1J), whereas maxillary injury sites remained filled with connective/fibrous tissue (Fig. 1L). Therefore, in addition to their distinct embryonic origins, and a measurable osteogenic capacity of bone grafts derived from the two skeletal elements, craniofacial and long bones have different rates of healing.
We reasoned that this difference would likely manifest as a change in the rate or AZD1208 in vivo extent of implant osseointegration. Our primary interest is in addressing failures in oral implant osseointegration. Given the different healing potentials of long bones and craniofacial bones, we opted to develop an oral implant model system that would afford us with the ability to rigorously assess the program of oral implant osseointegration. We first carried out a series of experiments in which implants were placed in the tibia. The surgical procedure,
the osseointegration response, and the molecular and cellular characteristics of this process have been documented elsewhere [6], [11], [14], [15], [17], [26] and [27]. Here, we show that new bone, originating from the tibial marrow cavity, is first evident on post-surgical day 5 (Supplemental Fig. 1A). The peri-implant bone is osseointegrated Fulvestrant cell line by day 7 (Supplemental Fig. 1B), and undergoes extensive remodeling at subsequent time points (Supplemental Fig. 1C–E). We compared osseointegration in the tibia with osseointegration in the maxilla. MycoClean Mycoplasma Removal Kit Maxillary injuries were created immediately anterior to the first molar, along the alveolar crest in the edentulous space. After anesthesia, the oral cavity was rinsed with povidone–iodine solution (Fig. 2A) and a full thickness crestal incision was performed (Fig. 2B).
The flap was raised and the alveolar bone was accessed (Fig. 2C). In an attempt to reduce trauma to the alveolar bone, a pilot hole was first created using a 0.3 mm drill, followed by a 0.45 mm drill (Fig. 2D). The implant (0.6 mm; Fig. 2E) was subsequently screwed into place (Fig. 2F). The gingival tissue was sutured in place, effectively enclosing the implant (Fig. 2G). The position of the implant was anterior to the first molar, along the edentulous ridge, perforating the sinus in all cases (Fig. 2H). After 14 days, the enclosed implant could be visualized through the tissue (Fig. 2I). Thus, the procedure used to place a murine oral implant was very similar to the procedure used for humans. We first evaluated murine implants using histological analyses and found that within 7 days, there was evidence of bone formation in the peri-implant space (Fig. 3A). Upon close examination, the new bone appeared as an extension of the periosteal surfaces of the native maxillary bone (Fig. 3A′,A″). Fibroblasts also occupied the space between the cut edge of the bone and the implant surface (Fig. 3A′,A″). On day 14, more new bone was in contact with the implant surface (Fig. 3B, B′ and E).