Abstract

The amelogenins are extracellular matrix proteins, produced by ameloblasts during tooth enamel formation. These proteins are unique to enamel and are required for normal development of enamel mineral. The purpose of this application is to investigate regulation of expression of the X- chromosomal amelogenin gene, by analyzing the 3.5 KB fragment able to direct expression of a reporter gene to ameloblasts in transgenic mice, by sequence analysis and testing selected segments for activity using transgenic mice. We will also create in vivo a murine null mutation for the amelogenin gene, and express leucine rich amelogenin protein (RAP) in transgenic mouse enamel to determine whether overexpression will interfere with the normal function of amelogenin proteins. Mating of the knockout and LRAP mice will yield offspring which secrete LRAP as the only amelogenin protein in developing enamel.
The specific aims are: (1) to characterize the regulatory sequences of the X-chromosomal amelogenin gene, using transgenic mice; (2) to construct a """"""""knockout"""""""" mouse for the X-chromosomal amelogenin gene; (3) to construct a transgenic mouse that overexpresses LRAP in ameloblasts under control of the amelogenin regulatory sequence; and (4) to replace the amelogenin protein with LRAP in mouse tooth enamel. In these experiments, teeth from the 3 genetically altered mouse lines will be compared histologically for tissue alterations, and for quality and composition of mineral crystal, in order to better understand the role of the organic matrix in the mineralization process.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Dental & Craniofacial Research (NIDCR)
Type
Research Project (R01)
Project #
5R01DE011089-03
Application #
2430125
Study Section
Special Emphasis Panel (ZRG4-OBM-2 (06))
Project Start
1995-06-01
Project End
1999-03-31
Budget Start
1997-06-01
Budget End
1998-05-31
Support Year
3
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
University of Pennsylvania
Department
Anatomy/Cell Biology
Type
Schools of Dentistry
DUNS #
042250712
City
Philadelphia
State
PA
Country
United States
Zip Code
19104

  Publications

Guo, J; Lyaruu, D M; Takano, Y et al. (2015) Amelogenins as potential buffers during secretory-stage amelogenesis. J Dent Res 94:412-20
Pugach, Megan K; Ozer, Fusun; Mulmadgi, Raj et al. (2014) Shear bond strength of dentin and deproteinized enamel of amelogenesis imperfecta mouse incisors. Pediatr Dent 36:130-6
Li, Yong; Konicki, William S; Wright, J Timothy et al. (2013) Mouse genetic background influences the dental phenotype. Cells Tissues Organs 198:448-56
Pugach, M K; Suggs, C; Li, Y et al. (2013) M180 amelogenin processed by MMP20 is sufficient for decussating murine enamel. J Dent Res 92:1118-22
Xue, Hui; Li, Yong; Everett, Eric T et al. (2013) Ameloblasts require active RhoA to generate normal dental enamel. Eur J Oral Sci 121:293-302
Gibson, Carolyn W; Li, Yong; Suggs, Cynthia et al. (2011) Rescue of the murine amelogenin null phenotype with two amelogenin transgenes. Eur J Oral Sci 119 Suppl 1:70-4
Wright, J Tim; Li, Yong; Suggs, Cynthia et al. (2011) The role of amelogenin during enamel-crystallite growth and organization in vivo. Eur J Oral Sci 119 Suppl 1:65-9
Gibson, Carolyn W (2011) The Amelogenin Proteins and Enamel Development in Humans and Mice. J Oral Biosci 53:248-256
Pugach, M K; Ozer, F; Li, Y et al. (2011) The use of mouse models to investigate shear bond strength in amelogenesis imperfecta. J Dent Res 90:1352-7
Li, Yong; Pugach, Megan K; Kuehl, Melissa A et al. (2011) Dental enamel structure is altered by expression of dominant negative RhoA in ameloblasts. Cells Tissues Organs 194:227-31

Showing the most recent 10 out of 37 publications