Radiographic and immuno-histochemical evaluation of root perforation repair using MTA with or without platelet-rich fibrin or concentrated growth factors as an internal matrix in dog’s teeth: in vivo animal study

The Institutional Research Ethics Committee (REC), Faculty of Dentistry, Suez Canal University, Egypt, reviewed and approved this work (No.335/2021). All methods are reported in accordance with ARRIVE guidelines for the reporting of animal experiments (https://​www.​arriveguidelines​.​org).

Dogs were chosen for this study from the animal house at Suez Canal University’s Faculty of Veterinary Medicine. These dogs were used in this scientific purpose because they had already been requested and slated for euthanasia for veterinary reasons (e.g. behavioural issues, life-changing circumstances, convenience, overpopulation). Every attempt was made to reduce animal suffering and the quantity of used animals.

The oral cavity was disinfected with povidone-iodine (Betadine, 10%, Mundi Pharma, Cairo, Egypt). Rubber dam (TOR VM, Moscow, Russia) was used to isolate the teeth by applying the rubber dam clamp (butterfly #210 or # 202) + sheet first, followed by the rubber dam frame (Fig. S2). Additional seal with light-cured resin barrier (Opal Dam, Ultra Dent, South Jordan, USA) around the tooth neck (CEJ) was done. The crown and rubber dam sheet surface were disinfected with 30% hydrogen peroxide (H₂O₂, LUNA pharmaceutical, Cairo, Egypt), followed by 2.5% sodium hypochlorite (NaOCl, DEXA company for chemicals, Cairo, Egypt).

In all included teeth, a standard endodontic access cavity was performed with a sterile round, Endo-Z burs (Dentsply Maillfer, Ballaigues, Switzerland), and water cooling. Patency was tested with a #10 k-file (Micro Mega, Besancon, France). The working length was 1 mm from the apex using a Root ZX electronic apex locator (J Morita Corp, Tokyo, Japan). The canal orifice was opened and flared in an anti-curvature motion with Fanta blue rotary orifice opener files (#17/12, Fanta, TX, USA). Root canal instrumentation was done using Fanta blue files up to AF4 35/04. Irrigation of each root canal was done with 2 mL sodium hypochlorite 2.5% between each file use. A final rinse of 3 mL of saline 9% (Otsuka pharmaceutical, Shanghai, China) and 3 mL of EDTA 17% solution (Prevest Denpro Limited Company, Jammu, India) was performed after canal instrumentation. The canals were subsequently dried using paper points #35/04 (Dentsply, Tulsa, USA) and obturated using a single cone technique with gutta-percha (#35/04) (Dentsply, Tulsa, USA) and AH plus sealer (Dentsply, Konstanz, Germany).

In the teeth of contaminated perforation (subdivision 1) (n = 40) from the three experimental (MTA, MTA + PRF, MTA + CGF) and positive control groups, contaminated furcation perforations were created as follows: Each perforation was done at the floor of the pulp chamber (midway between mesial and distal canal orifices) using a high-speed long shank round bur # 4 (#4RC; SybronEndo Europe, Amersfoort, Netherlands) with coolant. The perforation width was standardised to 1.5 mm, and its length was extended to 2 mm in the alveolar bone [8]. Radiograph was taken to check the correct position and depth of furcation perforation. The access cavities and the created perforation sites were left without any coronal seal for 4 weeks to allow bacterial contamination from saliva in the mouth cavity to cause infection and inflammation. For pain and infection control, the dogs were given 10 mg/kg intramuscular cefotaxime sodium (Wockhardt UK Ltd, Wrexham, UK) and 1.1 mg/kg diclofenac sodium (Voltaren, Novartis Pharma, Basel, Switzerland) once a day for 5 days following surgery.

After 4 weeks, in contaminated perforations (subdivision 1), periapical radiographs were taken to confirm the presence of bone resorption and a lesion at the furcation area. While in non-contaminated perforations (subdivision 2), the temporary filling was removed, and an immediate furcation perforation was performed in the same manner as indicated in subdivision 1 but without oral contamination.

The access cavities and the perforations were flushed with 2.5% sodium hypochlorite, followed by 9% normal saline. Excavator was used to curet the perforation site to remove any inflammatory tissues or debris. The bleeding was stopped by washing the region with 9% sterile saline solution and applying pressure with wet cotton pellets [8, 17, 33, 34]. In the two subdivisions of the positive control group (group II), the experimental perforation was left without any perforation repair material.

Ten millilitres of autologous venous blood was collected from the cubital region of the dog’s forearm in a 10-mL sterile test tube without anticoagulant and immediately spun at 3000 rpm for 12 min in a table-top centrifuge. The final product had three layers: (a) RBC at the bottom, (b) PRF clot in the middle and (c) platelet-deficient plasma in the uppermost layers (PPP). The central clot’s platelet-rich fibrin (PRF) was carefully extracted with a tweezer.

As described in the PRF, but the autologous venous blood was centrifuged using a one-step centrifugation methodology (Medifuge, Silfradent, Sofia, Italy): 30-s acceleration, 2 min 2700 rpm, 4 min 2400 rpm, 4 min 2700 rpm, 3 min 3000 rpm, 36-s deceleration and stop. Below the dividing line, the ensuing intermediate layer comprising CGF was taken.

Pieces of PRF and CGF with average standardised size of 1.5 × 2 mm were packed, respectively, in groups MTA + PRF (IV) and MTA + CGF (V) into their corresponding interradicular area (bone and periodontal defects) by using hand pluggers to the level of cementoenamel junction (CEJ). After that, a 3-mm MTA plug was packed over the platelet concentrates matrix. The access cavity in all groups was definitively sealed with glass ionomer filling (Medifill: Promedica, Neumunster, Germany). After doing different treatment modalities for perforation repair, periapical radiographs were taken immediately for all teeth using a digital sensor (EzSensor Classic, Vatech, Gyeonggi-do Korea). A Rinn (XCP) sensor holder (Rinn, Dentsply Sirona, Charlotte, USA) was employed to achieve image consistency for the immediate postoperative and follow-up radiographic fields. A small individual occlusal stent was fabricated from acrylic resin (Duralay, Reliance, Alsip, USA) to be used for setting the sensor at a standard angulation in relation to the teeth [39]. Images were captured using an X-ray imaging system (Fischer, Sindelfingen, Germany).

Radiographs for all groups and subgroups were saved as a baseline for later comparison after the follow-up period. Dogs were housed in the animal home at Suez Canal University’s Faculty of Veterinary Medicine for three months, providing follow-up care as described previously [11].

After 3 months, the dogs were euthanised with an intravenous barbiturate overdose of 6% pentobarbital (120 mg/kg, Nembutal, Akorn, Lake Forest, USA) [8, 40].

The intra-observer agreement for the radiographic, histologic and immunohistochemical observations was calculated using kappa coefficient. Level of agreement was suggested according to the kappa results as follows: values ≤ 0 as indicating no agreement and 0.01–0.20 as none to slight, 0.21–0.40 as fair, 0.41–0.60 as moderate, 0.61–0.80 as substantial and 0.81–1.00 as almost-perfect agreement [46, 47].

Regarding the intergroup comparison, the positive control group (II) showed a significant loss in the mean inter-radicular bone density compared to all study groups. On the other hand, different treatment modalities in groups MTA (III), MTA + PRF (IV) and MTA + CGF (V) demonstrated a statistically significant increase in mean inter-radicular bone density over the positive control group (II) (P < 0.001). Groups MTA + PRF and MTA + CGF showed a non-statistically significant increase in mean bone density compared to the MTA group, independent of subdivision. Still, the follow-up radiographs of these groups (MTA, MTA + PRF and MTA + CGF) showed significantly decreased mean inter-radicular bone density than the negative control group (I). In terms of intragroup comparisons, all teeth of contaminated perforations subdivision (1) showed a less statistically significant increase in mean bone density than those of non-contaminated subdivision (2) in groups MTA, MTA + PRF and MTA + CGF (P = 0.002, < 0.001, 0.012 respectively). However, the positive control group showed no statistically significant variations across subdivisions (P = 0.522).

Histologic analysis for the teeth in the negative control group (I) indicated normal alveolar bone with osseous remodelling. Trabecular spaces were typically occupied by fatty bone marrow and blood arteries/arterioles. There were no inflammatory alterations in the periodontium, and the periodontal ligament fibres were oriented obliquely (Fig. 4A).

All experimental groups demonstrated a significant increase in the frequency of epithelial proliferation compared to the negative control group (I), while there was significantly less frequent epithelial proliferation in groups MTA, MTA + PRF and MTA + CGF than in the positive control group. At the same time, no significant differences were detected between groups MTA, MTA + PRF and MTA + CGF. The non-contaminated subdivisions showed non-statistically significant less frequency of epithelial proliferation than the contaminated subgroup in all groups.