Recombinant human IL-6 expressed inE. coli undergoes selective N-terminal degradation: Evidence that the protein consists of a stable core and a nonessential flexible N-terminal |
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| Authors: | Amanda E I Proudfoot Steven C Brown Alain R Bernard Jean-Yves Bonnefoy Eric H Kawashima |
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| Institution: | 1. Glaxo Institute for Molecular Biology S.A., 1228 Plan-les Ouates, Geneva, Switzerland
2. Glaxo Research Institute, Research Triangle Park, 27709, North Carolina
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| Abstract: | A synthetic gene for human interleukin-6 has been expressed inE. coli. The protein has been purified and renatured and has the same activity as natural human IL-6 using the 7TD1 cell proliferation assay. The protein undergoes specific cleavage by a thiol protease, yielding two new N-termini at Arg-9 and His-15. The truncated proteins retain full biological activity. The degradation results in the loss of sharp amide resonances in the1H-NMR spectrum, and little change to the ultraviolet CD spectrum. Several amino acid type assignments could be made for these sharp amides using a DQF-COSY 2D-NMR experiment. The N-terminal 15 amino acids exist as a flexible, random coil, attached to a central structure. |
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