Abstract
The sulfur isotope record provides key insight into the history of Earth's redox conditions. A detailed understanding of the metabolisms driving this cycle, and specifically microbial sulfate reduction (MSR), is crucial for accurate paleoenvironmental reconstructions. This includes a precise knowledge of the step-specific sulfur isotope effects during MSR. In this study, we aim at resolving the cellular-level fractionation factor during dissimilatory sulfite reduction to sulfide within MSR, and use this measured isotope effect as a calibration to enhance our understanding of the biochemistry of sulfite reduction. For this, we merge measured isotope effects associated with dissimilatory sulfite reduction with a quantitative model that explicitly links net fractionation, reaction reversibility, and intracellular metabolite levels. The highly targeted experimental aspect of this study was possible by virtue of the availability of a deletion mutant strain of the model sulfate reducer Desulfovibrio vulgaris (strain Hildenborough), in which the sulfite reduction step is isolated from the rest of the metabolic pathway owing to the absence of its QmoABC complex (ΔQmo). This deletion disrupts electron flux and prevents the reduction of adenosine phosphosulfate (APS) to sulfite. When grown in open-system steady-state conditions at 10% maximum growth rate in the presence of sulfite and lactate as electron donor, sulfur isotope fractionation factors averaged −15.9‰ (1 σ = 0.4), which appeared to be statistically indistinguishable from a pure enzyme study with dissimilatory sulfite reductase. We coupled these measurements with an understanding of step-specific equilibrium and kinetic isotope effects, and furthered our mechanistic understanding of the biochemistry of sulfite uptake and ensuing reduction. Our metabolically informed isotope model identifies flavodoxin as the most likely electron carrier performing the transfer of electrons to dissimilatory sulfite reductase. This is in line with previous work on metabolic strategies adopted by sulfate reducers under different energy regimes, and has implications for our understanding of the plasticity of this metabolic pathway at the center of our interpretation of modern and palaeo-environmental records.
Highlights
The sulfur (S) isotopic composition of marine sedimentary sulfates (SO24−) and sulfides (H2S) encodes a composite of chemical and biological information on Earth’s past sedimentary environments (Canfield, 2004)
We present results from a series of chemostat experiments run at 10% of maximum growth rate, chosen to assess conditions close to the upper limit of this cellular-scale isotope effect
We explore the intrinsic isotope effects associated with sulfite reduction, reaction reversibility, and the degree to which isotopic equilibrium influences net cellular fractionation
Summary
The sulfur (S) isotopic composition of marine sedimentary sulfates (SO24−) and sulfides (H2S) encodes a composite of chemical and biological information on Earth’s past sedimentary environments (Canfield, 2004) This record has been used extensively to identify major secular changes in Earth’s surface conditions, including the initial rise of atmospheric oxygen (Farquhar et al, 2000; Habicht et al, 2002; Bekker et al, 2004), the Precambrian origin of different microbial metabolisms (Canfield, 1998; Johnston et al, 2005), and the onset of bioturbation in the early Paleozoic Era (Canfield and Farquhar, 2009; Tarhan et al, 2015). The ultimate product of this metabolism is sulfide, as shown below in the reaction network 1
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