posted on 2017-07-14, 13:02authored byJaswir Basran, Elizabeth S. Booth, Michael Lee, Sandeep Handa, Emma L. Raven
Indoleamine 2,3-dioxygenase (IDO) and tryptophan 2,3-dioxygenase (TDO) are heme-containing enzymes that catalyze the O2-dependent oxidation of l-tryptophan (l-Trp) in biological systems. Although many decades have passed since their discovery, the mechanism of tryptophan oxidation has not been established. It has been widely assumed that IDO and TDO react using the same mechanism, although there is no evidence that they do. For IDO, a Compound II (ferryl) species accumulates in the steady state and is implicated in the mechanism; in TDO, no such species has ever been observed. In this paper, we examine the kinetics of tryptophan oxidation in TDO. We find no evidence for the accumulation of Compound II during TDO catalysis. Instead, a ternary [Fe(II)-O2, l-Trp] complex is detected under steady state conditions. The absence of a Compound II species in the steady state in TDO is not due to an intrinsic inability of the TDO enzyme to form ferryl heme, because Compound II can be formed directly through a different route in which ferrous heme is reacted with peroxide. We interpret the data to mean that the rate-limiting step in the IDO and TDO mechanisms is not the same.
Funding
This work was supported by grants from EPSRC (studentship to E.S.B.) and BBSRC (BB/L004585/1, fellowship to E.L.R.).
History
Citation
Biochemistry, 2016, 55 (49), pp. 6743-6750
Author affiliation
/Organisation/COLLEGE OF MEDICINE, BIOLOGICAL SCIENCES AND PSYCHOLOGY/MBSP Non-Medical Departments/Molecular & Cell Biology
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ACS Publications website at DOI: 10.1021/acs.biochem.6b01005.
Reactivity of XcTDO with O2 (Figure S1), formation of
the [Fe(II)−O2, L-Trp] ternary complex in TDOs
(Figure S2), oxidation of 5-fluoro-Trp by ferrous
XcTDO (Figure S3), and formation of Compound II
in TDO in the presence of substrate (Figure S4) (PDF)