ABSTRACT
Objetivo: caracterizar o processo de reparo ósseo peri-implantar em maxilas de ratas ovariectomizadas com síndrome metabólica induzida por dieta de cafeteria, tratadas com risedronato e instalação de implantes funcionalizados com [Ru(terpy)(bdq)NO]3+ (TERPY). Materiais e métodos: os testes in vitro realizados na Fase 1 avaliou as propriedades biológicas e físico-químicas da melhor concentração da TERPY frente às respostas osteogênicas, para a funcionalização dos implantes pela técnica de LbL. A realização de experimentos in vivo na Fase 2 avaliou o efeito da superfície funcionalizada durante o reparo ósseo peri-implantar. Para isso, 48 ratas Wistar foram divididas em: SHAM CONV (n=8), OVX SM CONV (n=8), OVX SM RIS CONV (n=8), SHAM TERPY (n=8), OVX SM TERPY (n=8) e OVX SM RIS TERPY (n=8). Em t=0, as ratas foram submetidas à cirurgia fictícia (SHAM) e à cirurgia de ovariectomia bilateral (OVX); após a recuperação da cirurgia, os animais receberam a dieta de cafeteria (SM). Passados 30 dias (t=30), o tratamento medicamentoso com risedronato de sódio (0,7 mg/kg/semana) (RIS) ou solução salina (0,3 ml), via gavagem, foi iniciado e realizado até o momento da eutanásia. Sessenta dias após o início do tratamento medicamentoso (t=90), a cirurgia de exodontia do primeiro molar superior foi realizada junto à instalação imediata dos implantes de forma bilateral (CONV ou TERPY). Quatorze dias após a cirurgia de instalação dos implantes (t=104), todos os grupos experimentais receberam a injeção intramuscular do fluorocromo calceína (20 mg/kg) e após 10 dias (t=114), do fluorocromo vermelho de alizarina (25 mg/kg). Aos 28 dias pós-operatórios (dia da eutanásia, t=118), os animais foram anestesiados e, nas maxilas do lado direito, os implantes foram submetidos ao torque reverso e imediatamente após a remoção dos implantes, foi realizada a coleta do tecido ósseo para análise de PCR tempo real para avaliação da expressão relativa de ALP, iBSP, OCN, OPG, RANKL, TRAP e VEGF, seguido da eutanásia dos animais; as maxilas do lado esquerdo foram coletadas para a análise de Micro-CT (BV/TV, Tb.Th, Tb.N, Tb.Sp e i.S) e, após o escaneamento, as mesmas passaram pelo processamento para análise da dinâmica óssea por fluorocromos (MAR e ELCOI). Os dados foram submetidos à análise estatística, com o nível de significância de 5% (p<0,05). Resultados: Fase 1: poucas diferenças foram observadas entre as duas concentrações avaliadas e assim, a menor concentração do fármaco foi selecionada (10µM). Fase 2: os implantes funcionalizados com a TERPY apresentaram os maiores valores absolutos de torque de remoção para todos os grupos e com diferença estatística para OVX SM TERPY (p=0,0402). A associação sistêmica entre o risedronato e a TERPY em ratas ovariectomizadas (OVX SM RIS TERPY) demonstrou expressão aumentada para iBSP e equilíbrio entre OPG e RANKL, corroborando com os dados obtidos para MAR (p=0,0052) e com os parâmetros de BV/TV, Tb.Th e i.S da análise microtomográfica para esse mesmo grupo. Conclusão: o desempenho clínico dos implantes funcionalizados com TERPY foi favorável, e, quando associado à administração sistêmica de risedronato de sódio, os resultados se tornam mais promissores(AU)
Objective: characterize the peri-implant bone tissue repair process in maxilla of ovariectomized rats with metabolic syndrome induced by cafeteria diet, treated with risedronate and through placement the implants functionalized with [Ru(terpy)(bdq)NO]3+ (TERY). Materials and methods: in vitro tests performed in Phase 1 evaluated the biological and physicochemical properties of the better concentration of TERPY against osteogenic responses, for the functionalization of implants using the LbL technique. In vivo experiments in Phase 2 evaluated the effect of functionalized surface during peri-implant bone repair. For this, 48 female rats were divided: SHAM CONV (n=8), OVX SM CONV (n=8), OVX SM RIS CONV (n=8), SHAM TERPY (n=8), OVX SM TERPY (n=8) and OVX SM RIS TERPY (n=8). At t=0, the rats underwent unreal surgery (SHAM) and bilateral ovariectomy surgery (OVX); after recovery from surgery, animals received cafeteria diet (SM). After 30 days (t=30), drug treatment with risedronate sodium (0.7 mg/kg/week) (RIS) or saline solution (0.3 ml), via gavage, was started and sustained out until the time of euthanasia. Sixty days after the start of drug treatment (t=90), the maxillary first molar extraction surgery was performed followed by the immediate installation of the implants bilaterally (CONV or TERPY). Fourteen days after implant placement surgery (t=104), all experimental groups received intramuscular injection of the fluorochrome calcein (20 mg/kg) and after 10 days (t=114), the red fluorochrome alizarin (25 mg/kg). After 28 postoperative days (day of euthanasia, t=118), the animals were anesthetized and, in the maxillary on the right side, the implants were subjected to reverse torque and immediately after removal of the implants, bone tissue was collected for real-time PCR analysis to measure the relative expression of ALP, iBSP, OCN, OPG, RANKL, TRAP e VEGF, followed by euthanasia of animals; the left side maxillary were collected for Micro-CT analysis (BV/TV, Tb.Th, Tb.N, Tb.Sp e i.S) and, after scanning, they underwent processing for analysis of bone dynamics by fluorochromes (MAR and ELCOI). Data values were subjected to statistical analysis, with a significance level of 5% (p<0.05). Results: Phase 1: few differences were observed between the two concentrations evaluated and thus, the lowest drug concentration was selected (10µM). Phase 2: the implants functionalized with TERPY presented the highest absolute values of removal torque for all groups and with statistical difference for OVX SM TERPY (p=0.0402). The systemic association between risedronate and TERPY in ovariectomized rats (OVX SM RIS TERPY) showed increased expression for iBSP and balance between OPG and RANKL, corroborating the data obtained for MAR (p=0.0052) and with the parameters BV/TV, Tb.Th and i.S of the microtomographic analysis for this same group. Conclusion: the clinical performance of implants functionalized with TERPY was favorable, and when associated with the systemic administration of risedronate sodium, the results become more promising(AU)
Subject(s)
Animals , Rats , Bone Regeneration , Dental Implants , Estrogens , Nitric Oxide , Osteonecrosis , Osseointegration , Rats, Wistar , Bisphosphonate-Associated Osteonecrosis of the Jaw , Bone-Implant InterfaceABSTRACT
Abstract The hypothesis of this study was that the peri-implant bone healing of the group of pinealectomized rats would differ from the control group. The samples were subjected to immunohistochemical, microtomographic (total porosity and connectivity density), and fluorochrome (mineralized surface) analyses. Objectives The goal of this study was to investigate the cellular changes and bone remodeling dynamics along the bone/implant interface in pinealectomized rats. Material and Methods The total of 18 adult male rats (Rattus norvegicus albinus, Wistar) was divided into three groups (n=6): control (CO), pinealectomized without melatonin (PNX) and pinealectomized with melatonin (PNXm). All animals were submitted to the first surgery (pinealectomy), except the CO group. Thirty days after the pinealectomy without melatonin, the second surgery was conducted, in which all animals received an implant in each tibia (36 titanium implants with surface treatment were installed - Implalife® São Paulo, SP, Brazil). By gavage, the rats of the PNX group received the vehicle solution, and the procedure. Results Immunohistochemical analysis for runt-related transcription factor 2 (RUNX2), alkaline phosphatase (ALP), osteopontin (OP) and osteocalcin (OC) showed that the bone repair process in the PNXm group was similar to that of the CO group, whereas the PNX group showed a delay. The microtomographic parameters of total porosity [Po(tot)] and bone surface (BS) showed no statistically significant differences, whereas for the connective density (Conn.Dn) a statistical difference was found between the CO and PNXm groups. Fluorochrome analysis of the active mineralized surface showed statistically significant difference between the CO and PNX and between the CO and PNXm groups. Conclusion The absence of the pineal gland impaired the bone repair process during osseointegration, however the daily melatonin replacement was able to restore this response.
Subject(s)
Animals , Male , Pineal Gland/surgery , Osseointegration/drug effects , Bone Density Conservation Agents/pharmacology , Bone-Implant Interface , Melatonin/pharmacology , Tibia/drug effects , Tibia/injuries , Tibia/pathology , Titanium , Immunohistochemistry , Osteocalcin/analysis , Reproducibility of Results , Treatment Outcome , Rats, Wistar , Implants, Experimental , Dental Implantation, Endosseous , Alkaline Phosphatase/analysis , Core Binding Factor Alpha 1 Subunit/analysis , Osteopontin/analysis , X-Ray Microtomography , Fluorescent DyesABSTRACT
This study aimed to evaluate the diffusion capacity of calcium hydroxide pastes with different vehicles through dentinal tubules. The study was conducted on 60 extracted single-rooted human teeth whose crowns had been removed. The root canals were instrumented and divided into 4 groups according to the vehicle of the calcium hydroxide paste: Group I - distilled water; Group II - propylene glycol; Group III - 0.2 percent chlorhexidine; Group IV - 2 percent chlorhexidine. After placement of the root canal dressings, the teeth were sealed and placed in flasks containing deionized water. After 1, 2, 7, 15, 30, 45 and 60 days, the pH of the water was measured to determine the diffusion of calcium hydroxide through the dentinal tubules. The data were recorded and statistically compared by the Tukey test. The results showed that all pastes presented a similar diffusion capacity through dentin. Group IV did not present difference compared to group I. Group II presented difference compared to the other groups, as did Group III. In conclusion, groups I and IV presented a better diffusion capacity through dentin than groups II and III; 2 percent chlorhexidine can be used as a vehicle in calcium hydroxide pastes.