Abstract

Deciphering structure/function relationships underpins the acquisition of biomedical knowledge while providing the basis to create novel materials and drugs. A powerful tool for deciphering structure/function outcomes has been germline genetic manipulation in mice. In this application, we apply germline manipulation to link structure to function for the enamel matrix protein ameloblastin. Enamel is a composite bioceramic tissue with unique material properties that are owed to its mode of biological fabrication. Ameloblast cells create an extracellular enamel protein matrix that serves to control both crystallite habit and the organization of crystallite bundles, allowing thousands of nanoscale crystallites to be organized and grouped together under the control of a single cell. We hypothesize that the grouping and organization of the nanocrystallites by a single ameloblast cell is the outcome achieved by the function(s) of critical domain(s) within the ameloblastin protein. The ameloblastin protein has been described as being organized into at least two domains, an N'- and a C'- terminal domain [Iwata et al. '07], based on the finding that following cleavage the N'- and C'- ameloblastin domains are no longer found in the same physical site in the enamel rod. The N'-terminus is enriched around the rod boundaries, much as a sheath covers a knife blade, while the C'-terminal domain behaves quite differently. We hypothesize that the N'-terminus of ameloblastin is likely responsible for the cell-to-matrix interactions that maintain the highly patterned rod-to-interrod boundaries observed in enamel. We hypothesize that the C'-terminus is responsible for the protein-to-mineral interactions producing the enamel bioceramic tissue. Outcomes will be measured by changes to stereotypic enamel architecture and by analysis of the material properties of the enamel in the knockin condition compared to wildtype animals. The outcomes from this experimental strategy will contribute to our understanding of functional genomics and proteomics while furthering our understanding of the formation of the only ectoderm-derived biomineralized tissue in the vertebrate body. Preliminary data from our research team suggest that this knockin approach will yield novel insights into the structure/function relationship for the ameloblastin protein, the second most abundant protein contributing to enamel organic matrix assembly and biomineralization.

Public Health Relevance

The function(s) for the second most abundant protein of the forming mammalian enamel matrix is not known. Here, we map the function(s) of ameloblastin protein domains to the production of the enamel matrix required to control enamel biomineralization. In performing this project we will create an animal model useful to study caries, the most prevalent-, infectious-disease of humankind and provide one more design specification for creating an enamel biomimetic, useful for restoring enamel lost to trauma and disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Dental & Craniofacial Research (NIDCR)
Type
Research Project (R01)
Project #
5R01DE013045-12
Application #
8106413
Study Section
Special Emphasis Panel (ZRG1-MOSS-K (09))
Program Officer
Lumelsky, Nadya L
Project Start
1998-08-01
Project End
2015-05-31
Budget Start
2011-06-01
Budget End
2012-05-31
Support Year
12
Fiscal Year
2011
Total Cost
$383,820
Indirect Cost

  Institution

Name
University of Southern California
Department
Dentistry
Type
Schools of Dentistry
DUNS #
072933393
City
Los Angeles
State
CA
Country
United States
Zip Code
90089

  Publications

Yin, Kaifeng; Lin, Wenting; Guo, Jing et al. (2017) MiR-153 Regulates Amelogenesis by Targeting Endocytotic and Endosomal/lysosomal Pathways-Novel Insight into the Origins of Enamel Pathologies. Sci Rep 7:44118
Mounir, Maha M F; Matar, Moustafa A; Lei, Yaping et al. (2016) Recombinant Amelogenin Protein Induces Apical Closure and Pulp Regeneration in Open-apex, Nonvital Permanent Canine Teeth. J Endod 42:402-12
Nurbaeva, M K; Eckstein, M; Snead, M L et al. (2015) Store-operated Ca2+ Entry Modulates the Expression of Enamel Genes. J Dent Res 94:1471-7
Yin, Kaifeng; Lei, Yuejuan; Wen, Xin et al. (2015) SLC26A Gene Family Participate in pH Regulation during Enamel Maturation. PLoS One 10:e0144703
Zhou, Yan; Snead, Malcolm L; Tamerler, Candan (2015) Bio-inspired hard-to-soft interface for implant integration to bone. Nanomedicine 11:431-4
Geng, Shuhui; White, Shane N; Paine, Michael L et al. (2015) Protein Interaction between Ameloblastin and Proteasome Subunit ? Type 3 Can Facilitate Redistribution of Ameloblastin Domains within Forming Enamel. J Biol Chem 290:20661-73
Yang, Ting; Zhang, Yanli; Zheng, Dongdong et al. (2015) High-fluoride promoted phagocytosis-induced apoptosis in a matured ameloblast-like cell line. Arch Oral Biol 60:84-90
Snead, Malcolm L (2015) Biomineralization of a self-assembled-, soft-matrix precursor: Enamel. JOM (1989) 67:788-795
Yucesoy, Deniz T; Hnilova, Marketa; Boone, Kyle et al. (2015) Chimeric peptides as implant functionalization agents for titanium alloy implants with antimicrobial properties. JOM (1989) 67:754-766
Jang, Hae Lin; Lee, Keunho; Kang, Chan Soon et al. (2015) Biofunctionalized ceramic with self-assembled networks of nanochannels. ACS Nano 9:4447-57

Showing the most recent 10 out of 51 publications