2016
DOI: 10.1007/s00204-016-1726-7
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Activation of the Nrf2-ARE pathway by the Alternaria alternata mycotoxins altertoxin I and II

Abstract: The mycotoxins altertoxin I and II (ATX I and II) are secondary metabolites produced by Alternaria alternata fungi and may occur as food and feed contaminants, especially after long storage periods. Although the toxic potential of altertoxins has been previously investigated, little is known about the pathways that play a role in their intracellular metabolism. In order to identify potential targets of ATX I and ATX II, the two toxins were tested for interaction with the nuclear factor erythroid-derived 2-like… Show more

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Cited by 36 publications
(40 citation statements)
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“…The mechanisms behind its mode of action could not be clarified so far. Nevertheless, genotoxicity was observed at comparatively low concentrations, but no enhanced levels of reactive oxygen species, glutathione depletion, or topoisomerase inhibition [11, 12]. Besides, AOH, AME, and some of their metabolites additionally exhibit estrogenic potential [13, 14] which may be enhanced by combinatory toxic effects [1517].…”
Section: Introductionmentioning
confidence: 99%
“…The mechanisms behind its mode of action could not be clarified so far. Nevertheless, genotoxicity was observed at comparatively low concentrations, but no enhanced levels of reactive oxygen species, glutathione depletion, or topoisomerase inhibition [11, 12]. Besides, AOH, AME, and some of their metabolites additionally exhibit estrogenic potential [13, 14] which may be enhanced by combinatory toxic effects [1517].…”
Section: Introductionmentioning
confidence: 99%
“…The fate of ATXII during food production is still unknown and currently subject to intensive research, thus still hampering any reliable exposure estimation. Applied in mammalian cell culture, ATXII triggers genotoxic and mutagenic damage (Fleck et al 2012; Pahlke et al 2016; Schwarz et al 2012), enhances intracellular ROS (reactive oxygen species) levels and activates the redox-sensitive Nrf2/ARE pathway (Jarolim et al 2017; Pahlke et al 2016). In spite of that, it was recently described that the toxin may be rapidly and efficiently biotransformed in differentiated Caco2 cells (Fleck et al 2014a).…”
Section: Introductionmentioning
confidence: 99%
“…Ethyl acetate extracts were prepared after 21 days of incubation from rice which was inoculated with Alternaria alternata strain DSM 62010 as described in Schwarz et al (2012a). Fractionation of the ethyl acetate extracts by solid-phase extraction (SPE) and isolation of the toxins with HPLC were conducted according to Jarolim et al (2016). For isolation individual fractions were collected, concentrated under reduced pressure (40 °C), and freeze-dried in duplicate, yielding ATX II and STTX III in high purities (>97 % HPLC–UV, 270 nm).…”
Section: Methodsmentioning
confidence: 99%
“…For isolation individual fractions were collected, concentrated under reduced pressure (40 °C), and freeze-dried in duplicate, yielding ATX II and STTX III in high purities (>97 % HPLC–UV, 270 nm). ATX I and ALP were re-purified using the HPLC system and column mentioned in Jarolim et al (2016) and the following gradient. Monitoring the effluent (4.2 ml/min) at 350 nm, chromatography was performed starting with a mixture (80/20, v/v) of aqueous formic acid (0.1 % in H 2 O) and MeCN, the MeCN content was increased to 45 % within 16 min and to 70 % within 4 min, followed by column washing and re-equilibration.…”
Section: Methodsmentioning
confidence: 99%
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