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Primary Structure Effects on Peptide Group Hydrogen Exchange

Yawen Bai, +3 more
- 01 Sep 1993 - 
- Vol. 17, Iss: 1, pp 75-86
TLDR
The results provide the information necessary to evaluate measured protein NH to ND exchange rates by comparing them with rates to be expected for the same amino acid sequence is unstructured aligo‐ and polypeptides.
Abstract
The rate of exchange of peptide group NH hydrogens with the hydrogens of aqueous solvent is sensitive to neighboring side chains. To evaluate the effects of protein side chains, all 20 naturally occurring amino acids were studied using dipeptide models. Both inductive and steric blocking effects are apparent. The additivity of nearest-neighbor blocking and inductive effects was tested in oligo- and polypeptides and, surprisingly, confirmed. Reference rates for alanine-containing peptides were determined and effects of temperature considered. These results provide the information necessary to evaluate measured protein NH to ND exchange rates by comparing them with rates to be expected for the same amino acid sequence is unstructured oligo- and polypeptides. The application of this approach to protein studies is discussed.

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Journal ArticleDOI

Ligand binding promiscuity of human liver fatty acid binding protein: structural and dynamic insights from an interaction study with glycocholate and oleate.

TL;DR: A thorough NMR investigation of glycocholate (GCA) binding to human liver fatty acid binding protein found GCA was found to occupy the large internal cavity of hL‐FABP, without requiring major conformational rearrangement of the protein backbone; rather, this led to increased stability, similar to that estimated for the hL-FABp:oleate complex.
Patent

Method for characterization of the fine structure of protein binding sites

TL;DR: The binding sites of binding proteins and their binding partners are characterized at the individual amino acid level by a combination of heavy hydrogen (tritium or deuterium) exchange labeling and sequential degradation (preferably, by carboxypeptidase) and analysis of labeled fragments under slowed exchange conditions as mentioned in this paper.
Journal ArticleDOI

NMR Structure of the SARS-CoV Nonstructural Protein 7 in Solution at pH 6.5.

TL;DR: Data on conformational equilibria and intramolecular rate processes in nsp7 in solution at pH 6.5, which provide further insights into the polymorphisms implicated by a comparison of the three presently available nSp7 structures, are included.
Journal ArticleDOI

Protein vivisection reveals elusive intermediates in folding

TL;DR: A buried aliphatic residue is substituted with a charged residue to destabilize and unfold a specific region of the protein, reversibly trapping a folding intermediate in which the beta5-strand is unfolded.
References
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Journal ArticleDOI

MLEV-17-based two-dimensional homonuclear magnetization transfer spectroscopy

TL;DR: In this article, a new mixing scheme based on the MLEV-16 composite pulse decoupling cycle (II) was proposed, which is less sensitive to pulse imperfections and provides net magnetization transfer over a substantial bandwidth with only limited rf power.
Journal ArticleDOI

Use of glass electrodes to measure acidities in deuterium oxide1,2

TL;DR: In this article, a pH meter reading in D/sub 2/O solutions was 0-40 pH unit lower than in H/sub O solutions, attributed to the glass electrode.
Journal ArticleDOI

Dithiothreitol, a New Protective Reagent for SH Groups*

W. Wallace Cleland
- 01 Apr 1964 - 
TL;DR: Strominger, J. L. H. (1960), Instruction Manual and Handbook, Beckman/Spinco Model 120 Amino Acid Analyzer, Palo Alto, California,Beckman Instruments Inc., Spinco Division.
Journal ArticleDOI

A two-dimensional nuclear overhauser enhancement (2d noe) experiment for the elucidation of complete proton-proton cross-relaxation networks in biological macromolecules

TL;DR: The 2D NOE experiment has the principal advantage that it avoids detrimental effects arising from the limited selectivity of preirradiation in crowded spectral regions, and yields with a single instrument setting a complete network of NOE's between all the protons in the macromolecule.
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