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Design, synthesis, and conformational studies of the hGM-CSF derived peptide (13-27)-Gly-(75-87).

作者信息

Peggion E, Mammi S, Schievano E, Revoltella R P, Galoppini C, Rovero P

机构信息

University of Padova, Department of Organic Chemistry, Biopolymers Research Center, CNR, Via Marzolo 1, 35131 Padova, Italy.

出版信息

Biopolymers. 1999 Oct 15;50(5):545-54. doi: 10.1002/(SICI)1097-0282(19991015)50:5<545::AID-BIP8>3.0.CO;2-0.

DOI:10.1002/(SICI)1097-0282(19991015)50:5<545::AID-BIP8>3.0.CO;2-0
PMID:10479737
Abstract

An analogue of the human granulocyte-macrophage colony-stimulating factor (hGM-CSF), hGM-CSF(13-27)-Gly-(75-87) was synthesized by solid phase methodology. This analogue was designed to comprise helices A and C of the native growth factor, linked by a glycine bridge. Helices A and C form half of a four-helix bundle motif in the crystal structure of the native factor and are involved in the interaction with alpha- and beta-chains of the heterodimeric receptor. A conformational analysis of the synthetic analogue by CD, two-dimensional nmr spectroscopy, and molecular dynamics calculations is reported. The analogue is in a random structure in water and assumes a partially alpha-helical conformation in a 1 : 1 trifluoroethanol/water mixture. The helix content in this medium is approximately 70%. By 2D-nmr spectroscopy, two helical segments were identified in the sequences corresponding to helices A and C. In addition to medium- and short-range NOESY connectivities, a long-range cross peak was found between the Cbeta proton of Val(16) and NH proton of His(87) (using the numbering of the native protein). Experimentally derived interproton distances were used as restraints in molecular dynamics calculations, utilizing the x-ray coordinates as the initial structure. The final structure is characterized by two helical segments in close spatial proximity, connected by a loop region. This structure is similar to that of the corresponding domain in the x-ray structure of the native growth factor in which helices A and C are oriented in an antiparallel fashion. The N-terminal residues Gly-Pro of helix C are involved in an irregular turn connecting the two helical segments. As a consequence, helix C is appreciably shifted and slightly rotated with respect to helix A compared to the x-ray structure of the native growth factor. These small differences in the topology of the two helices could explain the lower biological activity of this analogue with respect to that of the native growth factor.

摘要

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