Abstract

To achieve the long-term goal of restoring dental enamel, it is necessary to understand the fundamental chemical and biological principles of extracellular matrix assembly and the manner they control mineral nucleation and growth. There is still a large gap in our understanding of the underlying molecular mechanisms by which enamel matrix proteins assemble and interact with cells to control nucleation and oriented growth of hydroxyapatite crystals, and possibly cell movement and polarization. This is particularly true of ameloblastin protein, which is the focus of our proposed study. The goal of this proposal is therefore to advance our understanding of ameloblastin?s structure and function through a systematic investigation of its interactions with different targets. We hypothesize that the highly organized carbonated hydroxyapatite crystals in enamel continuously grow and form prismatic structures by means of complex ameloblastin-cell, ameloblastin- amelogenin, and ameloblastin-mineral interactions. Two major aims are proposed to systematically examine the above hypothesis by applying in vitro chemical models, cell culture and animal models for amelogenesis.
Aim I : To investigate ameloblastin-cell membrane interactions and identify the interacting domains using in vitro synthetic liposomes and ameloblast-like cell culture model systems. We will design several mouse models with point mutations in the interacting domains identified, and examine the consequence of these mutations on enamel prismatic structure, ameloblast morphology, and the attachment of the cells to the matrix. We hypothesize that ameloblastin interacts with ameloblast cells via a domain in the sequence encoded by exon 5 and functions to anchor the mineralizing extracellular matrix to the enamel-forming cells affecting cell polarization, migration, and the formation of Tomes? processes.
Aim II : To investigate ameloblastin-amelogenin interactions on the nanoscale in vivo and in vitro, and to identify their interacting domains using solution NMR spectroscopy. We will study the dynamics of calcium phosphate mineralization events on the nanoscale when ameloblastin is combined with amelogenin, using high resolution in situ atomic force (AFM) and Cryo- transmission electron microscopy (TEM). We hypothesize that amelogenin and ameloblastin form hetereomolecular entities that are functional during different stages of amelogenesis to control crystal formation. We anticipate to gain more insight into the structure, assembly properties and function of ameloblastin. We will define a novel cell- membrane- binding domain on ameloblastin protein. Novel protein- protein-interacting domains on the ameloblastin and amelogenin sequences will be identified. The effect of ameloblastin combined with amelogenin on mineralization will be elucidated and mineral-binding domains will be identified. These studies will advance understanding of the molecular function of ameloblastin in enamel biomineralization and will contribute to our efforts to fabricate synthetic enamel.

Public Health Relevance

The goal of this proposal is to unravel the detailed molecular mechanisms of ameloblastin interactions with cell membrane, with mineral and with amelogenin, and hence to contribute to the fundamental knowledge as relevant to enamel formation. The outcomes will advance understanding of the molecular function of ameloblastin in enamel biomineralization and will contribute to our efforts to fabricate enamel bioinspired materials. We propose that such biomaterials could be developed as a future generation of dental restorative material and the procedures developed for their creation are expected to have applications beyond dental material field.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Dental & Craniofacial Research (NIDCR)
Type
Research Project (R01)
Project #
2R01DE013414-14A1
Application #
9660330
Study Section
Special Emphasis Panel (ZRG1)
Program Officer
Wan, Jason
Project Start
2019-05-01
Project End
2023-04-29
Budget Start
2019-05-01
Budget End
2020-04-30
Support Year
14
Fiscal Year
2019
Total Cost
Indirect Cost

  Institution

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

  Publications

Prajapati, S; Ruan, Q; Mukherjee, K et al. (2018) The Presence of MMP-20 Reinforces Biomimetic Enamel Regrowth. J Dent Res 97:84-90
Mukherjee, Kaushik; Ruan, Qichao; Nutt, Steven et al. (2018) Peptide-Based Bioinspired Approach to Regrowing Multilayered Aprismatic Enamel. ACS Omega 3:2546-2557
Klein, Ophir D; Duverger, Olivier; Shaw, Wendy et al. (2017) Meeting report: a hard look at the state of enamel research. Int J Oral Sci 9:e3
Ruan, Qichao; Liberman, David; Zhang, Yuzheng et al. (2016) Assembly of Layered Monetite-Chitosan Nanocomposite and Its Transition to Organized Hydroxyapatite. ACS Biomater Sci Eng 2:1049-1058
Ren, Dongni; Ruan, Qichao; Tao, Jinhui et al. (2016) Amelogenin Affects Brushite Crystal Morphology and Promotes Its Phase Transformation to Monetite. Cryst Growth Des 16:4981-4990
Mazumder, P; Prajapati, S; Bapat, R et al. (2016) Amelogenin-Ameloblastin Spatial Interaction around Maturing Enamel Rods. J Dent Res 95:1042-8
Su, Jingtan; Chandrababu, Karthik Balakrishna; Moradian-Oldak, Janet (2016) Ameloblastin peptide encoded by exon 5 interacts with amelogenin N-terminus. Biochem Biophys Rep 7:26-32
Ruan, Qichao; Liberman, David; Bapat, Rucha et al. (2016) Efficacy of amelogenin-chitosan hydrogel in biomimetic repair of human enamel in pH-cycling systems. J Biomed Eng Inform 2:119-128
Prajapati, Saumya; Tao, Jinhui; Ruan, Qichao et al. (2016) Matrix metalloproteinase-20 mediates dental enamel biomineralization by preventing protein occlusion inside apatite crystals. Biomaterials 75:260-270
Bauskar, Aditi; Mack, Wendy J; Mauris, Jerome et al. (2015) Clusterin Seals the Ocular Surface Barrier in Mouse Dry Eye. PLoS One 10:e0138958

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