We asked how mucoperiosteal denudation could have Ganetespib cost such a profound effect on facial growth. We first created a mouse model of mucoperiosteal denudation that specifically involved the midpalatal suture complex then used histology, immunohistochemistry, finite element (FE) modeling, micro-CT analyses, and quantitative

molecular readouts to draw a direct link between the surgical procedure, the healing response, and the resulting palatal growth inhibition. In doing so we gained critical insights into how a commonly employed surgical procedure could have the unintended consequence of impeding midfacial development. All procedures were approved by the Stanford Committee on Animal Research. Gas anesthesia was delivered to post-natal day 7 (P7) C57BL/6 pups, and the palatal mucoperiosteal denudation was performed before awakening. With the use of a dissecting microscope, a 1 mm diameter full thickness punch was made in the middle of the hard palate and the mucoperiosteum was removed with forceps; care was taken to leave the underlying skeletal tissues intact. The anterior border of the punch is made immediately posterior to the first pair of discontinuous palatal rugae (Supplemental Fig. 1B). The wound healed

by secondary intention. Age-matched littermates that were unoperated served as controls. Tissue samples were fixed in 4% paraformaldehyde at 4 °C overnight, decalcified in 19% EDTA at room temperature for 10 days, and dehydrated for paraffin embedding. Coronal sections were cut at a thickness of 8 μm. Histology was performed using Gomori Trichrome, Movat’s Pentachrome, selleck chemical and Safranin O/Fast Amino acid Green/Hematoxylin staining following standard

staining procedures [28]. Picrosirius red staining was completed and imaged under polarized light as described [28]. For alkaline phosphatase (ALP) staining, slides were pre-incubated in NTMT buffer for 15 min and then stained in ALP solution containing 2 mL NTMT, 10 μl NBT (Roche), and 7.5 μl BCIP (Roche) for 30 min at 37 °C. Tartrate resistant acid phosphatase (TRAP) staining was performed using a Leukocyte Acid Phosphatase Kit (Sigma, St. Louis, MO). Immunohistochemistry for Ki67, Osteopontin, collagen I, collagen II, and X was carried out as described [28]. In brief, slides were immersed in 0.2% Triton for 5 min then incubated in Antigen Unmasking Solution (Vector Laboratories, diluted 1:100) at 95 °C for 20 min. After returning to room temperature slides were immersed in 3% hydrogen peroxide for 5 min and blocked in 5% goat serum for 30 min. Slides were incubated in corresponding primary antibodies (Ki67 rabbit polyclonal antibody, Thermo Scientific, diluted 1:100; Osteopontin rabbit polyclonal, Abcam, diluted 1:2000; Collagen I rabbit polyclonal antibody, Calbiochem, diluted 1:500; Collagen II rabbit polyclonal antibody, Millipore, diluted 1:50; Collagen X rabbit polyclonal antibody, Calbiochem, diluted 1:500) overnight at 4 °C.