PROJECT SUMMARY/ABSTRACT Regulation of stem cell functions is crucial for tissue formation, growth, and homeostasis. In many tissues and organs, stem cells give rise to transit amplifying cells (TACs), an undifferentiated progenitor population. TACs function as transient but indispensable integrators of stem cell niche components. However, we have limited understanding of how mesenchymal stem cells (MSCs) interact with TACs and provide feedback to MSCs in regulating tissue homeostasis. The adult mouse incisor provides an excellent model for stem cell study because it grows continuously. MSCs are a Gli1+ cell population surrounding the neurovascular bundle (NVB) near the proximal region in the adult mouse incisor, making it an ideal model in which to investigate the regulatory mechanisms of MSCs. The NVB may secrete signaling molecules, providing a niche for MSCs in the adult incisor. However, the functional significance of signaling molecules from the nerve within the NVB and the molecular mechanism by which they regulate MSCs are largely unknown. Significantly, our preliminary data shows that the trigeminal nerve secretes Fgf1, which acts directly on MSCs via FGFR1 to regulate tissue homeostasis, as loss of Fgfr1 in Gli1+ MSCs leads to retarded incisor growth, similar to the phenotype seen with compromised innervation. Fgf signaling regulates important downstream epigenetic regulators such as Arid1a and Arid1b to control the fate of TACs. Furthermore, loss of Arid1a specifically inhibits Wnt5a signaling, which may provide feedback to MSCs. Importantly, we have recently discovered that Runx2+/Gli1+ cells in the adult incisor are MSC niche cells, strategically positioned to coordinate MSC-to-TAC transition. Our study suggests that Runx2 is regulated by the epigenetic regulator Arid1b and controls p53 activity to mediate MSC-to-TAC transition and feedback to MSCs. Collectively, based on our preliminary data and taking advantage of well-established animal models, we propose to test the hypotheses that Fgf signaling from the trigeminal nerve regulates MSCs in the adult mouse incisor, Arid1a and Arid1b act downstream of Fgf signaling to control MSC-to-TAC transition, and Arid1b-Runx2 interaction regulates p53 activity to control TAC differentiation and feedback to MSCs to maintain tissue homeostasis. We propose the following specific aims to test our hypotheses. Specific Aim 1: To investigate whether Fgf signaling from the trigeminal nerve plays a crucial role in regulating MSCs in the adult mouse incisor. We will explore the molecular mechanism of Fgf signaling and its downstream targets in regulating the fate of MSCs to maintain mesenchymal tissue homeostasis. Specific Aim 2: To determine the role of Fgf- regulated Arid1a and Arid1b activity in controlling the MSC-to-TAC transition and maintenance of incisor tissue homeostasis. We will explore the mechanisms by which TAC fate is altered and their impact on MSCs in Arid1a and Arid1b mutant mice. Spec...