Dental development is a complex and reciprocal process between epithelial and mesenchymal, including tooth morphogenesis, hard tissue differentiation and mineralization, root formation and eruption. The neural crest ectomesenchyme gives rise to the cells that eventually form the tooth (1). Furthermore, neural crest-derived cells, Schwann cell precursors (SCPs) and Schwann cells (SCs) have been shown to maintain mesenchymal stem cell reservoir and participate in the tooth growth and development (2). SCs, as the major glial cell type of the peripheral nerve system (PNS), originate from the neural crest in a well-defined development step. Neural crest cells developed into SCPs and then converted into immature SCs (iSCs). iSCs differentiated into myelinated SCs (mSCs) and non-myelinated SCs (nmSCs) through the radial sorting (3). The phenotypic plasticity of SCs plays essential roles in the normal development of peripheral nerves and the response to nerve injury. It is commonly recognized that dental pulp tissue is densely packed with nerve fibers and requires a continuous supply of nerve cells. SCs, as one of the progenitor cells of dental-derived stem cells and major glial cell type of PNS (2), are believed to contribute to tooth development and injury repair. However, there are limited studies regarding the phenotypes and phenotype change of SCs during tooth development. The factors that affect the participation of SCs in pulp injury repair are also not fully understood.
Calcium, as an intracellular messenger, regulates cell growth, differentiation and apoptosis. L-type calcium channel (LTCC) is a transmembrane protein involved in several biological processes varying from neurogenesis (4), osteogenesis (5), and cardiomyogenesis (6). Our previous studies found that Cav1.2 was the primary type of LTCC expressed in the human dental pulp and plays a significant role in the odontogenic differentiation of dental pulp cells (7) and NG2+ pericytes (8). Cav1.2 is also found abundantly expressed in nerve fibers, SCs and astrocytes during the repair and regeneration of the pulp after tooth injury (9). Thus, we hypothesize that Cav1.2 also plays an essential role in SCs odontogenic differentiation and participates in the renewal of dentine after damage. Our previous study has successfully established the induction of SCs into odontoblasts
Therefore, the present study sought to clarify the phenotypes of SCs at different stages of tooth germ develop-ment. Furthermore, we investigated whether Cav1.2 functions in SCs odontogenic differentiation process
We extract the cellular RNA from the tooth germ cells of rats at different phases (E14.5, E16.5, E18.5, P1, and P7) using Trizol reagent (Invitrogen) to construct a cDNA library. The constriction of each cDNA library was implemented following the manufacturer’s suggestions, and next-generation sequencing was carried out using an Illumina HiSeq 2000 platform (IGA). RNA-seq analysis was conducted to identify and visualize the expression of differentially expressed genes (DEGs) involved in tooth germ development. Besides, we established the protein-protein interactions (PPIs) network by integrating protein information from the Search Tool for the Retrieval of Interacting Genes database (https://string-db.org/) to further explore the relationships among the DEGs at the protein level.
We chose 12-week-old Sprague-Dawley rats for the study. Rats were housed under a 12:12 light-dark cycle with free access to food and water. All procedures used in this study were conducted in accordance with the Animal Care Committee for the Care and Use of Laboratory Animals of Fudan University. The female mice were mated with male mice at a ratio of 2:1. Then we checked the progesterone plugs and regarded the noon that progesterone plugs appeared as embryonic development at 0.5 day. We select pregnant mice that 14.5 days, 16.5 days, and 18.5 days pregnancy (i.e., E14.5, E16.5, E18.5) and mice that 1 day, 7 days and 10 days postnatal (i.e., P1, P7, P10) as research objects. Pregnant SD rats in different periods were given intraperitoneal anesthesia (10% chloral hydrate, 0.5 mL/100 g). Then we checked the anesthesia effect 15 minutes later. After that, we opened the abdomen along the abdominal midline and exposed the uterus. We were lifting up the cervix of the uterus with forceps and exposing beaded fetal rats. Then we placed them gently on plates full of phosphate buffer saline (PBS). Afterwards, we washed them off and evacuated the placenta and tear membrane. Then we separated fetal rat heads, washed them off with PBS again and fixed them in 4% paraformaldehyde solution (PFA). SD rats at P1 were sacrificed, separated heads, washed off with PBS and fixed in 4% PFA. SD rats at P7 were sacrificed, separated heads and washed off with PBS. Then we removed the mandible integrally along the bilateral auriculotemporal region, washed them off and fixed them in 4% PFA for more than 48 hours. After that, we washed the mandible off with PBS many times, immersed them in 10% ethylene diamine tetraacetic acid (EDTA) which was 20 times the volume of the mandible and replaced the solution every two days. The mandible was decalcified until it was like rubber, elastic and easily through by pin. Then we washed off the separated heads of different periods in PFA and mandible in EDTA with flowing water for 4 hours, placed them in 75% ethanol overnight, dehydrated them the next day and embedded them in paraffin. Then these paraffin specimens were sectioned in the coronal plane and the slice thickness was 5 μm. All experiments were approved by the Ethical Review Committee of Fudan University (Shanghai, China) (approval no. JS-178).
SCs were seeded at a density of 5,000 cells/cm2 in 6-well plates and cultured overnight in Schwann cell medium (SCM; ScienCell) (Supplementary Methods). At about 60% confluence, SCM was replaced with odontogenic differentiation medium (ODM), which was consisted of α-minimal essential medium (HyClone), 10% FBS (ScienCell), 5 mmol/L glycerol-2-phosphate (Sigma-Aldrich), 10 nmol/L dexame-thasones (Sigma-Aldrich), 50 μg/mL ascorbic acid (Sigma-Aldrich), 100 U/mL penicillin (Sigma-Aldrich), 100 U/mL streptomycins (Sigma-Aldrich), with or without nimodipine (Bayer). All solutions were freshly prepared immediately before use. The medium was changed every 3 days.
SCs were cultured on the 24-well plates with a cell culture slide. After removing the medium, cells were washed with PBS and fixed with 4% paraformaldehyde. Subsequently, the slides were treated with 0.3% Triton X-100. The cells were blocked with 5% BSA. Specific primary antibodies targeting each marker (S100 [1:200; Abcam]; dentin sialoprotein [DSP, 1:50; Santa Cruz Biotechnology]; Cav1.2 [1:50; Santa Cruz Biotechnology]) were added at different concen-trations. The slides were incubated overnight at 4℃ and washed twice with PBS, then incubated with the secondary antibody (Alexa Fluor 594 AffiniPure goat anti-rabbit IgG, 1:200; Jackson ImmunoResearch) for 2 hours at room temperature (RT). After the nuclei were visualized by 4’,6-diamidino-2-phenylindole (DAPI, 1:1,000; Calbiochem), the slides were analyzed with a microscope (Eclipse 80i; Nikon).
Total RNA was extracted using TRIzol (Invitrogen) from the cells cultured in the SCM and ODM with or without nimodipine for 14 days. Approximately 2 μg total RNA was used to synthesize cDNA using the RevertAid First-strand cDNA Synthesis Kit (Thermo Scientific). Odontogenesis was evaluated in the SCs based on the expression of specific genes (
Alizarin Red S staining was used to examine calcium phosphate formation after 28 days of odontogenic differentiation. After removing ODM, the cells were gently washed with PBS and fixed with 4% paraformaldehyde for 15 minutes at RT, followed by washing with PBS and stained with a 0.2% Alizarin Red S (pH 4.2) (Sigma-Aldrich) for 30 minutes in the dark. Then excess dye was removed by repeated washing with PBS.
Induced model mice were given intraperitoneal anesthesia with 2% pentobarbital sodium (80 mg/kg) and ground right mandibular incisor for 2 mm with a high-speed air turbine drill. The left mandibular incisor was taken as a control group. We chose the right incisors at different time points after injury (0, 2, 6, 12, 24, 48, 72 hours, 5 days, and 1 week) for observation. We kept the mice warm and avoided hypothermia during the whole period.
Mice of the pulp injury model were allowed to survive for 0, 2, 6, 12, 24, 48, 72 hours, 5 days, and 1 week. After each survival period, mice were anesthetized with 2% pentobarbital sodium (80 mg/kg) and fixed by cardiac perfusion with 4% PFA. After that, mandibles with incisors were extracted completely, and excess soft tissue was removed. Then mandibles were further fixed in 4% PFA overnight. 24 hours later, mandibles were washed off with PBS and immersed in 10% EDTA which was 20 times the volume of the mandible. The decalcifying solution was changed every two days. The completion of the decalcification-mandible was elastic and easily through by pin-specimens were washed off with PBS and embedded in paraffin, sectioned in the coronal plane at a thickness of 5 μm.
Immunohistochemical and immunofluorescence staining used standard protocol on 5 μm coronal paraffin sections of the embryonic heads and mice mandibles. Primary antibodies were applied to the tissue and incubated at 4℃ overnight. Primary antibodies were MBP101 (1:150, ab62631; Abcam), S100β (1:200, ab52642; Abcam), growth-associated protein 43 (GAP43, 1:200, ab75810; Abcam), Ki67 (1:100, ab15580; Abcam), green fluores-cent protein (GFP, 1:200; Cell Signaling Technology), anti-Cav1.2 (1:200; Alomone Labs), CY3 (1:200; Abcam) and Dylight 488 (1:200; Abcam) secondary antibodies were used. And additional staining was done with DAPI (KeyGEN BioTECH). Dako solution was used to prevent quenching.
GraphPad Prism 7.0 software was used for all statistical analyses presented. Statistical significance was determined by using a one-way ANOVA. Each number was displayed as the mean±SD, and p<0.05 was considered statistically significant.
The examined embryonic and postnatal stages were E14.5, E16.5, E18.5, P1, and P7, representing the bud stage, cap stage, early bell stage, late bell stage and hard tissues formation stage, respectively. H&E staining results showed a significant morphological change as time went on (Supplementary Fig. S1). RNA-seq was constructed in different stages (E14.5, E16.5, E18.5, P1, and P7) of tooth germ development. DEGs associated with nervous system development were shown in Supplementary Data 1. Based on the PPIs network analysis, we found that genes related to the nervous system play an important role in the whole process of tooth germ development (Fig. 1A). Previous studies showed that SCs exist in different phenotypes, which have various molecular markers (Supplementary Table S2). We analyzed genes associated with SCs specific markers to validate the effect of SCs in tooth germ development. Results showed that they vary in the expression level in different developmental stages of tooth germs (Supplementary Table S3). Then we chose genes that existed in different phenotypes of SCs (specific markers) and carried out a PPI network analysis (Fig. 1B). The development of tooth germs may be significantly impacted by nerve growth factor, nerve growth factor receptor (also known as p75NTR), and cell adhesion molecules.
Among the genes primarily associated with cell proliferation, neuron growth and SCs development, we analyzed the expression of five marker genes, i.e., Mki67, GAP43, S100β, glial fibrillary acidic protein (GFAP) and myelin basic protein (MBP), which displayed dynamic expressions during various SCs development stages (Fig. 1C). Specifically, Mki67, a marker of proliferation Ki67, is linked to cell division (11); GAP43 is a neuronal growth-associated protein, highly expressed during the development and regeneration of nerves (12). S100β is a Ca2+-binding protein predominately found in astrocytes in the central nervous system (CNS) and SCs (13). It is present in all SCs stages except for SCPs (14). GFAP is uniquely found in astrocytes in the CNS, non-myelinating SCs in the PNS, and enteric glial cells. It emerges at a relatively late stage in SCs development, mainly expressed in iSCs during embryonic development and nmSCs after birth (15). MBP is mainly found in the oligodendrocytes in CNS and mSCs in the PNS (16, 17). Consequently, it may be reasonable to suggest that the expressions of S100β, GFAP, and GAP43 in the tooth germs were contributed by SCs.
The dynamic expressions of GAP43 indicated that the neuron growth activity reached its peak at E16.5 during tooth development within the tooth germs. The expression of Mki67 was considerably higher between E14.5 and P1, suggesting that a majority of cells in tooth germs may be in a proliferative state before P7. S100β, GFAP and GAP43 exhibited distinct expressions and trends, but they partially overlapped at various stages of tooth germ development (Fig. 1C). Given different phenotypic SCs possess diverse yet overlapping molecular markers (Supplementary Table S2), we postulate that the plasticity of SCs is present and may play a crucial role in tooth development.
Three specific markers (S100β, MBP101, and GAP43) were chosen to characterize SCs in tooth development. SCPs (S100β−/GAP43+/MBP101−), iSCs/nmSCs (S100β+/GAP43+/MBP101−) and mSCs (S100β+/GAP43−/MBP101+) were recognized from E14.5 to P7 during the rat tooth germ development.
On E14.5, the tooth germ of the rat mandibular first molar was in the bud stage (Supplementary Fig. S1A). Epithelial cells proliferated into ectomesenchyme in which cells also proliferated but did not differentiate, forming the tooth bud. S100β and GAP43 were expressed in ectomesenchyme, while MBP101 had weak expression in the mesenchyme (Fig. 2A, 2F). And the weak expression of Ki67 could be seen in every part of this stage (Supplementary Fig. S2A).
On E16.5, the tooth germ of the rat mandibular molar was in the cap stage (Supplementary Fig. S1B). Epithelial cells continued to proliferate, and the tooth bud changed to the shape of the cap and became an enamel organ. This period enamel organ consists of 3 layers of cells: outer enamel epithelium (OEE), inner enamel epithelium (IEE), and stellate reticulum (SR). Below the enamel organ, there was a cell coacervation area called dental papilla (DP), which would develop into dentin and pulp. The ectodermal mesenchymal cells surrounding the enamel organ and the edge of DP are densely packed into the connective tissue layer to form the dental follicle (also known as dental sac) (DF). And enamel knots began to form. S100 and GAP43 co-expressed in the OEE, IEE, mesenchyme, and DF throughout this time period. Strong expression was detected in the DP, while weak expression was seen in the dental lamina (DL) and SR. Furthermore, MBP101 was expressed weakly in mesenchyme at this time period (Fig. 2B, 2G). Ki67 expression was stronger than E14.5 (Supplementary Fig. S2B, S2C).
On E18.5, the enamel organ turned into the bell stage (Supplementary Fig. S1C). Ameloblasts and odontoblasts began to differentiate. There were 4 layers in the enamel organ, i.e., OEE, IEE, SR, and stratum intermedium (SI). The enamel organ continued to extend and enfolded DP. At this stage, the expressions of S100β and GAP43 were strong in DP and DF, but weak in IEE, OEE, and DL. And there was almost no expression of them in SR and SI. MBP101 expressed strongly in DP and DF, sporadically in SR, and almost none in the other part of the enamel organ (Fig. 2C, 2H). The signal of Ki67 was much greater than before (Supplementary Fig. S2D).
On P1, the tooth germ progressed to the late bell stage (Supplementary Fig. S1D). The enamel organ still consists of 4 layers of cells. IEE differentiated into ameloblasts, and DP cells near IEE became odontoblasts. Ameloblasts and odontoblasts secreted enamel and dentin matrices. And there was a little predentin formed. S100β and GAP43 had scattered expressions in DP but expressed strongly in SR. There was no expression in the other locations (Fig. 2D, Supplementary Fig. S3). MBP101 had a similar expression pattern to them (Fig. 2I). Besides, the expression of Ki67 achieved a peak at this stage (Supplementary Fig. S2E-S2H).
On P7, tooth germ was forming the hard tissue. Tooth roots began to form since P1. SR gradually disappeared, while SI still existed. Ameloblasts aggregated in IEE. Apparent enamel, dentin, and pulp formed (Supplementary Fig. S1E), and dentin thickened, and Hertwig epithelial root sheath formed on P10 (Supplementary Fig. S1F). During this period, the first molar was involved in the process of hard tissue formation (Fig. 2E, 2J). S100β and GAP43 are mostly expressed in the odontoblasts layer and co-expressed in the central and apical areas of the dental pulp (Fig. 2E, Supplementary Fig. S4). MBP101, on the other hand, is scattered in the dental pulp (Fig. 2J). Ki67 expression decreased in comparison to that in the early tooth germ development stage (Supplementary Fig. S5). The selected area in Supplementary Fig. S5A for observation was the odontoblasts of the pulp horn (Supplementary Fig. S5B), the central area of the pulp (Supplementary Fig. S5C), and the apical area (Supplementary Fig. S5D).
Briefly summary, the results showed that iSCs/nmSCs exist in ectomesenchyme, IEE, OEE, mesenchyme, DF, and most DP, whereas mSCs exist in mesenchyme. Developing into the bell stage, there are a large number of iSCs/nmSCs in DP and DF, but only small quantities in IEE, OEE and DL. And there was almost no existence in SR and SI. At the same time, mSCs exist most in DP and DF. Entering the late bell stage, a small number of iSCs/nmSCs and mSCs exist in DP, particularly in the odontoblast layer but a considerable number exist in SR. When the tooth germ is in the stage of hard tissue formation, iSCs/nmSCs are mostly found in the odontoblast layer and merely in the center of the dental pulp and the cusp. mSCs are scattered in the dental pulp. There was no obvious expression of SCPs found in the five time points studied in the present study.
The cultured cells appeared with a fusiform morphology and showed two neurites and a small cell body, positively expressing S100, a phenotypic marker of SCs. We also observed the positive Cav1.2 expression in SCs (Supplementary Fig. S6A). To examine the role of LTCC in the odontogenic differentiation of SCs, we used nimodipine to block LTCC. Different concentrations of nimodipine were added to SCM to determine its effect on the growing proliferation of SCs (Supplementary Methods). The cell proliferation curve showed that nimodipine had no significant effect on the proliferation of SCs compared with control during the first 5 days. After 7 days, high doses of nimodipine (2.5, 5, and 10 μM nimodipine) might gradually inhibit cellular proliferation. In contrast, 0.1 and 1 μM nimodipine had no significant effect on SCs growth (Supplementary Fig. S6B). Therefore, 1 μM nimodipine was used to inhibit LTCC during the odontogenic differentiation of SCs.
DSP, a specific marker of odontoblasts, was positive in both OD groups with or without nimodipine treatment after odontogenic differentiation for 14 days but negative in the control group (Fig. 3A). Real-time PCR results showed that the expression of
To examine whether SCs-derived cells could produce regenerative dentine after injury, we used PLP1-CreERT2/Rosa26-GFP mice to trace SCs and progeny (Supplementary Methods). According to the Jackson Laboratory instructions, we performed the mice genotype detection and got PLP1-CreERT2/Rosa26-GFP mice (Supplementary Fig. S7A), in which SCs and progeny were labelled by GFP after Tamoxifen induction. During the repair time, we observed that the mice’s left mandibular incisors length recovered to control length within one week after injury (Supplementary Fig. S7B). Therefore, we observed the changes in the expression of SCs and Cav1.2 in the pulp of mice after incisor injury within one week. The immunostaining results indicated almost no GFP+ cells (SCs and their progeny) in the cusp, middle and apex of control incisors, similar to that injured group (0 hour) without recovery. However, as the recovery time progressed, GFP+ cells increased gradually, and they were most visible at 48 and 72 hours after injury (Fig. 4A-4C) but weak at other time points (Fig. 4A-4C, Supplementary Fig. S7C-S7E). Notably, after 48 hours of recovery, some GFP+ cells migrated from the apex to the cusp of incisors and existed at the odontoblasts layer near the injured site at 5 days after injury (Fig. 4D), indicating that SCs could differentiate into odontoblasts to produce regenerative dentin after injury.
Cav1.2 channel expression was also investigated at the same time points following injury. In the tooth cusps, we observed a marked decrease in the Cav1.2 staining from 0 to 24 hours after injury compared to the non-injured control group. Starting from 48 hours after injury, its staining was enhanced gradually (Fig. 4A, Supplementary Fig. S7C). In the middle of tooth, Cav1.2 was almost absent from the odontoblast layer and pulp cells, however, the localization of Cav1.2 returned after injury and increased gradually, with the highest expression at 72 hours and then kept stable (Fig. 4B, Supplementary Fig. S7D). At the apex, there was a small amount of Cav1.2 expression in the control, 0 and 2 hours groups, but there was no significant difference among these three groups. By 6 hours after injury, Cav1.2 expression increased gradually, peaking at 72 hours and subsequently declined (Fig. 4C, Supplementary Fig. S7E).
The expression trends of SCs and Cav1.2 were similar. Both showed a notable strong staining pattern at 48 and 72 hours after injury. We also detected the co-staining of SCs (GFP+) and Cav1.2 (red). Regions of overlap were shown in yellow in the neurovascular bundle (Fig. 4E), indicating that Cav1.2 may be involved in the process of SCs participating in dentin regeneration after injury.
Neural crest cells are multipotent cells that contribute to generating most of the cell types for the peripheral nervous system (PNS) during the development (18). Besides giving origin to SCs, they are known to differentiate into dental mesenchymal stem cells (19). Moreover, perivascular cells (20) and SCs (2) have been identified as two distinct sources of dental mesenchymal stem cells. SCs could mai-ntain mesenchymal stem cell reservoir in the dental pulp and participate in tooth development, self-renewal and injury repair (2). All support that SCs are closely linked to tooth development and injury repair.
The nervous and oral systems are evidently close in anatomical location, organogenesis and disease development. For tooth eruption (21), elongation of the root, dentin formation and response to stimulations from surroundings (22, 23), an intact nerve supply is required. In this study, we found that the PNS-related genes are closely related to tooth germ development based on the PPI analysis. Furthermore, the expression of SCs-associated genes showed the existence of different phenotypes of SCs, emphasizing the importance of SCs in tooth development. The whole process of SCs development involves SCPs, iSCs and mature SCs which are classified as mSCs and nmSCs. iSCs differentiate to pro-myelinating SCs that build a one-to-one relationship with large-caliber axons and finally transform into mature mSCs (24). In contrast, some nmSCs stay in contact with groups of small caliber axons and form so-called Remak bundles. Their morphology and antigenic marker expression, are similar to that of iSCs during development primarily (25). The development of SCs goes through different phenotypes that are adapted to support the balance between proliferation and differentiation (26).
From the beginning of tooth germ formation, iSCs/nmSCs exist in the ectoderm mesenchyme and gradually migrate into the enamel organ and DP, most obvious in the papilla. The results show that SCs may be involved in the neurodevelopment of tooth germs. SCs are mainly distributed in DP and SR in the late bell stage. Studies have shown that in the area where the ameloblasts are polarized in the enamel organ, capillaries are distributed in three regions: penetrate the outer epithelial layer of the enamel, cross and diverge with the SR layer and a large number of branches and anastomosis with SI (27). Due to the distribution of capillaries in SR and a large number of SCs existing in this period, it is speculated that SCs in SR may be the basis of the dental pulp nerve. During the entire tooth germ development process, SCs primarily exist in the phenotype of iSCs/nmSCs. This phenotype is a relatively stable and rapid proliferation phenotype (28), which may promote the further development of the tooth germ. Studies have found that although the proliferation rate of SCs precursors is very high, the maximum proliferation rate occurs in iSCs, which have similar performance in rats and mice (28, 29). We thus speculate that is the reason why most SCs exist as iSCs/nmSCs, mainly in the tooth development process. Furthermore, it has been reported that SCs were one of the sources of stem cells (2), which, in conjunction with our findings, implies that iSCs/nmSCs may be the primary phenotype when combined with our findings.
Cav1.2 is closely related to the tooth formation and osteogenesis. Our previous studies proved that knockdown of Cav1.2 could inhibit the odontogenic differentiation of DPSCs (7) and the mineralization of rat DP stem cells (30). The results in the present study confirmed that SCs could differentiate into odontoblasts
Not contradicting, in the later stage of odontogenic differentiation, the formation of mineralized nodules in the nimodipine-treated group was reduced. It is reasonable that the mineralization of the extracellular matrix (ECM) of dentin requires the odontoblasts to efficiently transfer calcium into the ECM (38). However, the continuous treatment of nimodipine blocked the LTCC pathway, interfering with calcium transport and reducing calcium nodule formation, as observed in our study and previous studies (7). Taken together, calcium may play different roles in different cells and various stages of cell differen-tiation. The specific role of calcium in the odontogenic differentiation of different cells is worth further study.
We used the PLP1-CreERT2/Rosa26-GFP tracing mice as the injury model and found that SCs participated in the dentine regeneration after damage, consistent with the results of Kaukua et al. (2). GFP+ cells were almost absent in the control group, but GFP+ cells gradually increased after injury. At 72 hours after injury, their expression was most apparent. They tended to the odontoblast layer near the injured site, showing that SCs of mice incisors’ apex migrated from the deep pulp tissue to the odontoblast layer at the cusp injured site, which demonstrated that SCs proliferated, migrated, and differentiated into odontoblasts, and participated in the formation of the regenerative dentine.
Previous studies have confirmed that Cav1.2 presents temporal and spatial expression characteristics in dental pulp after injury, and it also plays an important role in the repair process of dental pulp injury (8, 9). To further study the role of Cav1.2 in the repair process of SCs after the dental pulp injury
In summary, SCs, as a part of PNS, play an essential role in tooth germ development. SCs have different phenotypes in different stages of tooth germ development. These phenotypes are coordinated in the whole process to ensure tooth development. Furthermore, SCs could be differentiated into odontoblasts
Supplementary data including one supplementary data, three tables, seven figures, and supplementary methods can be found with this article online at https://doi.org/10.15283/ijsc23205
There is no potential conflict of interest to declare.
Conceptualization: JH, TW, YJ, SZ. Data curation: JH, TW, DL, JY, YH. Formal analysis: JH, TW. Funding acquisition: YJ, SZ. Methodology: JH, TW. Project administration: YJ, SZ. Resources: YJ, SZ. Software: JH, TW, YJ. Supervision: YJ, SZ. Validation: YJ, SZ. Visualization: YJ, SZ. Writing – original draft: JH, TW. Writing – review and editing: JH, YJ, SZ.
This research was supported by the National Natural Science Foundation of China (grant numbers 82071109, 82301056).
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