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Predicted secondary structure of bovine prothrombin fragment 1 and related proteins in different environments by circular dichroism spectroscopy.
Balbes, L M; Pedersen, L G; Hiskey, R G.
Affiliation
  • Balbes LM; Department of Chemistry, University of North Carolina, Chapel Hill.
Int J Pept Protein Res ; 40(2): 127-33, 1992 Aug.
Article in En | MEDLINE | ID: mdl-1446970
ABSTRACT
Circular dichroism spectroscopy was used to investigate the structure of bovine prothrombin fragment 1 (BF1) and related proteins in several environments. The conformational change induced in BF1 by the addition of Mg[II] ions was found to be different from that induced by Ca[II] or Sr[II]. The Ca[II] and Sr[II] conformations appear to differ only slightly from the apo-metal conformation. The conformation of the 1-45 fragment of prothrombin, however, is markedly different than the conformation of the same fragment in the presence of either Ca[II] of Mg[II]; both of the latter structures differ substantially from one another. The presence of phospholipids has almost no effect on the structure of either BF1 or the 1-45 fragment; in the presence of both phospholipids and Ca[II] a structural change is seen for the 1-45 fragment but not BF1 (relative to the protein alone). The addition of phospholipids to the Mg[II]/BF1 structure did not induce a CD-detectable conformational change, while the addition of phospholipids to the Ca[II]/BF1 or Sr[II]/BF1 structures induced a change to a conformation similar in secondary structure composition to the relative apometal structures.
Subject(s)
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Collection: 01-internacional Database: MEDLINE Main subject: Peptide Fragments / Protein Precursors / Prothrombin Type of study: Prognostic_studies / Risk_factors_studies Limits: Animals Language: En Journal: Int J Pept Protein Res Year: 1992 Document type: Article
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Collection: 01-internacional Database: MEDLINE Main subject: Peptide Fragments / Protein Precursors / Prothrombin Type of study: Prognostic_studies / Risk_factors_studies Limits: Animals Language: En Journal: Int J Pept Protein Res Year: 1992 Document type: Article