Stephen W. Ragsdale
University of Wisconsin–Milwaukee
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Critical Reviews in Biochemistry and Molecular Biology | 1991
Stephen W. Ragsdale
We know of three routes that organisms have evolved to synthesize complex organic molecules from CO2: the Calvin cycle, the reverse tricarboxylic acid cycle, and the reductive acetyl-CoA pathway. This review describes the enzymatic steps involved in the acetyl-CoA pathway, also called the Wood pathway, which is the major mechanism of CO2 fixation under anaerobic conditions. The acetyl-CoA pathway is also able to form acetyl-CoA from carbon monoxide. There are two parts to the acetyl-CoA pathway: (1) reduction of CO2 to methyltetrahydrofolate (methyl-H4folate) and (2) synthesis of acetyl-CoA from methyl-H4folate, a carboxyl donor such as CO or CO2, and CoA. This pathway is unique in that the major intermediates are enzyme-bound and are often organometallic complexes. Our current understanding of the pathway is based on radioactive and stable isotope tracer studies, purification of the component enzymes (some extremely oxygen sensitive), and identification of the enzyme-bound intermediates by chromatographic, spectroscopic, and electrochemical techniques. This review describes the remarkable series of enzymatic steps involved in acetyl-CoA formation by this pathway that is a key component of the global carbon cycle.
Analytical Biochemistry | 1989
Scott R. Harder; Benjamin A. Feinberg; Stephen W. Ragsdale
In this paper we describe an anaerobic titrator made virtually from glass with a small amount of high vacuum epoxy mounted directly to a quartz EPR tube. A complete titration may be carried out with as little as 600 microliters of sample. This cell features the anaerobic manipulation of an electrochemically poised solution from an electrochemical pouch to an EPR tube. The cell uses a gold foil working electrode and Ag/AgCl reference and counter electrodes. The reference and counter electrodes are isolated from the sample by leached Vycor glass. In the work reported here, we used this cell to determine the equilibrium redox potential of methyl viologen in an EPR titration. With methyl viologen as an indicator we found that the cell has a residual oxygen level of 1.5 microM with a leak rate of 0.005 nmol/min. After moving the solution into the EPR tube, freezing, performing EPR, and thawing, the potential of the methyl viologen solution drifted only 2 mV. During the titration, the poised potentials were stable, drifting only 1 mV/min. Formal potentials as low as -630 mV in a vitamin B12-type protein have been determined with this cell (S. R. Harder, W.-P. Lu, B. A. Feinberg, and S. W. Ragsdale (1989) Biochemistry, in press).
Biochemistry | 1990
Ruma Banerjee; Scott R. Harder; Stephen W. Ragsdale; Rowena G. Matthews
Journal of Biological Chemistry | 1987
Stephen W. Ragsdale; P A Lindahl; E Münck
Journal of Biological Chemistry | 1990
Paul A. Lindahl; E. Münck; Stephen W. Ragsdale
Journal of Biological Chemistry | 1990
Wei-Ping Lu; S. R. Harder; Stephen W. Ragsdale
Proceedings of the National Academy of Sciences of the United States of America | 1989
D L Roberts; J E James-Hagstrom; Denise K. Garvin; C M Gorst; J A Runquist; J R Baur; F C Haase; Stephen W. Ragsdale
Journal of Biological Chemistry | 1990
Paul A. Lindahl; Stephen W. Ragsdale; E. Münck
Biochemistry | 1989
Scott R. Harder; Wei Ping Lu; Benjamin A. Feinberg; Stephen W. Ragsdale
Journal of Biological Chemistry | 1991
Wai-Ping Lu; Stephen W. Ragsdale