocytes, and endothelial cells [11, 12, 29, 30]. eATP has different functions, but it depends on various factors like cell types and types of activated receptors [31]. It acts as a danger signal called Danger-Associated-Molecular-Pattern Molecule (DAMP). It binds and activates the purinergic receptors on the cell surfaces, then initiates the inflammatory signal cascade and regulates the immune response [32, 33]. As the released ATP cannot be entered into the cell membrane easily to precede intracellular signalling events, it would rather interact with purinergic P2 receptors on the cell surface.
Purinergic P2 receptors are usually related to ATP. It has 2 subtypes according to signaling properties: metabotropic P2Y receptors (P2YRs) and inotropic P2X receptors (P2XRs). P2Y receptors (P2YRs) are classical G-protein-coupled receptors expressed in mammalian cells are eight subtypes (P2Y1, P2Y2, P2Y4, P2Y6, P2Y11, P2Y12, P2Y13, P2Y14). P2Y receptors are activated by ATP, ADP, UTP, UDP, UDP glucose, and NAD (nicotinamide adenine dinucleotide). The intracellular signaling event of P2Y1, P2Y2, P2Y4, P2Y6, and P2Y11 is related to PLC-IP3R signaling pathway resulting in increased intracellular Ca2+ level. P2Y12, P2Y13, P2Y14 receptors are mediated by AC-cAMP signaling pathway; ATP binds to these receptors leading to the inhibition of adenylyl cyclase (AC) and decreased intracellular cAMP levels [34, 35]. P2X receptors (P2XRs) are nucleotide-gated ion channel receptors with seven subtypes (P2X1, P2X2, P2X3, P2X4, P2X5, P2X6, P2X7) when ligand (nucleotide) gated ion channels P2X receptors are activated by ATP. These are homo/hetero-trimers, eATP binds to receptors, ion channels opened, K+ efflux and an influx of Ca2+ and Na+ occur resulting in increased intracellular calcium and membrane depolarization [36, 37].
eATP gives different functions to different cell types; one of the dependent factors is the types of purinergic receptors. Different receptor activation by ATP influences many cell functions including proliferation, inflammation, immune response, and others. eATP is involved in the suppression of endometrial stem cell proliferation and migration [38]. eATP-P2Y1 receptor activation reduces the proliferation of BMSCs [39]. On the other hand, eATP could induce mouse embryonic stem cell proliferation through PKC, PI3K/Akt, and MAPK signaling pathways. Therefore, eATP has different effects on cell proliferation in different environments through various signaling [13].
eATP plays a significant role in the control of inflammation of different cell types through diverse P2 receptor interactions. In MG-5 microglial cell lines, eATP induces the maturation and release of IL1β by enhancing IL1β converting enzyme/ caspase [14]. eATP also stimulates other pro-inflammatory cytokine IL6 release in human thyrocytes that plays role in the control of thyroid function. eATP dose-dependently induced IL6 release through P2Y receptor in human thyrocytes [15]. ATP can also induce anti-inflammatory cytokine IL10 expression and this induction is related to the crosstalk between P2Y1 and P2Y11 receptor activation in microglial cells. However, this induction effect is also dependent on intracellular Ca2+ release or the cAMP-activated PKA pathway [40]. In human blood cells, eATP-P2Y11 interaction maintains the balance of inflammatory mechanism by increasing IL10 and decreasing TNFα [41]. P2X7 receptor activation induces TNFα release by LPS-induced microglial cells of rat [42]. This receptor activation also induces inflammation by different mechanisms in different cell types; upregulates IL1β expression by stimulating NALP3 inflammasome and caspase 1 in P.gingivalis induced gingival epithelial cells [43], promotes IL6 expression by LPS pretreated primary human skin fibroblasts [44]. Another P2X receptor (P2X5) activation induces inflammasomes and IL1β secretion in murine osteoclasts [45].
Activation of P2Y2 and P2Y4 receptors by ATP regulates tumor growth and progression by inducing transcription factors, ERK1/2, p38 and JNK1 phosphorylation in MCF-7 cells [46]. eATP is involved in the regulation of human gingival tissue destruction by inhibiting IL1-induced matrix metalloproteinases (MMPs) expression via CD39 expression [47]. ATP-dependent P2X3 receptor activation increases endometrial pain by inducing neurogenic inflammation [48].
Various P2 receptors activation by ATP imparts in an immune response. eATP plays a regulatory role in the immune response by adjusting specific CD4+ T cells response by activation of different P2 receptors. 250 nM ATP upregulates the survival and proliferation of T lymphocytes by increasing the secretion of IL2. A higher dose 1 mM of eATP enhances apoptosis and inhibits activated CD4+ T cells functions through P2X7 receptor activation and enhances the proliferation of regulatory T cells by activation of P2Y2 receptors. Hence, the effect of eATP on specific CD4+ T cells response depends on the concentration of nucleotide [49]. eATP supports the immunoregulatory mechanism of dendritic cells. It inhibits Th1 cytokine IL12 and stimulates Th2 cytokines IL10. It also provides immunosuppressive action by inducing IDO expression through P2Y11 receptor in monocyte-derived dendritic cells primed with IFNγ [50]. ATP-P2 receptor activation has the full ability of immunosuppression by activating naïve T reg cells [51]. P2X7 receptor activation by 1000 μM eATP induces immunomodulatory cytokine IFNγ release in Japanese flounder head kidney cells [52]. eATP is involved in the immunosuppressive function of BMSCs primed with IFNγ by downregulating IDO expression via P2X7 receptor activation [16]. In conclusion, eATP has diverse functions of different cell subsets through various P2 receptors. Different functions of ATP that depend on various cell types and different receptor activation are described in Table 2.
As stated in Table 2, eATP has diverse effects on various functions according to different receptor activation and cell types. PDLCs have different types of purinergic receptors on the cell surface. Many previous studies proved that eATP and P2 receptor signalling had different functions on PDLCs.
Roles of eATP in various functions of PDLCs
eATP has numerous effects on the functions of PDLCs. It depends on different receptor interactions. One or more subtypes of purinergic P2 receptors are found on all types of cells. Previous study’s result clarified P2X7, P2Y1, P2Y2, P2Y4, P2Y6 and P2Y12 receptors expression has been detected in the periodontal ligament cells, that was detected in the 9 days cultured conditions [53]. As ATP can bind to various P2 receptors, the interaction of eATP and P2 receptor signalling had different functions on PDLCs, including proliferative function, inflammatory response, immunosuppressive function, osteogenesis, bone destructive function, and other various functions. One receptor can involve in different mechanism of PDLCs’ functions, sometimes more than one receptor is involved in each function. Different roles of eATP affect the numerous functions of PDLCs through different signalling, as shown in Table 3.
Effects of eATP on the proliferation of PDLCs
eATP modulates the proliferation of different cell types through specific purinergic receptors. Extracellular ATP and slowly hydrolyzable ATP (ATPγS) suppress the PDLCs proliferation but not the same mechanism. ATP induced PDLCs growth arrest by increasing p21WAF1/cip1 that regulates cell proliferation by inhibiting the cell cycle through the cyclin kinase pathway. Extracellular ATPγS induced cellular apoptotic responses. Ectonucleotidases including CD39 which are present in serum rescued the suppressive effect of PDLCs proliferation by ATP and ATPγS [54].
Effects of eATP on the inflammatory function of PDLCs
Mechanical stress induced the release of ATP by PDLCs. The released ATP activates specific purinergic P2 receptors on the cell surface and has been shown to regulate the trigger of pro-inflammatory cytokines/ chemokines. ATP induces the maturation or the release of pro-inflammatory cytokines /chemokines by PDLSCs. P2X7 receptor agonist (BzATP) enhanced the release of IL8 and CCL20 without influencing cell viability. Specific P2X7 receptor irreversible inhibitor, oxidized ATP (oATP) or A-74003 counteracted the eATP-induced IL8 and CCL 20 release. This inductive effect is followed by an increase in intracellular Ca2+ signalling. Generally, these results suggested that mechanical stress induced pro-inflammatory chemokines IL8 and CCL20 release by PDLSCs through eATP-P2X7 receptor interaction [55].
Mechanical stress is also involved in the maintenance of periodontium homeostasis by controlling the major pro-inflammatory mediator IL1β processing and release by PDLCs. Continuous compressive loading upregulated IL1β expression through the release of ATP in PDLCs. IL1β expression was markedly inhibited by a P2X7 receptor inhibitor or siRNA targeting the P2X7 receptor. As the P2X7 receptor is an ion channel receptor mostly permeable to calcium, intracellular calcium inhibitors markedly inhibited eATP-induced IL1β expression. According to this result, eATP-P2X7 receptor signalling and intracellular calcium signalling mechanisms are importantly imparted in mechanical stress-induced PDLCs inflammation through induction of pro-inflammatory cytokine, IL1 β production [12]. In next to the latter study, the role of pannexin1 (Panx1) in ATP-induced IL1 β expression in PDLCs was examined. The release of ATP is decreased by using a Panx1 inhibitor. Blocking Panx 1 also inhibited the release of IL1β which was induced by mechanical stress or ATP. Vesicular trafficking inhibitors reduced the release of IL1β by stimulated cells. Therefore, Panx-1 is contributed to the release of ATP and also to the release of IL1β induced by mechanical stress or ATP treatment [56].
Effects of eATP and immunomodulatory function of PDLCs
The immunomodulatory function of PDLCs is very important in host immune responses by suppressing inflammation, initiating the repairing process, and getting efficient regeneration. eATP stimulates the immunomodulatory function of PDLCs by promoting immunomodulatory molecules IDO and IFNγ release. Inhibition of P2X7 receptor by using chemical P2X7 antagonists; BBG and KN62, siRNA targeting P2X7 receptor, calcium chelator (EGTA), and PKC inhibitor significantly reduced eATP-induced IDO and IFNγ expression. Specific P2X7 receptor agonists (BzATP) dramatically induced eATP induced these two molecules’ expression. Hence P2X7receptor activation and intracellular calcium signalling are related to an immunomodulatory property of PDLCs. The eATP takes part in the immunosuppressive action of PDLCs [57].
Effects of eATP on osteogenic differentiation of PDLCs
One of the major functions of PDLCs is the differentiation function. eATP has also a key role in the maintenance of osteogenic differentiation of PDLCs. ATP-P2X7 receptor interaction decreases osteogenesis on inflammatory mediated PDLSCs through the PI3k-Akt-mTOR signalling pathway [58]. ATP enhances the osteogenic potential of PDLSCs by enhancing osteogenic genes Runx2 and OCN expression after 1 week of ATP treatment in an osteogenic medium. ATP treatment also demonstrated a highly expressed P2X7 receptor in PDLSCs. Moreover, ATP activates the P2X7 receptor, enhancing the PDLSCs osteogenesis [59]. PDLCs can differentiate into osteoblastic cells under cyclic tensile force. Continuous cyclic tensile force applied for 6 h stimulated osteogenic protein BMP9 synthesis and induced mineralization of PDLCs within 14 days of mineralization. Loss of function and overexpression experiments using suramin (a broad-spectrum P2Y antagonist), specific P2Y1 antagonist (MRS2179), or specific P2Y1 receptor agonist revealed the involvement of P2Y1 receptor in the induction of BMP9 synthesis. Experiments using U‐73122 (a phospholipase C [PLC] inhibitor), and thapsigargin (enhancer of intracytosolic calcium) also suggested the synthesis of BMP9 is related to an increased level of intracellular Ca2+ through the PLC pathway. These results indicated that eATP-P2Y1 signalling participated in CTF-induced BMP9 synthesis and in vitro mineralization [60]. Compressive including intermittent compressive force (ICF) and continuous compressive force (CCF) significantly increased extracellular ATP levels and ICF involved in the upregulation of osteogenic gene osterix expression through transforming growth factor β pathway. However, exogenous ATP treatment did not show an effect on the osteogenic differentiation of PDLCs [10].
Effects of eATP on the bone-destructive function of PDLCs
Mechanical stress induced the release of ATP by PDLCS and also promotes osteopontin (OPN) expression in PDLCs via the Rho kinase pathway. Osteopontin is the protein involved in bone destruction. Mechanical stress-induced ATP upregulates OPN which is mediated by the P2Y1-Rho kinase signalling pathway. Therefore, stress-induced ATP plays part in alveolar bone destruction [61]. In another study, mechanical stress-induced ATP increased bone-destructive protein RANKL expression. Upregulation of RANKL expression was mediated by the same P2Y1 receptor activation but through a different pathway. Indomethacin (an inhibitor of COX), H89 (cAMP-dependent protein kinase inhibitor) and pyrrolidine dithiocarbamate (NFκB inhibitor) inhibited RANKL expression, PGE2 production and NFκB translocation. Thus, eATP participates in the maintenance of bone homeostasis mediated by the P2Y1-NFκB-COX-RANKL axis in the periodontal tissue [62]. Therefore, eATP is related to bone homeostasis function by inducing different bone-destructive protein expressions through different signalling pathways.
Effects of eATP on PDL repair
PDLCs are mechanosensitive cells, receiving mechanical stress from dental occlusion or orthodontic tooth movement. Mechanical stress like centrifuge-mediated gravity loading increased ATP in the extracellular environment and extracellular signal-regulated kinases (ERK) phosphorylation in PDLCs. ERK phosphorylation imparts in the remodelling of periodontal tissues. Gravity loading induced ATP release and ERK phosphorylation in PDLCs which in turn would enhance the growth and survival of PDLCs. Stress-induced-ATP is involved in the stimulation of periodontal tissue remodelling via the P2Y receptor especially P2Y4 and P2Y6 during orthodontic tooth movement [63].
Effects of eATP on other functions of PDLCs
Continuous compressive stress causes the induction of ATP release by PDLCs. The mechanism of ATP release is dependent on the opening of hemichannel protein especially connexin 43. Also, this mechanism is regulated by the intracellular Ca2+ signalling pathway. Nevertheless, hemichannel gap junction proteins play important role in the function and behaviour of the PDLCs [11].
PDLCs respond to orthodontic tooth movement-related nociceptive pain by releasing ATP. Vesicular nucleotide transporter (VNUT) takes part in the uptake of ATP into secretory vesicles and this ATP binds to P2X3 receptor on trigerminal nerve resulting in tooth movement-induced pain. VNUT inhibitors (clodronic acid) suppressed the release of ATP induced by mechanical stimulation. Systemic administration of clodronic acid inhibited face-grooming behaviour (an indicator of nociception) followed by 1 day of experimental tooth movement. Moreover, ATP could regulate nociceptive pain control related to orthodontic tooth movement [64].
Discussion And conclusion
Many previous studies proved that eATP has a variety of effects on the functions of different cell types. ATP acts as an intracellular source of energy as well as involved in various intracellular signalling events. Different cell types including PDLCs could release ATP into the extracellular environment in response to mechanical stimuli and inflammatory conditions, and the released ATP has a possibility to take part in different PDLCs’ functions. The released ATP by PDLCs acts as a danger signal that stimulates inflammatory reactions, interestingly it also involves in the immunosuppressive action of PDLCs suggesting its biphasic effects on the bone remodeling of PDLCs. Nevertheless, PDLCs are one of the key players in the homeostasis of the periodontium and PDLCs have various kinds of functions. The role of eATP on PDLCs’ functions and the detailed mechanism is lesser compared to other cell types, so many further studies are required to assess the effect of eATP on different PDLCs’ functions such as angiogenesis, differentiation, and their detailed mechanism that help to get future successful periodontal regeneration therapy.
The periodontal regeneration is a complicated process, and the final goal of periodontal regeneration is the removal of destructive tissue as well as the replacement of new functional structure. To fulfill this goal, PDLCs therapy is a priority for the regeneration but there are a lot of limitations; for example, inflammatory resident tissues that release inflammatory cytokines and change the regenerative ability of host tissue leading to poor prognosis of the cell treatment and failure. Therefore, adjunct strategies such as different growth factors, natural biomaterials are needed to induce cell homing, promote resident cell proliferation and differentiation, induce immunomodulation of host system, regulate cell signalling to get endogenous periodontal regeneration [65]. Nowadays, many studies found that different growth factors, signalling molecules, drugs used as adjuncts to conventional periodontal therapy. For example, local delivery of recombinant PDGF-BB using βTCP carrier promote periodontal wound healing by inducing the expression of ICTP, VEGF, PDGF [66]. Local application of recombinant FGF to infrabony defect improve alveolar bone growth [67]. Many growth factors and small molecules released by cells become target to improve regeneration process. According to the previous studies’ results, eATP may be a promising therapeutic tool for future periodontal regenerative therapy. The inductive and inhibition effect of eATP via different purinergic P2 receptor signaling may be applied in creating therapeutic material used as adjuncts for conventional periodontal therapy.
Taken together, eATP plays important role in the control of pro-inflammatory cytokine and chemokine release, inhibition of proliferation, stimulating immunosuppressive action as well as inhibiting or stimulating osteogenic differentiation of PDLCs through various purinergic P2 receptors and signalling pathways (Fig. 2). These findings improve the knowledge about the released nucleotide ATP support PDLCs to regulate periodontal tissue homeostasis and regeneration process. Understanding the role of eATP on PDLCs functions beneficially applied for the development of new adjunct strategies for the periodontal healing process. With the addition of new advancing technologies, eATP may be utilized as a therapeutic molecule to improve future periodontal regeneration therapy as an adjunct molecule after periodontal surgery to improve the healing process of periodontal defect or used after scaling to control the progress of the periodontal disease. However, further studies are needed to extend the insight of eATP on the periodontal regeneration process.
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Funding
This study was supported by the NSRF via the Program Management Unit for Human Resources & Institutional Development, Research and Innovation (B16F640118). MK was supported by the Ratchadapisek Sompote Fund for Postdoctoral Fellowship, Chulalongkorn University.
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MK, PL, TO contributed to conceptualization and methodology. MK and PL contributed to writing, original draft preparation, review, and editing. JM, WM, HE and TO contributed to review and editing. MK, PL and TO contributed to funding acquisition. All authors have read and agreed to the published version of the manuscript.
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Appendix
Appendix
Appendix 1 List of abbreviations
eATP | Extracellular adenosine triphosphate |
ATP | Adenosine triphosphate |
PDLCs | Periodontal ligament cells |
VEGF | Vascular Endothelial Growth Factor |
FGF2 | Fibroblast growth factor 2 |
IL | Interleukin |
PKC | Protein kinase C |
PI3K | Phosphatidylinositol 3-kinase |
Akt | Ak mouse strain transforming serine-threonine protein kinase |
MAPK | Mitogen activated protein kinase |
MG-5 | Microglial cell line 5 |
IDO | Indoleamine-pyrrole 2,3-dioxygenase |
BMSCs | Bone marrow mesenchymal stem cells |
PRISMA | Preferred Reporting Items for Systematic Reviews and Meta Analyses |
PDL | Periodontal ligament |
PDLSCs | Periodontal ligament stem cells |
rhBMP-2 | Recombinant bone morphogenetic protein-2 |
PDGF | Platelet-derived growth factor |
TGF-β1 | Transforming growth factor β1 |
LPS | Lipopolysaccharides |
IFNγ | Interferon-gamma |
HLA-G | Human leukocyte antigen G |
Poly I:C | polyinosinic-polycytidylic acid |
TLR3 | Toll like receptor 3 |
iATP | Intracellular adenosine triphosphate |
TNFα | Tumor necrosis factor alpha |
Mg | Magnesium |
DAMP | Danger-Associated- Molecular-Pattern Molecule |
P2 | Purinergic 2 receptor |
P2YRs | P2Y family of purinergic receptors |
P2YRs | P2X family of purinergic receptors |
ADP | Adenosine diphosphate |
AMP | Adenosine monophosphate |
UDP | Uridine diphosphate |
UTP | Uridine triphosphate |
NAD | Nicotinamide-adenine dinucleotide |
PLC | Phospholipase C |
IP3 | Inositol triphosphate |
AC | Adenylyl cyclase |
cAMP | Cyclic adenosine monophosphate |
K+ | Potassium |
Ca2+ | Calcium |
PKA | Protein kinase A |
NALP3 | NACHT, LRR and PYD domains-containing protein 3 |
P. gingivalis | Porphyromonas gingivalis |
ERK | Extracellular signal-regulated kinases |
p38 | 38-kDa protein |
JNK | c-Jun N-terminal kinase |
MCF-7 | Breast cancer cell line acronym for Michigan Cancer Foundation-7 |
MMPs | Matrix metalloproteinases |
CD | Cluster of differentiation |
CD39 | Ectonucleoside triphosphate diphosphohydrolase-1 |
CD4+ T cells | Helper T cells |
Treg | Regulatory T cells |
ATPγS | Slowly hydrolysable ATP |
BzATP | 2’(3’)-O-(4-Benzoylbenzoyl) adenosine-5’-triphosphate tri(triethylammonium) salt |
CCL20 | Chemokine (C-C motif) ligand 20 |
oATP | Oxidized adenosine triphosphate |
A-74003 | Artificial P2X7 receptor antagonist |
siRNA | Small interfering RNA |
Panx1 | Pannaxin-1 |
BBG | Brilliant Blue G |
KN62 | 4-[(2 S)-2-(N-Methylisoquinoline-5-sulfonamido)-3-oxo-3-(4-phenylpiperazin-1-yl) propyl] phenyl isoquinoline-5-sulfonate |
EGTA | Ethylene glycol-bis(2-aminoethylether)-N,N,N′,N′-tetraacetic acid |
mTOR | Mammalian target of rapamycin |
BMP9 | Bone morphogenetic protein 9 |
MRS2179 | Competitive antagonist at P2Y1 receptors |
U-73122 | Phospholipase C and 5-lipooxygenase inhibitor |
CTF | Cyclic tensile force |
ICF | Intermittent compressive force |
CCF | Continuous compressive force |
OPN | Osteopontin |
Rho | Ras homologous (Rho) protein |
RANKL | Receptor activator of nuclear factor-kappa B ligand |
COX | Cyclo-oxygenase |
H-89 | Potent and selective inhibitor of cyclic AMP-dependent protein kinase |
NFκB | Nuclear factor kappa B |
PGE2 | Prostaglandin E2 |
VNUT | Vesicular nucleotide transporter |
Runx2 | Runt related transcription factor 2 |
OCN | Osteocalcin |
βTCP | Beta tricalcium phosphate |
ICTP | pyridinoline cross- linked carboxyterminal telopeptide of Type I collagen |
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Kyawsoewin, M., Manokawinchoke, J., Namangkalakul, W. et al. Roles of extracellular adenosine triphosphate on the functions of periodontal ligament cells. BDJ Open 9, 28 (2023). https://doi.org/10.1038/s41405-023-00147-7
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DOI: https://doi.org/10.1038/s41405-023-00147-7