Materials Map

Discover the materials research landscape. Find experts, partners, networks.

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The Materials Map is an open tool for improving networking and interdisciplinary exchange within materials research. It enables cross-database search for cooperation and network partners and discovering of the research landscape.

The dashboard provides detailed information about the selected scientist, e.g. publications. The dashboard can be filtered and shows the relationship to co-authors in different diagrams. In addition, a link is provided to find contact information.

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The Materials Map is still under development. In its current state, it is only based on one single data source and, thus, incomplete and contains duplicates. We are working on incorporating new open data sources like ORCID to improve the quality and the timeliness of our data. We will update Materials Map as soon as possible and kindly ask for your patience.

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in Cooperation with on an Cooperation-Score of 37%

Topics

Publications (3/3 displayed)

  • 2012Probing the orientation of electrostatically immobilized protein G B1 by time-of-flight secondary ion spectrometry, sum frequency generation, and near-edge X-ray adsorption fine structure spectroscopy55citations
  • 2010Probing the orientation of surface-immobilized protein G B1 using ToF-SIMS, sum frequency generation, and NEXAFS spectroscopy85citations
  • 2010Multi-technique Characterization of Adsorbed Peptide and Protein Orientation26citations

Places of action

Chart of shared publication
Gamble, Lara J.
2 / 3 shared
Stayton, Patrick S.
3 / 3 shared
Baio, Joe E.
1 / 13 shared
Weidner, Tobias
3 / 29 shared
Castner, David G.
3 / 12 shared
Nguyen, Phuong Cac T.
1 / 1 shared
Baio, J. E.
2 / 5 shared
Mccrea, Keith
1 / 1 shared
Samuel, N. T.
1 / 1 shared
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2012
2010

Co-Authors (by relevance)

  • Gamble, Lara J.
  • Stayton, Patrick S.
  • Baio, Joe E.
  • Weidner, Tobias
  • Castner, David G.
  • Nguyen, Phuong Cac T.
  • Baio, J. E.
  • Mccrea, Keith
  • Samuel, N. T.
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article

Probing the orientation of surface-immobilized protein G B1 using ToF-SIMS, sum frequency generation, and NEXAFS spectroscopy

  • Gamble, Lara J.
  • Stayton, Patrick S.
  • Weidner, Tobias
  • Nguyen, Phuong Cac T.
  • Castner, David G.
  • Baugh, Loren
  • Baio, J. E.
Abstract

<p>The ability to orient active proteins on surfaces is a critical aspect of many medical technologies. An important related challenge is characterizing protein orientation in these surface films. This study uses a combination of time-of-flight secondary ion mass spectrometry (ToF-SIMS), sum frequency generation (SFG) vibrational spectroscopy, and near-edge X-ray absorption fine structure (NEXAFS) spectroscopy to characterize the orientation of surface-immobilized Protein G B1, a rigid 6 kDa domain that binds the Fc fragment of IgG. Two Protein G B1 variants with a single cysteine introduced at either end were immobilized via the cysteine thiol onto maleimide-oligo(ethylene glycol)-functionalized gold and bare gold substrates. X-ray photoelectron spectroscopy was used to measure the amount of immobilized protein, and ToF-SIMS was used to measure the amino acid composition of the exposed surface of the protein films and to confirm covalent attachment of protein thiol to the substrate maleimide groups. SFG and NEXAFS were used to characterize the ordering and orientation of peptide or side chain bonds. On both substrates and for both cysteine positions, ToF-SIMS data showed enrichment of mass peaks from amino acids located at the end of the protein opposite to the cysteine surface position as compared with nonspecifically immobilized protein, indicating end-on protein orientations. Orientation on the maleimide substrate was enhanced by increasing pH (7.0-9.5) and salt concentration (0-1.5 M NaCl). SFG spectral peaks characteristic of ordered α-helix and β-sheet elements were observed for both variants but not for cysteine-free wild type protein on the maleimide surface. The phase of the α-helix and β-sheet peaks indicated a predominantly upright orientation for both variants, consistent with an end-on protein binding configuration. Polarization dependence of the NEXAFS signal from the N 1s to π* transition of β-sheet peptide bonds also indicated protein ordering, with an estimated tilt angle of inner β-strands of 40-50° for both variants (one variant more tilted than the other), consistent with SFG results. The combined results demonstrate the power of using complementary techniques to probe protein orientation on surfaces.</p>

Topics
  • impedance spectroscopy
  • surface
  • phase
  • x-ray photoelectron spectroscopy
  • gold
  • spectrometry
  • selective ion monitoring
  • secondary ion mass spectrometry
  • vibrational spectroscopy
  • near-edge X-ray absorption fine structure spectroscopy