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Home / Equine Research Bank / Biophys Chem / Helix-rich transient and equilibrium intermediates of equine...
Biophysical chemistry2008; 134(1-2); 84-92; doi: 10.1016/j.bpc.2008.01.010

Helix-rich transient and equilibrium intermediates of equine beta-lactoglobulin in alkaline buffer.

Abstract: Acidic buffer conditions are known to stabilize helix-rich states of even those proteins with a predominantly beta-sheet native secondary structure. Here we investigated whether such states also exist under alkaline buffer conditions. The guanidine hydrochloride (GuHCl)-induced unfolding transition and kinetic refolding of equine beta-lactoglobulin (ELG) by GuHCl-jump were investigated at pH 8.7 by far-ultraviolet circular dichroism. We found that an equilibrium intermediate appeared in 45% ethylene glycol (EGOH) buffer with 1.5 M GuHCl. The intermediate is rich in non-native alpha-helix, which is similar to the helix-rich state of ELG at pH 4.0. A kinetic study was done on the folding rate of ELG and compared with bovine beta-lactoglobulin (BLG). Transient intermediates, which were observed as the burst phase of the refolding reaction, were also rich in alpha-helix. The activation enthalpy of ELG was calculated to be c.a. 80 kJ/mol, whereas that of BLG was c.a. 70 kJ/mol in the presence of 45% EGOH. The ellipticities of the transient intermediate of ELG show temperature dependence in the presence of 45% EGOH, whereas that of BLG did not show significant dependence. This study therefore extends the existence of helix-rich equilibrium and transient intermediates of predominantly beta-sheet proteins to alkaline buffer conditions.
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Publication Date: 2008-02-13 PubMed ID: 18295961DOI: 10.1016/j.bpc.2008.01.010Google Scholar: Lookup
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Summary

This research summary has been generated with artificial intelligence and may contain errors and omissions. Refer to the original study to confirm details provided. Submit correction.

The research examines whether proteins, primarily composed of a beta-sheet native structure, can maintain helix-rich states in alkaline buffer conditions. Results indicate that an equilibrium intermediate rich in non-native alpha-helix was present and that helix-rich equilibrium and transient intermediates in predominantly beta-sheet proteins can exist in alkaline buffer conditions.

Understanding Beta-Sheet and Alpha-Helix Protein Structures

  • The study revolves around proteins and their secondary structures. Proteins have two common secondary structures, alpha-helix and beta-sheet.
  • In an alpha-helix protein, the polypeptide chain is twisted into a right-handed coil or helix. In contrast, a beta-sheet is composed of beta strands connected laterally by at least two or three backbone hydrogen bonds, forming a twisted, pleated sheet.
  • This research seems to challenge the belief that helix-rich states are only possible under acidic buffer conditions, even for proteins with a predominantly beta-sheet native secondary structure.

Experimental Approach to the Research

  • The acid buffer conditions were replaced with alkaline buffer conditions during this experimental process. The study used equine beta-lactoglobulin (ELG) for the investigations.
  • The researchers employed far-ultraviolet circular dichroism to monitor GuHCl-induced unfolding transition and kinetic refolding of ELG at the slightly alkaline pH of 8.7.
  • The folding rate of ELG was also studied and compared with that of bovine beta-lactoglobulin (BLG).

Findings of the Study

  • The study found that an equilibrium intermediate appeared in a buffer containing 45% ethylene glycol (EGOH) and 1.5 M GuHCl. This intermediate was discovered to be rich in non-native alpha-helix, similar to the helix-rich state of ELG at pH 4.0, demonstrating that helix-rich states can also exist under alkaline conditions.
  • The study discovered that transient intermediates, observed as the initial (‘burst’) phase of the refolding reaction, were also rich in alpha-helix. The activation enthalpy of ELG, a measure of the energy involved in the process, was calculated to be approximately 80 kJ/mol.
  • The ellipticities (a measure of the change in polarization of light due to the protein structure) of the transient intermediate of ELG showed temperature dependence in the presence of 45% EGOH, indicating a change in protein structure with temperature.

Implications of the Findings

  • This study is significant as it extends the understanding of the existence of helix-rich equilibrium and transient intermediates of predominantly beta-sheet proteins to alkaline buffer conditions. This could have implications for protein engineering and biotechnological applications where control over protein structures is critically important.

Cite This Article

APA
Matsumura Y, Li J, Ikeguchi M, Kihara H. (2008). Helix-rich transient and equilibrium intermediates of equine beta-lactoglobulin in alkaline buffer. Biophys Chem, 134(1-2), 84-92. https://doi.org/10.1016/j.bpc.2008.01.010

Publication

Biophysical chemistry
ISSN: 0301-4622
NlmUniqueID: 0403171
Country: Netherlands
Language: English
Volume: 134
Issue: 1-2
Pages: 84-92

Researcher Affiliations

Matsumura, Yoshitaka
  • Department of Physics, Kansai Medical University, 18-89 Uyama-Higashi, Hirakata 573-1136, Japan.
Li, Jinsong
    Ikeguchi, Masamichi
      Kihara, Hiroshi

        MeSH Terms

        • Animals
        • Buffers
        • Ethylene Glycol / pharmacology
        • Guanidine / pharmacology
        • Horses
        • Hydrogen-Ion Concentration
        • Kinetics
        • Lactoglobulins / chemistry
        • Lactoglobulins / metabolism
        • Protein Denaturation / drug effects
        • Protein Renaturation / drug effects
        • Protein Structure, Secondary / drug effects
        • Temperature
        • Thermodynamics

        Citations

        This article has been cited 3 times.
        1. Qin ZJ, Shimizu A, Li J, Ikeguchi M, Shinjo M, Kihara H. α-helix formation rate of oligopeptides at subzero temperatures. Biophysics (Nagoya-shi) 2014;10:9-13.
          doi: 10.2142/biophysics.10.9pubmed: 27493493google scholar: lookup
        2. Matsumura Y, Shinjo M, Kim SJ, Okishio N, Gruebele M, Kihara H. Transient helical structure during PI3K and Fyn SH3 domain folding. J Phys Chem B 2013 May 2;117(17):4836-43.
          doi: 10.1021/jp400167spubmed: 23537292google scholar: lookup
        3. Matsumura Y, Shinjo M, Matsui T, Ichimura K, Song J, Kihara H. Structural study of hNck2 SH3 domain protein in solution by circular dichroism and X-ray solution scattering. Biophys Chem 2013 May-Jun;175-176:39-46.
          doi: 10.1016/j.bpc.2013.02.005pubmed: 23524290google scholar: lookup
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