Difference between revisions of "Biodegradation - 1,4-Dioxane"
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*[[1,4-Dioxane]] | *[[1,4-Dioxane]] | ||
*[[Biodegradation - Cometabolic]] | *[[Biodegradation - Cometabolic]] | ||
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'''Contributor(s):''' [[Dr. Shaily Mahendra]] and [[Dr. Michael Hyman]] | '''Contributor(s):''' [[Dr. Shaily Mahendra]] and [[Dr. Michael Hyman]] | ||
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'''Key Resource(s)''': | '''Key Resource(s)''': | ||
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| ''Pseudonocardia dioxanivorans'' CB1190 || THFMO || 0.19 ± 0.007 mg/hr/mg-protein || Mahendra and Alvarez-Cohen (2005, 2006)<ref name= "Mahendra2005">Mahendra, S. and Alvarez-Cohen, L., 2005. Pseudonocardia dioxanivorans sp. nov., a novel actinomycete that grows on 1, 4-dioxane. International Journal of Systematic and Evolutionary Microbiology, 55(2), pp.593-598. [https://doi.org/10.1099/ijs.0.63085-0 doi: 10.1099/ijs.0.63085-0]</ref><ref name= "Mahendra2006"/> | | ''Pseudonocardia dioxanivorans'' CB1190 || THFMO || 0.19 ± 0.007 mg/hr/mg-protein || Mahendra and Alvarez-Cohen (2005, 2006)<ref name= "Mahendra2005">Mahendra, S. and Alvarez-Cohen, L., 2005. Pseudonocardia dioxanivorans sp. nov., a novel actinomycete that grows on 1, 4-dioxane. International Journal of Systematic and Evolutionary Microbiology, 55(2), pp.593-598. [https://doi.org/10.1099/ijs.0.63085-0 doi: 10.1099/ijs.0.63085-0]</ref><ref name= "Mahendra2006"/> | ||
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− | | ''Actinomycete'' CB1190* || N/A || 0.33 mg/min/mg-protein || Parales et al. (1994)<ref name= "Parales1994">Parales, R.E., Adamus, J.E., White, N. and May, H.D., 1994. Degradation of 1, 4-dioxane by an actinomycete in pure culture. Applied and Environmental Microbiology, 60(12), pp.4527-4530. [https://doi.org/10.1128/aem.60.12.4527-4530.1994 doi:10.1128/aem.60.12.4527-4530.1994] [[media:1994-Parales-Degradation_of_1%2C4-Dioxane_by_an_Actinomycete_in_Pure_Culture.pdf| Article | + | | ''Actinomycete'' CB1190* || N/A || 0.33 mg/min/mg-protein || Parales et al. (1994)<ref name= "Parales1994">Parales, R.E., Adamus, J.E., White, N. and May, H.D., 1994. Degradation of 1, 4-dioxane by an actinomycete in pure culture. Applied and Environmental Microbiology, 60(12), pp.4527-4530. [https://doi.org/10.1128/aem.60.12.4527-4530.1994 doi:10.1128/aem.60.12.4527-4530.1994] [[media:1994-Parales-Degradation_of_1%2C4-Dioxane_by_an_Actinomycete_in_Pure_Culture.pdf| Article pdf]]</ref> |
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| ''Amycolata'' sp. CB1190* || N/A || 0.038 ± 0.012 mg/hr/mg-protein || Kelley et al. (2001) | | ''Amycolata'' sp. CB1190* || N/A || 0.038 ± 0.012 mg/hr/mg-protein || Kelley et al. (2001) | ||
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| ''Mycobacterium austroafricanum'' JOB5 || ? || 0.40 ± 0.06 mg/hr/mg-protein || House and Hyman (2010)<ref>House, A.J. and Hyman, M.R., 2010. Effects of gasoline components on MTBE and TBA cometabolism by Mycobacterium austroafricanum JOB5. Biodegradation, 21(4), pp.525-541. [https://doi.org/10.1007/s10532-009-9321-8 doi: 10.1007/s10532-009-9321-8]</ref>, Lan et al. (2013)<ref>Lan, R.S., Smith, C.A. and Hyman, M.R., 2013. Oxidation of cyclic ethers by alkane‐grown Mycobacterium vaccae JOB5. Remediation Journal, 23(4), pp.23-42. [https://doi.org/10.1002/rem.21364 doi: 10.1002/rem.21364]</ref><ref name= "Mahendra2006"/> | | ''Mycobacterium austroafricanum'' JOB5 || ? || 0.40 ± 0.06 mg/hr/mg-protein || House and Hyman (2010)<ref>House, A.J. and Hyman, M.R., 2010. Effects of gasoline components on MTBE and TBA cometabolism by Mycobacterium austroafricanum JOB5. Biodegradation, 21(4), pp.525-541. [https://doi.org/10.1007/s10532-009-9321-8 doi: 10.1007/s10532-009-9321-8]</ref>, Lan et al. (2013)<ref>Lan, R.S., Smith, C.A. and Hyman, M.R., 2013. Oxidation of cyclic ethers by alkane‐grown Mycobacterium vaccae JOB5. Remediation Journal, 23(4), pp.23-42. [https://doi.org/10.1002/rem.21364 doi: 10.1002/rem.21364]</ref><ref name= "Mahendra2006"/> | ||
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− | | ''Rhodococcus ruber'' ENV425 || ? || 10 mg/hr/g TSS || Lippincott et al. (2015)<ref name= "Lippincott2015">Lippincott, D., Streger, S.H., Schaefer, C.E., Hinkle, J., Stormo, J. and Steffan, R.J., 2015. Bioaugmentation and propane biosparging for in situ biodegradation of 1, 4‐dioxane. Groundwater Monitoring & Remediation, 35(2), pp.81-92. [https://doi.org/10.1111/gwmr.12093 doi: 10.1111/gwmr.12093]</ref>, Vainberg et al. (2006)<ref name= "Vainberg2006">Vainberg, S., McClay, K., Masuda, H., Root, D., Condee, C., Zylstra, G.J. and Steffan, R.J., 2006. Biodegradation of ether pollutants by Pseudonocardia sp. strain ENV478. Appl. Environ. Microbiol., 72(8), pp.5218-5224. [https://doi.org/10.1128/aem.00160-06 doi: 10.1128/AEM.00160-06] [[media:Vainberg2006.pdf| Article | + | | ''Rhodococcus ruber'' ENV425 || ? || 10 mg/hr/g TSS || Lippincott et al. (2015)<ref name= "Lippincott2015">Lippincott, D., Streger, S.H., Schaefer, C.E., Hinkle, J., Stormo, J. and Steffan, R.J., 2015. Bioaugmentation and propane biosparging for in situ biodegradation of 1, 4‐dioxane. Groundwater Monitoring & Remediation, 35(2), pp.81-92. [https://doi.org/10.1111/gwmr.12093 doi: 10.1111/gwmr.12093]</ref>, Vainberg et al. (2006)<ref name= "Vainberg2006">Vainberg, S., McClay, K., Masuda, H., Root, D., Condee, C., Zylstra, G.J. and Steffan, R.J., 2006. Biodegradation of ether pollutants by Pseudonocardia sp. strain ENV478. Appl. Environ. Microbiol., 72(8), pp.5218-5224. [https://doi.org/10.1128/aem.00160-06 doi: 10.1128/AEM.00160-06] [[media:Vainberg2006.pdf| Article pdf]]</ref> |
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| ''Pseudonocardia'' sp. ENV478 || THFMO || 21 mg/hr/g TSS || Masuda et al. (2012)<ref>Masuda, H., McClay, K., Steffan, R.J. and Zylstra, G.J., 2012. Biodegradation of tetrahydrofuran and 1, 4-dioxane by soluble diiron monooxygenase in Pseudonocardia sp. strain ENV478. Journal of Molecular Microbiology and Biotechnology, 22(5), pp.312-316. [https://doi.org/10.1159/000343817 doi: 10.1159/000343817]</ref>, Vainberg et al. (2006)<ref name= "Vainberg2006"/> | | ''Pseudonocardia'' sp. ENV478 || THFMO || 21 mg/hr/g TSS || Masuda et al. (2012)<ref>Masuda, H., McClay, K., Steffan, R.J. and Zylstra, G.J., 2012. Biodegradation of tetrahydrofuran and 1, 4-dioxane by soluble diiron monooxygenase in Pseudonocardia sp. strain ENV478. Journal of Molecular Microbiology and Biotechnology, 22(5), pp.312-316. [https://doi.org/10.1159/000343817 doi: 10.1159/000343817]</ref>, Vainberg et al. (2006)<ref name= "Vainberg2006"/> | ||
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| ''Aureobasidium pullmans'' NRRL 21064 || ? || 6-8 mg/L within a day || Patt and Abebe (1995)<ref name= "Patt1995">Patt, T.E. and Abebe, H.M., Upjohn Co, 1995. Microbial degradation of chemical pollutants. U.S. Patent 5,399,495. [[media:1995-Patt-Microbial_degradation_of_chemical_pollutants.pdf| Patent.pdf]]</ref> | | ''Aureobasidium pullmans'' NRRL 21064 || ? || 6-8 mg/L within a day || Patt and Abebe (1995)<ref name= "Patt1995">Patt, T.E. and Abebe, H.M., Upjohn Co, 1995. Microbial degradation of chemical pollutants. U.S. Patent 5,399,495. [[media:1995-Patt-Microbial_degradation_of_chemical_pollutants.pdf| Patent.pdf]]</ref> | ||
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− | | ''Graphium'' sp. ATCC 58400 (fungus) || CYP || 4 ± 1 nmol/min/mg dry weight (with Propane) <br/>9 ± 5 nmol/min/mg dry weight (with THF) || Skinner et al. (2009)<ref name= "Skinner2009">Skinner, K., Cuiffetti, L. and Hyman, M., 2009. Metabolism and cometabolism of cyclic ethers by a filamentous fungus, a Graphium sp. Appl. Environ. Microbiol., 75(17), pp.5514-5522. [https://doi.org/10.1128/aem.00078-09 doi:10.1128/AEM.00078-09] [[media:Skinner2009.pdf| Article | + | | ''Graphium'' sp. ATCC 58400 (fungus) || CYP || 4 ± 1 nmol/min/mg dry weight (with Propane) <br/>9 ± 5 nmol/min/mg dry weight (with THF) || Skinner et al. (2009)<ref name= "Skinner2009">Skinner, K., Cuiffetti, L. and Hyman, M., 2009. Metabolism and cometabolism of cyclic ethers by a filamentous fungus, a Graphium sp. Appl. Environ. Microbiol., 75(17), pp.5514-5522. [https://doi.org/10.1128/aem.00078-09 doi:10.1128/AEM.00078-09] [[media:Skinner2009.pdf| Article pdf]]</ref> |
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[[1,4-Dioxane]] (14D) does not readily biodegrade in most anaerobic environments<ref name= "Shen2008">Shen, W., Chen, H. and Pan, S., 2008. Anaerobic biodegradation of 1, 4-dioxane by sludge enriched with iron-reducing microorganisms. Bioresource technology, 99(7), pp.2483-2487. [https://doi.org/10.1016/j.biortech.2007.04.054 doi: 10.1016/j.biortech.2007.04.054]</ref>. However, multiple studies have demonstrated that 14D can be biodegraded by a variety of microorganisms under aerobic conditions<ref name= "Mahendra2006">Mahendra, S. and Alvarez-Cohen, L., 2006. Kinetics of 1, 4-dioxane biodegradation by monooxygenase-expressing bacteria. Environmental Science & Technology, 40(17), pp.5435-5442. [https://doi.org/10.1021/es060714v doi:10.1021/es060714v]</ref><ref>Mahendra, S., Petzold, C.J., Baidoo, E.E., Keasling, J.D. and Alvarez-Cohen, L., 2007. Identification of the intermediates of in vivo oxidation of 1, 4-dioxane by monooxygenase-containing bacteria. Environmental Science & Technology, 41(21), pp.7330-7336. [https://doi.org/10.1021/es0705745 doi: 10.1021/es0705745]</ref><ref name="Skinner2009"/><ref name = "Sun2011">Sun, B., Ko, K. and Ramsay, J.A., 2011. Biodegradation of 1, 4-dioxane by a Flavobacterium. Biodegradation, 22(3), pp.651-659. [https://doi.org/10.1007/s10532-010-9438-9 doi: 10.1007/s10532-010-9438-9]</ref>. A summary of microorganisms that are reported to aerobically biodegrade 14D is presented in Table 1. | [[1,4-Dioxane]] (14D) does not readily biodegrade in most anaerobic environments<ref name= "Shen2008">Shen, W., Chen, H. and Pan, S., 2008. Anaerobic biodegradation of 1, 4-dioxane by sludge enriched with iron-reducing microorganisms. Bioresource technology, 99(7), pp.2483-2487. [https://doi.org/10.1016/j.biortech.2007.04.054 doi: 10.1016/j.biortech.2007.04.054]</ref>. However, multiple studies have demonstrated that 14D can be biodegraded by a variety of microorganisms under aerobic conditions<ref name= "Mahendra2006">Mahendra, S. and Alvarez-Cohen, L., 2006. Kinetics of 1, 4-dioxane biodegradation by monooxygenase-expressing bacteria. Environmental Science & Technology, 40(17), pp.5435-5442. [https://doi.org/10.1021/es060714v doi:10.1021/es060714v]</ref><ref>Mahendra, S., Petzold, C.J., Baidoo, E.E., Keasling, J.D. and Alvarez-Cohen, L., 2007. Identification of the intermediates of in vivo oxidation of 1, 4-dioxane by monooxygenase-containing bacteria. Environmental Science & Technology, 41(21), pp.7330-7336. [https://doi.org/10.1021/es0705745 doi: 10.1021/es0705745]</ref><ref name="Skinner2009"/><ref name = "Sun2011">Sun, B., Ko, K. and Ramsay, J.A., 2011. Biodegradation of 1, 4-dioxane by a Flavobacterium. Biodegradation, 22(3), pp.651-659. [https://doi.org/10.1007/s10532-010-9438-9 doi: 10.1007/s10532-010-9438-9]</ref>. A summary of microorganisms that are reported to aerobically biodegrade 14D is presented in Table 1. | ||
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While several microorganisms have been isolated that can metabolize 14D<ref name= "Mahendra2006"/><ref name = "Kim2009"/><ref>Sei, K., Kakinoki, T., Inoue, D., Soda, S., Fujita, M. and Ike, M., 2010. Evaluation of the biodegradation potential of 1, 4-dioxane in river, soil and activated sludge samples. Biodegradation, 21(4), pp.585-591. [https://doi.org/10.1007/s10532-010-9326-3 doi: 10.1007/s10532-010-9326-3]</ref><ref name = "Sei2013"/><ref name = "Huang2014"/>, these organisms are not common. The best characterized 14D-metabolizing strain is ''Pseudonocardia dioxanivorans'' CB1190<ref name= "Mahendra2005"/>. This bacterium was originally enriched from industrial activated sludge, fed with [[wikipedia: Tetrahydrofuran | tetrahydrofuran]] (THF) and then subsequently fed with 14D<ref name= "Parales1994"/>. The doubling time of CB1190 was about 30 hours when it was grown in ammonium mineral salts medium at 30 °C amended with 5.5 mM (484 mg/L) 14D<ref name= "Parales1994"/>. | While several microorganisms have been isolated that can metabolize 14D<ref name= "Mahendra2006"/><ref name = "Kim2009"/><ref>Sei, K., Kakinoki, T., Inoue, D., Soda, S., Fujita, M. and Ike, M., 2010. Evaluation of the biodegradation potential of 1, 4-dioxane in river, soil and activated sludge samples. Biodegradation, 21(4), pp.585-591. [https://doi.org/10.1007/s10532-010-9326-3 doi: 10.1007/s10532-010-9326-3]</ref><ref name = "Sei2013"/><ref name = "Huang2014"/>, these organisms are not common. The best characterized 14D-metabolizing strain is ''Pseudonocardia dioxanivorans'' CB1190<ref name= "Mahendra2005"/>. This bacterium was originally enriched from industrial activated sludge, fed with [[wikipedia: Tetrahydrofuran | tetrahydrofuran]] (THF) and then subsequently fed with 14D<ref name= "Parales1994"/>. The doubling time of CB1190 was about 30 hours when it was grown in ammonium mineral salts medium at 30 °C amended with 5.5 mM (484 mg/L) 14D<ref name= "Parales1994"/>. | ||
− | Degradation of 14D by strain CB1190 may be inhibited by elevated concentrations of [[Chlorinated Solvents | chlorinated solvents]] and their degradation products, and by some metals. Inhibition of 14D degradation was strongest for 1,1-dichloroethene (1,1-DCE) followed by ''cis''-1,2-diochloroethene (cDCE) > trichloroethene (TCE) > 1,1,1-trichloroethane (TCA). 14D biodegradation was completely inhibited by 5 mg/L 1,1-DCE<ref>Mahendra, S., Grostern, A. and Alvarez-Cohen, L., 2013. The impact of chlorinated solvent co-contaminants on the biodegradation kinetics of 1, 4-dioxane. Chemosphere, 91(1), pp.88-92. [https://doi.org/10.1016/j.chemosphere.2012.10.104 doi: 10.1016/j.chemosphere.2012.10.104]</ref><ref name= "Hand2015"/><ref name= "Zhang2016">Zhang, S., Gedalanga, P.B. and Mahendra, S., 2016. Biodegradation kinetics of 1, 4-dioxane in chlorinated solvent mixtures. Environmental Science & Technology, 50(17), pp.9599-9607. [https://doi.org/10.1021/acs.est.6b02797 doi: 10.1021/acs.est.6b02797]</ref>. Cu(II) was the strongest metal inhibitor of 14D degradation by CB1190, causing an increase in the lag period at 1 mg/L and an order of magnitude reduction in 14D degradation rates at 10 and 20 mg/L Cu(II). 14D degradation was less sensitive to Cd(II) and Ni(II), while Zn(II) had no impact on 14D biodegradation at the maximum concentration tested (20 mg/L Zn)<ref>Pornwongthong, P., Mulchandani, A., Gedalanga, P.B. and Mahendra, S., 2014. Transition metals and organic ligands influence biodegradation of 1, 4-dioxane. Applied biochemistry and biotechnology, 173(1), pp.291-306. [https://doi.org/10.1007/s12010-014-0841-2 doi: 10.1007/s12010-014-0841-2]</ref>. | + | Degradation of 14D by strain CB1190 may be inhibited by elevated concentrations of [[Chlorinated Solvents | chlorinated solvents]] and their degradation products, and by some metals. Inhibition of 14D degradation was strongest for 1,1-dichloroethene (1,1-DCE) followed by ''cis''-1,2-diochloroethene (cDCE) > trichloroethene (TCE) > 1,1,1-trichloroethane (TCA). 14D biodegradation was completely inhibited by 5 mg/L 1,1-DCE<ref>Mahendra, S., Grostern, A. and Alvarez-Cohen, L., 2013. The impact of chlorinated solvent co-contaminants on the biodegradation kinetics of 1, 4-dioxane. Chemosphere, 91(1), pp.88-92. [https://doi.org/10.1016/j.chemosphere.2012.10.104 doi: 10.1016/j.chemosphere.2012.10.104]</ref><ref name= "Hand2015"/><ref name= "Zhang2016">Zhang, S., Gedalanga, P.B. and Mahendra, S., 2016. Biodegradation kinetics of 1, 4-dioxane in chlorinated solvent mixtures. Environmental Science & Technology, 50(17), pp.9599-9607. [https://doi.org/10.1021/acs.est.6b02797 doi: 10.1021/acs.est.6b02797] [[media:Zhang2016.pdf| Article pdf]]</ref>. Cu(II) was the strongest metal inhibitor of 14D degradation by CB1190, causing an increase in the lag period at 1 mg/L and an order of magnitude reduction in 14D degradation rates at 10 and 20 mg/L Cu(II). 14D degradation was less sensitive to Cd(II) and Ni(II), while Zn(II) had no impact on 14D biodegradation at the maximum concentration tested (20 mg/L Zn)<ref>Pornwongthong, P., Mulchandani, A., Gedalanga, P.B. and Mahendra, S., 2014. Transition metals and organic ligands influence biodegradation of 1, 4-dioxane. Applied biochemistry and biotechnology, 173(1), pp.291-306. [https://doi.org/10.1007/s12010-014-0841-2 doi: 10.1007/s12010-014-0841-2]</ref>. |
[[File:Mahendra1w2 Fig1.png|thumb|left|Figure 1. Growth Rates of Two 14D Metabolizers Versus 14D Concentration]] | [[File:Mahendra1w2 Fig1.png|thumb|left|Figure 1. Growth Rates of Two 14D Metabolizers Versus 14D Concentration]] | ||
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==Anaerobic Biodegradation== | ==Anaerobic Biodegradation== | ||
− | To date, there is little evidence of metabolic or cometabolic anaerobic 14D biodegradation. In a microcosm study using samples of aquifer material from several different 14D impacted sites, there was no evidence of 14D biodegradation<ref>Zenker, M.J., Borden, R.C. and Barlaz, M.A., 1999. Investigation of the intrinsic biodegradation of alkyl and cyclic ethers. The Fifth International In Situ and On-Site Bioremediation Symposium</ref>. However, there is one study that reported anaerobic growth of an iron-reducing bacterium on 14D<ref name= "Shen2008"/>. | + | To date, there is little evidence of metabolic or cometabolic anaerobic 14D biodegradation. In a microcosm study using samples of aquifer material from several different 14D impacted sites, there was no evidence of 14D biodegradation<ref>Zenker, M.J., Borden, R.C. and Barlaz, M.A., 1999. Investigation of the intrinsic biodegradation of alkyl and cyclic ethers. The Fifth International In Situ and On-Site Bioremediation Symposium. Battelle Press. Cincinnati, OH</ref>. However, there is one study that reported anaerobic growth of an iron-reducing bacterium on 14D<ref name= "Shen2008"/>. |
An indirect method of anaerobic 14D biodegradation exists via a microbially driven Fenton reaction. ''Shewanella oneidensis'', an Fe(III)-reducing facultative anaerobe, is able to generate hydroxyl radicals that can then break down 14D<ref>Sekar, R. and DiChristina, T.J., 2014. Microbially driven Fenton reaction for degradation of the widespread environmental contaminant 1, 4-dioxane. Environmental science & technology, 48(21), pp.12858-12867. [https://doi.org/10.1021/es503454a doi: 10.1021/es503454a]</ref>. Under anaerobic conditions, ''S. oneidensis'' produces Fe(II) that can then interact chemically with H<sub>2</sub>O<sub>2</sub> to yield HO• radicals which can oxidatively degrade 1,4-dioxane. | An indirect method of anaerobic 14D biodegradation exists via a microbially driven Fenton reaction. ''Shewanella oneidensis'', an Fe(III)-reducing facultative anaerobe, is able to generate hydroxyl radicals that can then break down 14D<ref>Sekar, R. and DiChristina, T.J., 2014. Microbially driven Fenton reaction for degradation of the widespread environmental contaminant 1, 4-dioxane. Environmental science & technology, 48(21), pp.12858-12867. [https://doi.org/10.1021/es503454a doi: 10.1021/es503454a]</ref>. Under anaerobic conditions, ''S. oneidensis'' produces Fe(II) that can then interact chemically with H<sub>2</sub>O<sub>2</sub> to yield HO• radicals which can oxidatively degrade 1,4-dioxane. | ||
==Molecular Biological Tools== | ==Molecular Biological Tools== | ||
− | [https://enviro.wiki/index.php?title=Quantitative_Polymerase_Chain_Reaction_(qPCR) Quantitative polymerase chain reaction (qPCR)] quantifies the abundance of specific microorganisms and functional genes capable of degrading a particular contaminant. qPCR analyses have been employed to quantify the abundance of microorganisms that can degrade 14D through the activity of tetrahydrofuran monooxygenase (THFMO) in samples from industrial activated sludge and groundwater<ref>Chiang, S.Y.D., Mora, R., Diguiseppi, W.H., Davis, G., Sublette, K., Gedalanga, P. and Mahendra, S., 2012. Characterizing the intrinsic bioremediation potential of 1, 4-dioxane and trichloroethene using innovative environmental diagnostic tools. Journal of Environmental Monitoring, 14(9), pp.2317-2326. [https://doi.org/10.1039/c2em30358b doi: 10.1039/C2EM30358B]</ref><ref>Gedalanga, P.B., Pornwongthong, P., Mora, R., Chiang, S.Y.D., Baldwin, B., Ogles, D. and Mahendra, S., 2014. Identification of biomarker genes to predict biodegradation of 1, 4-dioxane. Appl. Environ. Microbiol., 80(10), pp.3209-3218. [https://doi.org/10.1128/aem.04162-13 doi: 10.1128/AEM.04162-13]</ref><ref>Li, M., Mathieu, J., Liu, Y., Van Orden, E.T., Yang, Y., Fiorenza, S. and Alvarez, P.J., 2013. The abundance of tetrahydrofuran/dioxane monooxygenase genes (thmA/dxmA) and 1, 4-dioxane degradation activity are significantly correlated at various impacted aquifers. Environmental Science & Technology Letters, 1(1), pp.122-127. [https://doi.org/10.1021/ez400176h doi: 10.1021/ez400176h]</ref><ref name= "Li2013"/><ref name= "Zhang2016"/>. However, care is warranted in the interpretation of qPCR results in other cases (e.g. propane-stimulated cometabolic 14D degradation) where the role of enzymes such as propane monooxygenase (PrMO) in 14D degradation is less clearly established. Studies also suggest that these biomarkers can be used to detect the abundance of 14D-degraders ''in situ'' and quantify how they compete within the larger microbial community<ref>Miao, Y., Johnson, N.W., Gedalanga, P.B., Adamson, D., Newell, C. and Mahendra, S., 2019. Response and recovery of microbial communities subjected to oxidative and biological treatments of 1, 4-dioxane and co-contaminants. Water research, 149, pp.74-85. [https://doi.org/10.1016/j.watres.2018.10.070 doi:10.1016/j.watres.2018.10.070]</ref>. Microbial community analyses can be an asset towards guiding treatment strategies and predicting treatment synergies. | + | [https://enviro.wiki/index.php?title=Quantitative_Polymerase_Chain_Reaction_(qPCR) Quantitative polymerase chain reaction (qPCR)] quantifies the abundance of specific microorganisms and functional genes capable of degrading a particular contaminant. qPCR analyses have been employed to quantify the abundance of microorganisms that can degrade 14D through the activity of tetrahydrofuran monooxygenase (THFMO) in samples from industrial activated sludge and groundwater<ref>Chiang, S.Y.D., Mora, R., Diguiseppi, W.H., Davis, G., Sublette, K., Gedalanga, P. and Mahendra, S., 2012. Characterizing the intrinsic bioremediation potential of 1, 4-dioxane and trichloroethene using innovative environmental diagnostic tools. Journal of Environmental Monitoring, 14(9), pp.2317-2326. [https://doi.org/10.1039/c2em30358b doi: 10.1039/C2EM30358B]</ref><ref>Gedalanga, P.B., Pornwongthong, P., Mora, R., Chiang, S.Y.D., Baldwin, B., Ogles, D. and Mahendra, S., 2014. Identification of biomarker genes to predict biodegradation of 1, 4-dioxane. Appl. Environ. Microbiol., 80(10), pp.3209-3218. [https://doi.org/10.1128/aem.04162-13 doi: 10.1128/AEM.04162-13] [[media:Gedalanga2014.pdf| Article pdf]]</ref><ref>Li, M., Mathieu, J., Liu, Y., Van Orden, E.T., Yang, Y., Fiorenza, S. and Alvarez, P.J., 2013. The abundance of tetrahydrofuran/dioxane monooxygenase genes (thmA/dxmA) and 1, 4-dioxane degradation activity are significantly correlated at various impacted aquifers. Environmental Science & Technology Letters, 1(1), pp.122-127. [https://doi.org/10.1021/ez400176h doi: 10.1021/ez400176h]</ref><ref name= "Li2013"/><ref name= "Zhang2016"/>. However, care is warranted in the interpretation of qPCR results in other cases (e.g. propane-stimulated cometabolic 14D degradation) where the role of enzymes such as propane monooxygenase (PrMO) in 14D degradation is less clearly established. Studies also suggest that these biomarkers can be used to detect the abundance of 14D-degraders ''in situ'' and quantify how they compete within the larger microbial community<ref>Miao, Y., Johnson, N.W., Gedalanga, P.B., Adamson, D., Newell, C. and Mahendra, S., 2019. Response and recovery of microbial communities subjected to oxidative and biological treatments of 1, 4-dioxane and co-contaminants. Water research, 149, pp.74-85. [https://doi.org/10.1016/j.watres.2018.10.070 doi:10.1016/j.watres.2018.10.070]</ref>. Microbial community analyses can be an asset towards guiding treatment strategies and predicting treatment synergies. |
[https://enviro.wiki/index.php?title=Compound_Specific_Isotope_Analysis_(CSIA) Compound specific isotope analysis (CSIA)] refers to measurement of the isotopic ratios of individual chemical compounds and can be used to differentiate contaminant sources, delineate reaction pathways, and provide evidence of ''in situ'' contaminant degradation. CSIA methods are now available to measure isotopic fractionation of carbon and hydrogen<ref name= "Bennett2017"/>. For example, the aerobic biodegradation of 14D by a THF-grown 14D-degrading ''Pseudonocardia'' strain exhibited an isotopic fractionation factor (<big>''ε'' </big>) for carbon (<big>''ε''</big><sub>''c''</sub>) of −4.73 ± 0.9‰ and hydrogen (<big>ε</big><sub>''H''</sub>) of -147 ± 22‰, respectively. Smaller <big>''ε''</big><sub>''c''</sub>and <big>ε</big><sub>''H''</sub> values, (-2.7 ± 0.3‰ and -21 ± 2‰, respectively) were determined for aerobic 14D degradation by a propane-grown ''Rhodococcus'' strain. As many ''Pseudonocardia'' strains use THFMO to initiate 14D degradation, CSIA, in conjunction with qPCR analyses, may be able to discriminate the roles of metabolism and cometabolism in 14D biodegradation at field sites<ref>Gedalanga, P., Madison, A., Miao, Y., Richards, T., Hatton, J., DiGuiseppi, W.H., Wilson, J. and Mahendra, S., 2016. A Multiple Lines of Evidence Framework to Evaluate Intrinsic Biodegradation of 1, 4‐Dioxane. Remediation Journal, 27(1), pp.93-114. [https://doi.org/10.1002/rem.21499 doi: 10.1002/rem.21499]</ref>. | [https://enviro.wiki/index.php?title=Compound_Specific_Isotope_Analysis_(CSIA) Compound specific isotope analysis (CSIA)] refers to measurement of the isotopic ratios of individual chemical compounds and can be used to differentiate contaminant sources, delineate reaction pathways, and provide evidence of ''in situ'' contaminant degradation. CSIA methods are now available to measure isotopic fractionation of carbon and hydrogen<ref name= "Bennett2017"/>. For example, the aerobic biodegradation of 14D by a THF-grown 14D-degrading ''Pseudonocardia'' strain exhibited an isotopic fractionation factor (<big>''ε'' </big>) for carbon (<big>''ε''</big><sub>''c''</sub>) of −4.73 ± 0.9‰ and hydrogen (<big>ε</big><sub>''H''</sub>) of -147 ± 22‰, respectively. Smaller <big>''ε''</big><sub>''c''</sub>and <big>ε</big><sub>''H''</sub> values, (-2.7 ± 0.3‰ and -21 ± 2‰, respectively) were determined for aerobic 14D degradation by a propane-grown ''Rhodococcus'' strain. As many ''Pseudonocardia'' strains use THFMO to initiate 14D degradation, CSIA, in conjunction with qPCR analyses, may be able to discriminate the roles of metabolism and cometabolism in 14D biodegradation at field sites<ref>Gedalanga, P., Madison, A., Miao, Y., Richards, T., Hatton, J., DiGuiseppi, W.H., Wilson, J. and Mahendra, S., 2016. A Multiple Lines of Evidence Framework to Evaluate Intrinsic Biodegradation of 1, 4‐Dioxane. Remediation Journal, 27(1), pp.93-114. [https://doi.org/10.1002/rem.21499 doi: 10.1002/rem.21499]</ref>. |
Latest revision as of 05:05, 30 November 2021
1,4-Dioxane (14D) does not readily biodegrade in most environments. However, a variety of microorganisms have been identified that can biodegrade 14D through either direct growth-related metabolism or cometabolism. During metabolic biodegradation, microorganisms use 14D as the growth substrate, however growth is slow unless 14D concentrations are very high (>100 mg/L). During cometabolic biodegradation, an additional growth substrate must be supplied to support biomass growth and induce the appropriate 14D-degrading enzymes. Unlike metabolic degradation, cometabolic processes can reduce 14D to very low concentrations.
Related Article(s):
Contributor(s): Dr. Shaily Mahendra and Dr. Michael Hyman
Key Resource(s):
1,4-Dioxane Biodegradation
Strain | Induced Enzyme | Biodegradation Rate | Reference |
---|---|---|---|
Metabolism | |||
Pseudonocardia dioxanivorans CB1190 | THFMO | 0.19 ± 0.007 mg/hr/mg-protein | Mahendra and Alvarez-Cohen (2005, 2006)[2][3] |
Actinomycete CB1190* | N/A | 0.33 mg/min/mg-protein | Parales et al. (1994)[4] |
Amycolata sp. CB1190* | N/A | 0.038 ± 0.012 mg/hr/mg-protein | Kelley et al. (2001) |
Pseudonocardia benzenivorans B5 | THFMO | 0.01± 0.003 mg/hr/mg-protein | Mahendra and Alvarez-Cohen (2006)[3] |
Pseudonocardia carboxydivorans RM-31 | ? | 31.6 mg/L/hr | Matsui et al. (2016)[5] |
Afipia sp. D1 | ? | 0.052 to 0.263 mg/hr/mg-protein | Sei et al. (2013)[6] |
Mycobacterium sp. PH-06 | PrMO | 2.5 mg/L/hr | Kim et al. (2009)[7] |
Acinetobacter baumannii DD1 | ? | 2.38 mg/L/hr | Huang et al. (2014)[8] |
Xanthobacter flavus DT8 | ? | Similar to CB1190 | Chen et al. (2016)[9] |
Cordyceps sinensis (fungus) | ? | 0.011 mol/day | Nakamiya et al. (2005)[10] |
Cometabolism | |||
Mycobacterium austroafricanum JOB5 | ? | 0.40 ± 0.06 mg/hr/mg-protein | House and Hyman (2010)[11], Lan et al. (2013)[12][3] |
Rhodococcus ruber ENV425 | ? | 10 mg/hr/g TSS | Lippincott et al. (2015)[13], Vainberg et al. (2006)[14] |
Pseudonocardia sp. ENV478 | THFMO | 21 mg/hr/g TSS | Masuda et al. (2012)[15], Vainberg et al. (2006)[14] |
Rhodococcus RR1 | ? | 0.38 ± 0.03 mg/hr/mg-protein | Mahendra and Alvarez-Cohen (2006)[3] |
Rhodococcus jostii RHA1 | PrMO | N/A | Hand et al. (2015)[16], Li et al. (2013)[17] |
Flavobacterium | ? | N/A | Sun et al. (2011)[18] |
Pseudonocardia K1 | THFMO | 0.26 ± 0.013 mg/hr/mg-protein | Mahendra and Alvarez-Cohen (2006)[3] |
Burkholderia cepacia G4 | T2MO | 0.1± 0.006 mg/hr/mg-protein | Mahendra and Alvarez-Cohen (2006)[3] |
Ralstonia pickettii PKO1 | T3MO | 0.31± 0.007 mg/hr/mg-protein | Mahendra and Alvarez-Cohen (2006)[3] |
Pseudomonas mendocina KR1 | T4MO | 0.37± 0.04 mg/hr/mg-protein | Mahendra and Alvarez-Cohen (2006)[3] |
Aureobasidium pullmans NRRL 21064 | ? | 6-8 mg/L within a day | Patt and Abebe (1995)[19] |
Graphium sp. ATCC 58400 (fungus) | CYP | 4 ± 1 nmol/min/mg dry weight (with Propane) 9 ± 5 nmol/min/mg dry weight (with THF) |
Skinner et al. (2009)[20] |
1,4-Dioxane (14D) does not readily biodegrade in most anaerobic environments[21]. However, multiple studies have demonstrated that 14D can be biodegraded by a variety of microorganisms under aerobic conditions[3][22][20][18]. A summary of microorganisms that are reported to aerobically biodegrade 14D is presented in Table 1.
Under aerobic conditions 14D can be biodegraded through two physiologically distinct processes: (a) metabolism and (b) cometabolism. Metabolism is a process in which microorganisms use the organic contaminants as a carbon and energy source to support their growth. Cometabolism occurs when microorganisms degrade contaminants using non-specific enzymes but do not gain carbon or energy to support growth from the degradation process.
Aerobic Metabolism
While several microorganisms have been isolated that can metabolize 14D[3][7][23][6][8], these organisms are not common. The best characterized 14D-metabolizing strain is Pseudonocardia dioxanivorans CB1190[2]. This bacterium was originally enriched from industrial activated sludge, fed with tetrahydrofuran (THF) and then subsequently fed with 14D[4]. The doubling time of CB1190 was about 30 hours when it was grown in ammonium mineral salts medium at 30 °C amended with 5.5 mM (484 mg/L) 14D[4].
Degradation of 14D by strain CB1190 may be inhibited by elevated concentrations of chlorinated solvents and their degradation products, and by some metals. Inhibition of 14D degradation was strongest for 1,1-dichloroethene (1,1-DCE) followed by cis-1,2-diochloroethene (cDCE) > trichloroethene (TCE) > 1,1,1-trichloroethane (TCA). 14D biodegradation was completely inhibited by 5 mg/L 1,1-DCE[24][16][25]. Cu(II) was the strongest metal inhibitor of 14D degradation by CB1190, causing an increase in the lag period at 1 mg/L and an order of magnitude reduction in 14D degradation rates at 10 and 20 mg/L Cu(II). 14D degradation was less sensitive to Cd(II) and Ni(II), while Zn(II) had no impact on 14D biodegradation at the maximum concentration tested (20 mg/L Zn)[26].
An important challenge for in situ bioremediation of 14D is the slow growth of 14D metabolizers at typical groundwater concentrations. Figure 1 shows estimated growth rates for two 14D metabolizing organisms (P. dioxanivorans CB1190 and P. benzenivorans B5) computed using published kinetic parameters[3]. At a 14D concentration of 1000 µg/L, CB1190 and B2 have growth rates of 0.015 and 0.002 per day. At typical groundwater concentrations (<1000 µg/L), growth rates are expected to be less than the endogenous decay rate, resulting in a steady decline in the number of 14D metabolizers.
Aerobic Cometabolism
Unlike 14D-metabolizing microorganisms, 14D-cometabolizing organisms do not grow on 14D but can degrade this compound after growth on a primary, growth-supporting substrate. As cometabolically active microorganisms do not use co-substrates as either major carbon or energy sources, they can often degrade co-substrates at concentrations well below those that can be achieved by organisms that metabolize and grow on these co-substrates. A wide variety of bacteria[3] and some fungi[19][20] can cometabolically degrade 14D (see Table 1). These include model organisms that grow on primary substrates such as toluene or methane[3] and involve well-characterized enzymes such as soluble methane monooxygenase (sMMO) or toluene monooxygenases (TxMO), respectively. Other 14D-cometabolizing strains that grow on THF[14], ethane[27], and isobutane[28] have also been described.
Much of the research into 14D cometabolism has focused on high concentrations of 14D (≥100 mg/L), and less is currently known about the activity of specific microorganisms and their monooxygenases at lower, more environmentally relevant 14D concentrations (<100 µg/L). Despite this, many bacterial monooxygenases can concurrently oxidize multiple co-substrates, and recent field studies have demonstrated that cometabolic approaches involving either propane biostimulation and bioaugmentation[13] or propane biostimulation alone[29] can be highly effective treatment strategies for degrading contaminant mixtures that contain parts-per-billion concentrations of both 14D and associated chlorinated co-contaminants.
Anaerobic Biodegradation
To date, there is little evidence of metabolic or cometabolic anaerobic 14D biodegradation. In a microcosm study using samples of aquifer material from several different 14D impacted sites, there was no evidence of 14D biodegradation[30]. However, there is one study that reported anaerobic growth of an iron-reducing bacterium on 14D[21].
An indirect method of anaerobic 14D biodegradation exists via a microbially driven Fenton reaction. Shewanella oneidensis, an Fe(III)-reducing facultative anaerobe, is able to generate hydroxyl radicals that can then break down 14D[31]. Under anaerobic conditions, S. oneidensis produces Fe(II) that can then interact chemically with H2O2 to yield HO• radicals which can oxidatively degrade 1,4-dioxane.
Molecular Biological Tools
Quantitative polymerase chain reaction (qPCR) quantifies the abundance of specific microorganisms and functional genes capable of degrading a particular contaminant. qPCR analyses have been employed to quantify the abundance of microorganisms that can degrade 14D through the activity of tetrahydrofuran monooxygenase (THFMO) in samples from industrial activated sludge and groundwater[32][33][34][17][25]. However, care is warranted in the interpretation of qPCR results in other cases (e.g. propane-stimulated cometabolic 14D degradation) where the role of enzymes such as propane monooxygenase (PrMO) in 14D degradation is less clearly established. Studies also suggest that these biomarkers can be used to detect the abundance of 14D-degraders in situ and quantify how they compete within the larger microbial community[35]. Microbial community analyses can be an asset towards guiding treatment strategies and predicting treatment synergies.
Compound specific isotope analysis (CSIA) refers to measurement of the isotopic ratios of individual chemical compounds and can be used to differentiate contaminant sources, delineate reaction pathways, and provide evidence of in situ contaminant degradation. CSIA methods are now available to measure isotopic fractionation of carbon and hydrogen[28]. For example, the aerobic biodegradation of 14D by a THF-grown 14D-degrading Pseudonocardia strain exhibited an isotopic fractionation factor (ε ) for carbon (εc) of −4.73 ± 0.9‰ and hydrogen (εH) of -147 ± 22‰, respectively. Smaller εcand εH values, (-2.7 ± 0.3‰ and -21 ± 2‰, respectively) were determined for aerobic 14D degradation by a propane-grown Rhodococcus strain. As many Pseudonocardia strains use THFMO to initiate 14D degradation, CSIA, in conjunction with qPCR analyses, may be able to discriminate the roles of metabolism and cometabolism in 14D biodegradation at field sites[36].
Summary
14D is not readily biodegraded under ambient conditions in most environments. However, a variety of microorganisms have been identified that can biodegrade 14D through either growth-related metabolism or fortuitous cometabolism. Metabolic growth on the target pollutant is the more traditional approach for both above ground and in situ bioremediation approaches. However, approaches based on metabolic growth may not be feasible for treatment of 14D at typical concentrations. Cometabolic treatment approaches can reduce 14D to very low levels and have been demonstrated in the field. However, implementation of cometabolic treatment is more complex, and there is currently less engineering experience in the design and operation of these systems.
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