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nmrlearner 11-19-2010 08:29 PM

Cooperativity of a protein folding reaction probed at multiple chain positions by rea
 
Cooperativity of a protein folding reaction probed at multiple chain positions by real-time 2D NMR spectroscopy.

Related Articles Cooperativity of a protein folding reaction probed at multiple chain positions by real-time 2D NMR spectroscopy.

Biochemistry. 2000 Jul 11;39(27):7910-9

Authors: Steegborn C, Schneider-Hassloff H, Zeeb M, Balbach J

The refolding reaction of S54G/P55N ribonuclease T1 is a two-step process, where fast formation of a partly folded intermediate is followed by the slow reaction to the native state, limited by a trans --> cis isomerization of Pro39. The hydrodynamic radius of this kinetic folding intermediate was determined by real-time diffusion NMR spectroscopy. Its folding to the native state was monitored by a series of 128 very fast 2D (15)N-HMQC spectra, to observe the kinetics of 66 individual backbone amide probes. We find that the intermediate is as compact as the native protein with many native chemical shifts. All 66 analyzed amide probes follow the rate-limiting prolyl isomerization, which indicates that this cooperative refolding reaction is fully synchronized. The stability of the folding intermediate was determined from the protection factors of 45 amide protons derived from a competition between refolding and H/D exchange. The intermediate has already gained 40% of the Gibbs free energy of refolding with many protected amides in not-yet-native regions.

PMID: 10891071 [PubMed - indexed for MEDLINE]



Source: PubMed


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