Solution structure of leukemia inhibitory factor
Details
Publication Year 1998-05-29,Volume 273,Issue #22,Page 13738-13745
Journal Title
JOURNAL OF BIOLOGICAL CHEMISTRY
Publication Type
Journal Article
Abstract
The solution structure of a murine-human chimera of leukemia inhibitory factor (LIF), a 180-residue cytokine with a molecular mass of 20 kDa, has been determined using multidimensional heteronuclear NMR techniques, The protein contains four alpha-helices, the relative orientations of which are well defined on the basis of long-range range interhelical nuclear Overhauser effects. The helices are arranged in an up-up-down-down orientation, as found in other four-helix bundle cytokines, and the overall topology of the chimera is similar to that of the crystal structure of murine LIF (Robinson, R. C., Grey, L. M., Staunton, D,, Vankelecom, H. Vernallis, A. B., Moreau, J. F,, Stuart, D, I., Heath, J, K., and Jones, E, Y, (1994) Cell 77, 1101-1116), Differences between the structures are evident in the N-terminal region, where the peptide bond preceding pro(17) has a trans-conformation in solution but a cis-conformation in the crystal, and in the small antiparallel beta-sheet encompassing residues in the N terminus and the CD loop in the crystal structure, which is not apparent in solution. There are also minor differences in the extent of the helices. Other than at the N terminus, the main difference between the two structures occurs at the C-terminal end of the CD loop. As this loop is close to a receptor-binding site on LIF that makes a major contribution to high affinity binding to the LIF receptor alpha-chain, these differences between the solution and crystal structures should be taken into account in structural models of LIF receptor interactions.
Publisher
AMER SOC BIOCHEMISTRY MOLECULAR BIOLOGY INC
Keywords
CILIARY NEUROTROPHIC FACTOR; COUPLING-CONSTANTS; RECEPTOR-BINDING; CRYSTAL-STRUCTURE; LARGER PROTEINS; GROWTH-FACTORS; FACTOR LIF; MURINE; EXPRESSION; CYTOKINES
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Creation Date: 1998-05-29 12:00:00
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