Redox‐dependent dynamics of putidaredoxin characterized by amide proton exchange

Abstract

Multidimensional NMR methods were used to obtain ¹H-¹⁵N correlations and ¹⁵N resonance assignments for amide and side-chain nitrogens of oxidized and reduced putidaredoxin (Pdx), the Fe₂S₂ ferredoxin, which acts as the physiological reductant of cytochrome P-450_cam (CYP101). A model for the solution structure of oxidized Pdx has been determined recently using NMR methods (Pochapsky TC, Ye XM, Ratnaswamy G, Lyons TA, 1994, Biochemistry 53:6424–6432) and redox-dependent ¹H NMR spectral features have been described (Pochapsky TC, Ratnaswamy G, Patera A, 1994, Biochemistry 55:6433–6441). ¹⁵N assignments were made with NOESY-(¹H/¹⁵N) HMQC and TOCSY-(¹H/¹⁵N) HSQC spectra obtained using samples of Pdx uniformly labeled with ¹⁵N. Local dynamics in both oxidation states of Pdx were then characterized by comparison of residue-specific amide proton exchange rates, which were measured by a combination of saturation transfer and H₂O/D₂O exchange methods at pH 6.4 and 7.4 (uncorrected for isotope effects). In general, where exchange rates for a given site exhibit significant oxidation-state dependence, the oxidized protein exchanges more rapidly than the reduced protein. The largest dependence of exchange rate upon oxidation state is found for residues near the metal center and in a region of compact structure that includes the loop-turn Val 74-Ser 82 and the C-terminal residues (Pro 102-Trp 106). The significance of these findings is discussed in light of the considerable dependence of the binding interaction between Pdx and CYP101 upon the oxidation state of Pdx.