Abstract

The overall goal of this research is to elucidate the structure-function relationships of the biomineralization proteins driving the formation of enamel. Enamel is the most highly ordered biomineralization crystal and is uniquely designed to handle abrasions and mechanical stress. As with many biomineralization processes, though, very little is understood about the mechanisms controlling enamel nucleation and growth, although the presence of proteins has been deemed critical. Enamelins, tuftelins, ameloblastins and amelogenins are all present during enamel formation and all have been suggested as candidates for crystal nucleation. Amelogenin consists of 90% of the protein present during enamel growth, is necessary for proper enamel formation and is likely a major contributor in the development of the calcium phosphate crystal. In addition to a possible nucleation role, amelogenin forms unique self assembled nanospheres which are thought to be tied to the elongated growth of enamel crystals during development. Structure-function relationships will be elucidated primarily using solid state NMR (SSNMR), Quartz Crystal Microbalance (QCM) and constant composition kinetics (CCK) to study the immobilized protein under the wide variety of conditions found in developing enamel. SSNMR will be used to accurately determine the secondary structure, dynamics and amino acids important in binding the protein or protein self assembly to calcium phosphates. QCM will be used to investigate nucleation rates and protein binding kinetics. The surface specific interactions will be probed with CCK to determine crystal growth inhibition and change in crystal growth mechanism. Site directed mutations, shown to cause defects in enamel will also be studied, to further aid in understanding of the developing enamel interface. Correlating the SSNMR results with kinetic measurements will provide a great deal of insight into the importance of the secondary and quaternary structure of amelogenin in formation of the enamel matrix. These studies will yield an in depth understanding of the molecular level processes involved in the formation of teeth, and more generally will provide basic insight into protein/crystal interactions. ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Dental & Craniofacial Research (NIDCR)
Type
Research Project (R01)
Project #
5R01DE015347-02
Application #
7060029
Study Section
Oral, Dental and Craniofacial Sciences Study Section (ODCS)
Program Officer
Kousvelari, Eleni
Project Start
2005-05-01
Project End
2009-04-30
Budget Start
2006-05-01
Budget End
2007-04-30
Support Year
2
Fiscal Year
2006
Total Cost
$404,914
Indirect Cost

  Institution

Name
Battelle Pacific Northwest Laboratories
Department
Type
DUNS #
032987476
City
Richland
State
WA
Country
United States
Zip Code
99352

  Publications

Arachchige, Rajith Jayasinha; Burton, Sarah D; Lu, Jun-Xia et al. (2018) Solid-State NMR Identification of Intermolecular Interactions in Amelogenin Bound to Hydroxyapatite. Biophys J 115:1666-1672
Zerfaß, Christian; Buchko, Garry W; Shaw, Wendy J et al. (2017) Secondary structure and dynamics study of the intrinsically disordered silica-mineralizing peptide P5 S3 during silicic acid condensation and silica decondensation. Proteins 85:2111-2126
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
Tao, Jinhui; Buchko, Garry W; Shaw, Wendy J et al. (2015) Sequence-Defined Energetic Shifts Control the Disassembly Kinetics and Microstructure of Amelogenin Adsorbed onto Hydroxyapatite (100). Langmuir 31:10451-60
Buchko, Garry W; Shaw, Wendy J (2015) Improved protocol to purify untagged amelogenin - Application to murine amelogenin containing the equivalent P70?T point mutation observed in human amelogenesis imperfecta. Protein Expr Purif 105:14-22
Shaw, Wendy J (2015) Solid-state NMR studies of proteins immobilized on inorganic surfaces. Solid State Nucl Magn Reson 70:1-14
Tarasevich, Barbara J; Philo, John S; Maluf, Nasib Karl et al. (2015) The leucine-rich amelogenin protein (LRAP) is primarily monomeric and unstructured in physiological solution. J Struct Biol 190:81-91
Lu, Jun-Xia; Burton, Sarah D; Xu, Yimin S et al. (2014) The flexible structure of the K24S28 region of Leucine-Rich Amelogenin Protein (LRAP) bound to apatites as a function of surface type, calcium, mutation, and ionic strength. Front Physiol 5:254
Buchko, Garry W; Lin, Genyao; Tarasevich, Barbara J et al. (2013) A solution NMR investigation into the impaired self-assembly properties of two murine amelogenins containing the point mutations T21?I or P41?T. Arch Biochem Biophys 537:217-24
Tarasevich, Barbara J; Perez-Salas, Ursula; Masica, David L et al. (2013) Neutron reflectometry studies of the adsorbed structure of the amelogenin, LRAP. J Phys Chem B 117:3098-109

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