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In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

Here, we present a protocol for studying orthodontic tooth movement (OTM), serving as a suitable model for investigating the mechanisms of bone adaptation, root resorption, and the response of bone cells to mechanical stimuli. This comprehensive guide provides detailed information on the OTM model, micro-computed tomography acquisition, and subsequent analysis.

Abstract

Orthodontic tooth movement (OTM) represents a dynamic process in which the alveolar bone undergoes resorption at compression sites and deposition at tension sites, orchestrated by osteoclasts and osteoblasts, respectively. This mechanism serves as a valuable model for studying various aspects of bone adaptation, including root resorption and the cellular response to mechanical force stimuli. The protocol outlined here offers a straightforward approach to investigate OTM, establishing 0.35 N as the optimal force in a mouse model employing a nickel-titanium (NiTi) coil spring. Utilizing micro-computed tomography analysis, we quantified OTM by assessing the discrepancy in the linear distance at the cement-enamel junction. The evaluation also included an analysis of orthodontic-induced inflammatory root resorption, assessing parameters such as root mineral density and the percentage of root volume per total volume. This comprehensive protocol contributes to advancing our understanding of bone remodeling processes and enhancing the ability to develop effective orthodontic treatment strategies.

Introduction

Bone remodeling is an ongoing process orchestrated by osteoclasts, osteoblasts, bone lining cells, and osteocytes, essential for maintaining the integrity of the adult skeleton1,2. Primarily driven by the differentiation and activity of osteoclasts and osteoblasts, this dynamic process involves the resorption and deposition of bone, triggered by mechanical stress and loading3,4,5.

Animal experiments play a pivotal role in elucidating the intricate biological and cellular mechanisms underpinning orthodontic tooth movement (OTM)6,7. This process involves a diverse array of cell types, such as osteoblasts, osteoclasts, osteocytes, fibroblasts, and immune cells like macrophages and T cells, situated within the jawbone and periodontal ligament7,8. These cells dynamically respond to mechanical stimuli and changes in the local milieu, influencing the composition and architecture of the surrounding bone7,8. Moreover, they also trigger an inflammatory response at a cellular level, even though there are no pathogens present. This inflammatory response plays a role in increasing the turnover of bone tissue9.

Various animal models, including mice, rats, rabbits, dogs, and monkeys, have been utilized in experimental studies of OTM7,8,10. Among these, rodents, particularly mice, are favored for investigating the initial phases of tooth movement and bone remodeling6. Previous research has emphasized the advantages of using mouse models over rat models, primarily due to the widespread availability of genetically modified strains, enabling detailed exploration of genetic influences in OTM7,11. Currently, two main models are employed to induce tooth movement in mice. The first method entails inserting a nickel-titanium (NiTi) coil spring between the first upper molar and upper incisors4,12. The second approach involves placing an elastic band within the interdental space between the first and second upper molars13. The primary outcomes analyzed typically include the magnitude of the tooth movement and bone microarchitecture, preferably evaluated using micro-computed tomography (micro-CT)14. Ideally, assessing the integrity of dental roots is important to ensure that appropriate forces are employed to produce OTM4.

While micro-CT is widely acknowledged as the gold standard for evaluating the microarchitecture of mineralized tissues14, the absence of standardized methodologies and protocols for scanning, analyzing, and reporting data often presents challenges in discerning the precise procedures employed, interpreting results, and facilitating comparisons between different OTM models14,15.

Here, we present a step-by-step guide to the OTM mouse model, including micro-CT acquisition and analysis of OTM, bone microstructure, and dental roots. This method entails applying controlled mechanical force to the first molar to induce movement within the jawbone. The selection of this method stems from several factors, including feasibility, relevance, and precision. Such an approach enables detailed quantitative analysis, providing valuable insights into the biological processes underlying orthodontic tooth movement and facilitating the development of improved orthodontic treatment strategies in the future.

Protocol

All procedures strictly adhered to the ethical standards established by the Universidade Federal de Minas Gerais Ethics Committee (No. 166/2022). Before each experiment, a sample size calculation is mandatory. Use 8-10-week-old male C57BL6/J wild-type mice weighing approximately 20-30 g. The mice must be housed in a cage within a room maintained at 25 °C, adhering to a 12 h light/12 h dark cycle. Following coil attachment, the animal should be fed with a soft diet. Daily monitoring should include assessments of body weight and overall health.

1. Mechanically-induced alveolar bone remodeling

  1. Using distal cut pliers, cut the 0.25 x 0.76 inches NiTi open-coil spring to the following dimensions of six loops and two loop-shaped ends positioned perpendicular to the spring using orthodontic Weingart pliers.
  2. Shape the 0.20 mm diameter round chrome-nickel (CrNi) wire to the desired configuration with loop-shaped ends using Mathieu tweezers and a round-shaped instrument as a size reference.
  3. Put together the loop-shaped ends of the coil and the 0.20 mm round CrNi wire.
  4. Anesthetize the animal with an intraperitoneal injection of 0.2 mL of solution containing xylazine (10 mg/Kg) and ketamine (100 mg/Kg). Before starting the procedure, evaluate the depth of anesthesia using the pedal reflex. Carefully pinch one of the animal's toes using tweezers. The absence of a reflex indicates an adequate plane of general anesthesia. To avoid corneal injuries and post-operative pain, apply an ocular lubricant after the animal is anesthetized.
  5. Position the animal in dorsal decubitus on a surgical table, immobilizing its limbs to restrict movement and enable intraoral access.
  6. Utilize a mouth-opener, fashioned from 0.50 mm diameter wire and secured with a 0.08 mm wire, to facilitate full visualization while preventing head movement. Use the right side as the experimental side (OTM side) and the left side as the control without an orthodontic coil (Control side).
    NOTE: Enhanced visualization of intraoral structures must be achieved using a stereomicroscope and an optical light system.
  7. Clean and etch the right first molar and incisor surfaces using acetone and a self-etching primer, respectively. The system is self-etching, meaning it does not require prior acid conditioning.
    1. Apply the primer in a single step, which also functions simultaneously as an acid and an adhesive. Using a microbrush, collect a small amount of self-etching primer and apply it to the occlusal surface of the upper first molar and incisors. Care must be taken in this step to ensure that the self-etching primer does not reach the proximal surface between the first and second molars, as this could cause the dental elements to stick together, preventing tooth movement. Light cure the primer at the occlusal surface of the molars and incisors for 30 s.
  8. Bond the distal end of a six-loop NiTi open-coil spring to the occlusal surface of the right first maxillary molar with light-cured resin and light cure for 30 s. Add additional resin increment to the edge of the wire to avoid harm to the mice and light cure for 30 s.
  9. Activate the coil using a specifically designed apparatus consisting of a rail and crank mechanism attached to the surgical table. This enables longitudinal movement to slide back and forth.
  10. Connect the free loop-shaped end of the 0.20 mm round wire to the hook of the tension gauge.
  11. Upon activation of the crank, move the surgical table along the rail until the dynamometer registers a force of 0.35 N.
  12. Bond the 0.20 mm round wire to both upper incisors to anchor the coil. No further reactivation is performed during the experimental period. Cut the wire to detach the animal from the dynamometer.  Add another increment of resin so the metal edge of the device is not exposed and does not hurt the animal. Light cure for 30 s. Disassemble the animal from the table.
  13. The upper right first molar with a device imposing a force of 0.35 N in the mesial direction consists of the experimental side. Use the left side of the maxilla (without an orthodontic appliance) as a control4,16.
  14. Maintain this device for a period of 12 days without any activation being required. Do not use any pain control medication. Orthodontic movement occurs through an inflammatory process, and pain-relieving medication may negatively affect the arachidonic acid cascade, impacting the rate of bone remodeling and potentially invalidating the results.
  15. After the end of the surgery, treat the animals with a subcutaneous injection of saline solution to avoid dehydration during the adaptation period with the device. Keep the animal in an individual cage with heating until it is fully recovered and only after this period place the animal in collective cages.
  16. Euthanize the mouse on the 12th day performed by sedation with intraperitoneal injection of a 0.2 mL solution containing xylazine (10 mg/Kg) and ketamine (100 mg/Kg) followed by decapitation with sharp scissors.

2. Micro-CT measurements

  1. Harvest the maxillary bone with sharp scissors cutting all soft tissue, the zygomatic bone in the sagittal plane, and the frontonasal suture and the spheno-occipital synchondrosis in the coronal plane. Immerse the maxillary bone in 10% neutral buffered formalin (pH=7.4) for a fixation period of 48 h. After this period, change the formaldehyde solution to 70% alcohol.
  2. Perform micro-CT scanning of the maxillary bone with the following parameters for high-resolution scans: isotropic voxel size of 9 to 18 µm, X-ray settings of 50 kV, 0.5 mm aluminum filter, and rotation angle of 0.5°. More than one jaw can be fit during the microCT scanning.
  3. Reconstruct the acquired images using the microtomography reconstruction program indicated by the manufacturer of the micro-computed tomography (microCT) used17.
  4. Position the reconstructed images using the 3D Inspection program indicated by the manufacturer of the microtomography used.
  5. Quantify OTM by measuring the difference in linear distance between the cement-enamel junction (CEJ) of the first and second molars of the right hemi-maxilla (OTM side) relative to the left hemi-maxilla (control side). Utilize the proper microCT analyzer software with the line tool for this measurement17,18,19,20.
  6. Check the samples for the presence of orthodontic-induced inflammatory root resorption (OIIRR). Select the region of interest (ROI) of the disto-vestibular root of the first maxillary molar by using an irregular, anatomic region of interest drawn manually contouring method. Measure the following parameters: root mineral density (RMD; g/cm3) and percentage of root volume per total volume (RV/TV; %). Utilize the proper microCT analyzer software with the 3D volumetric tool for this measurement16,21.
  7. Conduct the reconstruction of the first maxillary molar using Mimics software and analyze the obtained data to draw conclusions regarding OTM and OIIRR in the experimental model16,21.

Results

This protocol enables the investigation of an OTM mouse model using a NiTi coil spring. With a force of 0.35 N applied, the mean CEJ distance on the control side between the first and second molars was 243.69 µm (Figure 1A, line A), whereas on the OTM side was measured at 284.66 µm (Figure 1A, line B). The difference between the OTM and control sides was 40.97 µm (Figure 1B). The linear distance betwe...

Discussion

Here, we describe a standardized protocol designed to elucidate the cellular and molecular mechanisms underlying bone remodeling during OTM. A thorough understanding of these mechanisms in mice requires a meticulously planned protocol to ensure accuracy and reliability7,11. Studies conducted by our research group have shown that this protocol effectively reduces operator variability by incorporating a tension gauge and a specially designed apparatus, establishing...

Disclosures

The authors have no conflicts of interest to declare.

Acknowledgements

We wish to express our sincere appreciation to Miss Beatriz M. Szawka for her contribution to the schematic diagram and to Mrs. Ilma Marçal de Souza for her technical support. J.A.A.A. is the recipient of a fellowship granted by Fundação Carlos Chagas Filho de Amparo à Pesquisa do Estado do Rio de Janeiro (FAPERJ, E-26/200.331/2024), Brazil. This study was supported by Conselho Nacional de Desenvolvimento Científico e Tecnológico (406928/2023-1), Fundação de Amparo a Pesquisa do Estado de Minas Gerais and Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (Finance code 001), Brazil. The authors thank Prof. Dr. Eduardo H. M. Nunes from LabBio/UFMG for the X-ray microtomography analysis.

Materials

NameCompanyCatalog NumberComments
AcetoneSigma-Aldrich67-64-1
Distal cut pliersQuinelatoQO.700.00
DynamometerSHIMPOFGE-5XY
Fiber Optic IlluminatorCole-ParmerN/A
ketamineSyntec100477-72-3
NiTi open-coil spring 0.25 x 0.76Lancer Orthodontics
Ø 0.20 mm round chrome-nickel (CrNi)Morelli55.01.208
Round CrNi Hard Elastic Orthodontic Wire Ø0.50 mm (.020 inch)Morelli55.01.050
Round CrNi Tie Wire Ø0.20 mm (.008 inch)Morelli55.01.208
StereomicroscopeQuimisQ7740SZ
Transbond Plus Self Etching Primer3MLE-Q100-1004-7
Weingart PlierQuinelatoQO.120.00
XylazineSyntec23076-35-9
MicroCT Analysis
Skyscan 1174v2Bruker1174v2
Software
NReconSkyscanN/A
DataViewerSkyscanN/A
CTAnSkyscanN/A
MimicsMaterialiseN/A

References

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Orthodontic Tooth MovementOTMAlveolar BoneResorptionDepositionOsteoclastsOsteoblastsBone AdaptationRoot ResorptionMechanical Force StimuliNickel titanium Coil SpringMicro computed TomographyInflammatory Root ResorptionRoot Mineral DensityBone RemodelingOrthodontic Treatment Strategies

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