Raman Analysis of Cysteine Thiols in Proteins

Stephen W. Raso
(in collaboration with Prof. George J. Thomas, Jr., University of Missouri-Kansas City)

Many proteins contain cysteine residues which are not involved in active sites, ligand binding or disulfide bonds. S-H stretching vibrations generate characteristic Raman bands, which are highly dependent on the environment of the sulfhydryl proton, and represent a valuable method for examining S-H interactions under physiological conditions (1). For the trimeric tailspike protein from bacteriophage P22, all eight cysteine residues (per monomer) are reduced in the native trimer, yet a subset facilitates proper subunit folding and assembly (2). Raman spectroscopy of the tailspike resolves the S-H region of the spectrum into multiple bands, indicating sulfhydryls in several environments (Fig. 1).

Some of the tailspike S-H bands are at extremely low wavenumbers; the band corresponding to one S-H vibration is at 2530 cm-1, a frequency lower than any reported previously. The complex band pattern in this region is diagnostic of the native folded tailspike protein. The Raman spectra of eight Cys to Ser mutant proteins have been analyzed permitting the identification of the specific contribution from each cysteine sulfhydryl to the various S-H bands (Fig. 2).

Cysteine Thiol to Tailspike Raman Spectrum

In addition, the hydrogen bonding environment of each of the eight tailspike cysteines was elucidated (Table 1). Raman spectroscopy provides H-bonding information about the native solution-state of a protein, unlike X-ray crystallographic methods wherein H-bonding interactions are inferred by the interatomic distances of potential H-bond donors and acceptors in the crystalline state.

Table 1: H-bonding Environment of Each Tailspike Cysteine Thiol

Cysteine Residue

Raman band (cm-1)

Proposed H-bonding Strength

169

2565

Moderately Strong

267

2550 (90%)
2585 (10%)

Strong
Weak/Acceptor

287

2550 (63%)
2585 (37%)

Strong
Weak/Acceptor

290

2585

Weak/Acceptor

458

2550

Strong

496

2585

Weak/Acceptor

a613

2530

Very Strong

635

2576

Moderately Weak

aThe 2530 cm-1 Raman marker of Cys 613 represents the strongest S-H--X hydrogen bond observed for a cysteine or model thiol in solution.

These techniques can be applied to other proteins to study the specific roles cysteine residues in protein structure and function. In addition, S-H Raman markers may be used to probe changes in protein conformation and cysteine oxidation.

 

References

1. Li, H. & Thomas, G.J., Jr. (1991) J. Am. Chem. Soc. 113, 456-462.

2. Robinson, A.S. & King, J. (1997) Nature Struct. Biol. 4, 450-455.