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Tracking atrazine degradation in soil combining 14C-mineralisation assays and compound-specific isotope analysis.
Gallego, Sara; Sungthong, Rungroch; Guyot, Benoît; Saphy, Adrien; Devers-Lamrani, Marion; Martin-Laurent, Fabrice; Imfeld, Gwenaël.
Affiliation
  • Gallego S; INRAE, Institut Agro Dijon, Université de Bourgogne Franche-Comté, Agroécologie Dijon, France.
  • Sungthong R; Institut Terre et Environnement de Strasbourg, Université de Strasbourg/EOST/ENGEES, CNRS UMR 7063, Strasbourg, F-67084, France.
  • Guyot B; Institut Terre et Environnement de Strasbourg, Université de Strasbourg/EOST/ENGEES, CNRS UMR 7063, Strasbourg, F-67084, France.
  • Saphy A; Institut Terre et Environnement de Strasbourg, Université de Strasbourg/EOST/ENGEES, CNRS UMR 7063, Strasbourg, F-67084, France.
  • Devers-Lamrani M; INRAE, Institut Agro Dijon, Université de Bourgogne Franche-Comté, Agroécologie Dijon, France.
  • Martin-Laurent F; INRAE, Institut Agro Dijon, Université de Bourgogne Franche-Comté, Agroécologie Dijon, France.
  • Imfeld G; Institut Terre et Environnement de Strasbourg, Université de Strasbourg/EOST/ENGEES, CNRS UMR 7063, Strasbourg, F-67084, France. Electronic address: imfeld@unistra.fr.
Chemosphere ; 363: 142981, 2024 Sep.
Article in En | MEDLINE | ID: mdl-39089341
ABSTRACT
The quantification of pesticide dissipation in agricultural soil is challenging. In this study, we investigated atrazine biodegradation in both liquid and soil experiments bioaugmented with distinct atrazine-degrading bacterial isolates. This was achieved by combining 14C-mineralisation assays and compound-specific isotope analysis of atrazine. In liquid experiments, the three bacterial isolates mineralised over 40% of atrazine, demonstrating their potential for extensive degradation. However, the kinetics of mineralisation and degradation varied among the isolates. Carbon stable isotope fractionation was similar for Pseudomonas isolates ADPT34 and ADP2T0, but slightly higher for Chelatobacter SR27. In soil experiments, atrazine primarily degraded into atrazine-desethyl, while atrazine-hydroxy was mainly observed in experiments with SR27. Atrazine mineralisation in soil by ADPT34 and SR27 exceeded 40%, whereas ADP2T0 exhibited a mineralisation rate of 10%. In experiments with ADPT34 and SR27, atrazine 14C-residues were predominantly found in the non-extractable fraction, whereas they accumulated in the extractable fraction in the experiment with ADP2T0. Compound-specific isotope analysis (CSIA) relies on changes of stable isotope ratios and holds potential to evaluate herbicide transformation in soil. CSIA of atrazine indicated atrazine biodegradation in water and solvent extractable soil fractions and varied between 29% and 52%, depending on the bacterial isolate. Despite atrazine degradation in both soil fractions, a significant portion of atrazine residues persisted, depending on the bacterial degrader, initial cell concentration, and mineralisation and degradation rates. Overall, our approach can aid in quantifying atrazine persistence and degradation in soil, and in optimizing bioaugmentation strategies for remediating soils contaminated with persistent herbicides.
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Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Atrazine / Soil / Soil Microbiology / Soil Pollutants / Biodegradation, Environmental / Herbicides Language: En Journal: Chemosphere Year: 2024 Document type: Article Affiliation country: France Country of publication: United kingdom

Full text: 1 Collection: 01-internacional Database: MEDLINE Main subject: Atrazine / Soil / Soil Microbiology / Soil Pollutants / Biodegradation, Environmental / Herbicides Language: En Journal: Chemosphere Year: 2024 Document type: Article Affiliation country: France Country of publication: United kingdom