Single-well push-pull tests evaluating isobutane as a primary substrate for promoting in situ cometabolic biotransformation reactions.

A series of single-well push-pull tests (SWPPTs) were performed to investigate the efficacy of isobutane (2-methylpropane) as a primary substrate for in situ stimulation of microorganisms able to cometabolically transform common groundwater contaminants, such as chlorinated aliphatic hydrocarbons and 1,4-dioxane (1,4-D). In biostimulation tests, the disappearance of isobutane relative to a nonreactive bromide tracer indicated an isobutane-utilizing microbial community rapidly developed in the aquifer around the test well. SWPPTs were performed as natural drift tests with first-order rates of isobutane consumption ranging from 0.4 to 1.4 day-1. Because groundwater contaminants were not present at the demonstration site, isobutene (2-methylpropene) was used as a nontoxic surrogate to demonstrate cometabolic activity in the subsurface after biostimulation. The transformation of isobutene to isobutene epoxide (2-methyl-1,2-epoxypropane) illustrates the epoxidation process previously shown for common groundwater contaminants after cometabolic transformation by alkane-utilizing bacteria. The rate and extent of isobutene consumption and the formation and transformation of isobutene epoxide were greater in the presence of isobutane, with no evidence of primary substrate inhibition. Modeled concentrations of isobutane-utilizing biomass in microcosms constructed with groundwater collected before and after each SWPPT offered additional evidence that the isobutane-utilizing microbial community was stimulated in the aquifer. Experiments in groundwater microcosms also demonstrated that the isobutane-utilizing bacteria stimulated in the subsurface could cometabolically transform a mixture of co-substrates including isobutene, 1,1-dichloroethene, cis-1,2-dichloroethene, and 1,4-D with the same co-substrate preferences as the bacterium Rhodococcus rhodochrous ATCC strain 21198 after growth on isobutane. This study demonstrated the effectiveness of isobutane as primary substrate for stimulating in situ cometabolic activity and the use of isobutene as surrogate to investigate in situ cometabolic reactions catalyzed by isobutane-stimulated bacteria.

Aerobic cometabolism of 1,4-dioxane by isobutane-utilizing microorganisms including Rhodococcus rhodochrous strain 21198 in aquifer microcosms: Experimental and modeling study.

Aerobic cometabolism of the emerging contaminant 1,4-dioxane (1,4-D) by isobutane-utilizing microorganisms was assessed in pure culture and aquifer microcosm studies. The bacterium Rhodococcus rhodochrous strain ATCC 21198 transformed low, environmentally-relevant concentrations of 1,4-D when grown on isobutane. Microcosms were constructed with aquifer solids from Fort Carson, Colorado, a site contaminated with 1,4-D and trichloroethene (TCE). Multiple additions of isobutane and 1,4-D over 300 days were transformed in microcosms biostimulated with isobutane and microcosms bioaugmented with strain 21198. Results showed that, over time and with sufficient inorganic nutrients, biostimulation of native microorganisms with isobutane was just as effective as bioaugmentation with strain 21198 to achieve 1,4-D transformation in the microcosms. The presence of TCE at 0.2 mg/L did not inhibit 1,4-D transformation, though TCE itself was not readily transformed. An iterative process was used to determine kinetic parameter values to fit Michaelis-Menten/Monod models to experimental data for simultaneous isobutane utilization, biomass growth, and cometabolic transformation of 1,4-D. Parameter optimization resulted in good model fit to the data over multiple transformations of isobutane and 1,4-D in both short- and long-term experiments. Results suggest low concentrations of 1,4-D studied in the microcosms were cometabolically transformed according to a pseudo first-order rate of 0.37 L/mg TSS/day of 21198. Isobutane consumption was modeled with a maximum rate of 2.58 mg/mg TSS/day and a half saturation constant of 0.09 mg/L. 1,4-D transformation was competitively inhibited by the presence of isobutane and transformation rates were significantly reduced when inorganic nutrients were limiting. Simulations of the repeated additions found a first-order microbial endogenous decay coefficient of 0.03 day-1 fit the alternating periods of active transformation and stagnation between isobutane and 1,4-D additions over approximately one year. The model fitting process highlighted the importance of determining kinetic parameters from data representing low concentrations typically found in the environment.