Templated biomineralization on self-assembled protein fibers

  1. K. Subburaman*,
  2. N. Pernodet*,
  3. S. Y. Kwak,,
  4. E. DiMasi,
  5. S. Ge*,
  6. V. Zaitsev*,
  7. X. Ba*,
  8. N. L. Yang§, and
  9. M. Rafailovich*
  1. *Department of Materials Science and Engineering, Stony Brook University, Stony Brook, NY 11794;
  2. National Synchrotron Light Source, Brookhaven National Laboratory, Upton, NY 11973; and
  3. §Department of Chemistry, City University of New York, Staten Island, NY 10314

  1. Edited by Lia Addadi, Weizmann Institute, Rehovot, Israel, and accepted by the Editorial Board August 7, 2006 (received for review April 11, 2006)

Abstract

Biological mineralization of tissues in living organisms relies on proteins that preferentially nucleate minerals and control their growth. This process is often referred to as “templating,” but this term has become generic, denoting various proposed mineral–organic interactions including both chemical and structural affinities. Here, we present an approach using self-assembled networks of elastin and fibronectin fibers, similar to the extracellular matrix. When induced onto negatively charged sulfonated polystyrene surfaces, these proteins form fiber networks of ≈10-μm spacing, leaving open regions of disorganized protein between them. We introduce an atomic force microscopy-based technique to measure the elastic modulus of both structured and disorganized protein before and during calcium carbonate mineralization. Mineral-induced thickening and stiffening of the protein fibers during early stages of mineralization is clearly demonstrated, well before discrete mineral crystals are large enough to image by atomic force microscopy. Calcium carbonate stiffens the protein fibers selectively without affecting the regions between them, emphasizing interactions between the mineral and the organized protein fibers. Late-stage observations by optical microscopy and secondary ion mass spectroscopy reveal that Ca is concentrated along the protein fibers and that crystals form preferentially on the fiber crossings. We demonstrate that organized versus unstructured proteins can be assembled mere nanometers apart and probed in identical environments, where mineralization is proved to require the structural organization imposed by fibrillogenesis of the extracellular matrix.

Footnotes

  • To whom correspondence should be addressed. E-mail: skwak{at}forsyth.org

  • Author contributions: K.S., N.P., S.Y.K., E.D., V.Z., X.B., and M.R. designed research; K.S., N.P., S.Y.K., E.D., V.Z., X.B., and M.R. performed research; S.G. and N.L.Y. contributed new reagents/analytic tools; K.S., N.P., S.Y.K., E.D., V.Z., X.B., and M.R. analyzed data; and K.S., N.P., S.Y.K., E.D., V.Z., X.B., and M.R. wrote the paper.

  • The authors declare no conflict of interest.

  • This paper was submitted directly (Track II) to the PNAS office. L.A. is a guest editor invited by the Editorial Board.

  • Abbreviations:
    ECM,
    extracellular matrix;
    SPS,
    sulfonated polystyrene;
    SMFM,
    shear modulation force microscopy;
    AFM,
    atomic force microscopy;
    SIMS,
    secondary ion mass spectroscopy
« Previous | Next Article »Table of Contents

This Article

  1. Published online before print September 26, 2006, doi: 10.1073/pnas.0602952103 PNAS October 3, 2006 vol. 103 no. 40 14672-14677
  1. » Abstract
  2. Figures Only
  3. Full Text
  4. Full Text (PDF)

Classifications

About Our New Site Design >>
Link: Advanced Search

This Week's Issue

  1. November 18, 2008, 105 (46)
  1. Current Issue
  1. Alert me to new issues of PNAS

Most