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Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria

Steroidal oestrogens (C(18)) are contaminants receiving increasing attention due to their endocrine‐disrupting activities at sub‐nanomolar concentrations. Although oestrogens can be eliminated through photodegradation, microbial function is critical for removing oestrogens from ecosystems devoid of...

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Autores principales: Hsiao, Tsun‐Hsien, Lee, Tzong‐Huei, Chuang, Meng‐Rong, Wang, Po‐Hsiang, Meng, Menghsiao, Horinouchi, Masae, Hayashi, Toshiaki, Chen, Yi‐Lung, Chiang, Yin‐Ru
Formato: Online Artículo Texto
Lenguaje:English
Publicado: John Wiley and Sons Inc. 2021
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8913865/
https://www.ncbi.nlm.nih.gov/pubmed/34523795
http://dx.doi.org/10.1111/1751-7915.13921
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author Hsiao, Tsun‐Hsien
Lee, Tzong‐Huei
Chuang, Meng‐Rong
Wang, Po‐Hsiang
Meng, Menghsiao
Horinouchi, Masae
Hayashi, Toshiaki
Chen, Yi‐Lung
Chiang, Yin‐Ru
author_facet Hsiao, Tsun‐Hsien
Lee, Tzong‐Huei
Chuang, Meng‐Rong
Wang, Po‐Hsiang
Meng, Menghsiao
Horinouchi, Masae
Hayashi, Toshiaki
Chen, Yi‐Lung
Chiang, Yin‐Ru
author_sort Hsiao, Tsun‐Hsien
collection PubMed
description Steroidal oestrogens (C(18)) are contaminants receiving increasing attention due to their endocrine‐disrupting activities at sub‐nanomolar concentrations. Although oestrogens can be eliminated through photodegradation, microbial function is critical for removing oestrogens from ecosystems devoid of sunlight exposure including activated sludge, soils and aquatic sediments. Actinobacteria were found to be key oestrogen degraders in manure‐contaminated soils and estuarine sediments. Previously, we used the actinobacterium Rhodococcus sp. strain B50 as a model microorganism to identify two oxygenase genes, aedA and aedB, involved in the activation and subsequent cleavage of the estrogenic A‐ring respectively. However, genes responsible for the downstream degradation of oestrogen A/B‐rings remained completely unknown. In this study, we employed tiered comparative transcriptomics, gene disruption experiments and mass spectrometry‐based metabolite profile analysis to identify oestrogen catabolic genes. We observed the up‐regulation of thiolase‐encoding aedF and aedK in the transcriptome of strain B50 grown with oestrone. Consistently, two downstream oestrogenic metabolites, 5‐oxo‐4‐norestrogenic acid (C(17)) and 2,3,4‐trinorestrogenic acid (C(15)), were accumulated in aedF‐ and aedK‐disrupted strain B50 cultures. Disruption of fadD3 [3aα‐H‐4α(3'‐propanoate)‐7aβ‐methylhexahydro‐1,5‐indanedione (HIP)‐coenzyme A‐ligase gene] in strain B50 resulted in apparent HIP accumulation in oestrone‐fed cultures, indicating the essential role of fadD3 in actinobacterial oestrogen degradation. In addition, we detected a unique meta‐cleavage product, 4,5‐seco‐estrogenic acid (C(18)), during actinobacterial oestrogen degradation. Differentiating the oestrogenic metabolite profile and degradation genes of actinobacteria and proteobacteria enables the cost‐effective and time‐saving identification of potential oestrogen degraders in various ecosystems through liquid chromatography–mass spectrometry analysis and polymerase chain reaction‐based functional assays.
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spelling pubmed-89138652022-03-17 Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria Hsiao, Tsun‐Hsien Lee, Tzong‐Huei Chuang, Meng‐Rong Wang, Po‐Hsiang Meng, Menghsiao Horinouchi, Masae Hayashi, Toshiaki Chen, Yi‐Lung Chiang, Yin‐Ru Microb Biotechnol Research Articles Steroidal oestrogens (C(18)) are contaminants receiving increasing attention due to their endocrine‐disrupting activities at sub‐nanomolar concentrations. Although oestrogens can be eliminated through photodegradation, microbial function is critical for removing oestrogens from ecosystems devoid of sunlight exposure including activated sludge, soils and aquatic sediments. Actinobacteria were found to be key oestrogen degraders in manure‐contaminated soils and estuarine sediments. Previously, we used the actinobacterium Rhodococcus sp. strain B50 as a model microorganism to identify two oxygenase genes, aedA and aedB, involved in the activation and subsequent cleavage of the estrogenic A‐ring respectively. However, genes responsible for the downstream degradation of oestrogen A/B‐rings remained completely unknown. In this study, we employed tiered comparative transcriptomics, gene disruption experiments and mass spectrometry‐based metabolite profile analysis to identify oestrogen catabolic genes. We observed the up‐regulation of thiolase‐encoding aedF and aedK in the transcriptome of strain B50 grown with oestrone. Consistently, two downstream oestrogenic metabolites, 5‐oxo‐4‐norestrogenic acid (C(17)) and 2,3,4‐trinorestrogenic acid (C(15)), were accumulated in aedF‐ and aedK‐disrupted strain B50 cultures. Disruption of fadD3 [3aα‐H‐4α(3'‐propanoate)‐7aβ‐methylhexahydro‐1,5‐indanedione (HIP)‐coenzyme A‐ligase gene] in strain B50 resulted in apparent HIP accumulation in oestrone‐fed cultures, indicating the essential role of fadD3 in actinobacterial oestrogen degradation. In addition, we detected a unique meta‐cleavage product, 4,5‐seco‐estrogenic acid (C(18)), during actinobacterial oestrogen degradation. Differentiating the oestrogenic metabolite profile and degradation genes of actinobacteria and proteobacteria enables the cost‐effective and time‐saving identification of potential oestrogen degraders in various ecosystems through liquid chromatography–mass spectrometry analysis and polymerase chain reaction‐based functional assays. John Wiley and Sons Inc. 2021-09-15 /pmc/articles/PMC8913865/ /pubmed/34523795 http://dx.doi.org/10.1111/1751-7915.13921 Text en © 2021 The Authors. Microbial Biotechnology published by Society for Applied Microbiology and John Wiley & Sons Ltd. https://creativecommons.org/licenses/by-nc/4.0/This is an open access article under the terms of the http://creativecommons.org/licenses/by-nc/4.0/ (https://creativecommons.org/licenses/by-nc/4.0/) License, which permits use, distribution and reproduction in any medium, provided the original work is properly cited and is not used for commercial purposes.
spellingShingle Research Articles
Hsiao, Tsun‐Hsien
Lee, Tzong‐Huei
Chuang, Meng‐Rong
Wang, Po‐Hsiang
Meng, Menghsiao
Horinouchi, Masae
Hayashi, Toshiaki
Chen, Yi‐Lung
Chiang, Yin‐Ru
Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria
title Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria
title_full Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria
title_fullStr Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria
title_full_unstemmed Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria
title_short Identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria
title_sort identification of essential β‐oxidation genes and corresponding metabolites for oestrogen degradation by actinobacteria
topic Research Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8913865/
https://www.ncbi.nlm.nih.gov/pubmed/34523795
http://dx.doi.org/10.1111/1751-7915.13921
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