Differences in neurotoxic effects of ochratoxin A, ochracin and ochratoxin-alpha in vitro.

A Bruinink, T Rasonyi, C Sidler
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引用次数: 48

Abstract

The mycotoxin ochratoxin A (OTA) is a chlorinated dihydroisocoumarin derivative connected through an amide-bond to L-phenylalanine. In a previous study we could show that competition with L-phenylalanine-dependent processes does not play a role in OTA neurotoxicity. To test whether the isocoumarin part is responsible for the neurotoxic effects, we determined in the present study the effects of the hydrolysis product of OTA, ochratoxin-alpha (OTalpha), and of ochracin on embryonic chick brain cell cultures. In addition, we investigated the interaction between OTA and ochracin regarding the neurotoxic effects. We report here that OTalpha did not affect brain cell cultures at concentrations up to 15 microM. With the exception of a small (20%) but significant reduction in cell culture, cellular protein at concentrations above 0.3 microM, in our cell cultures' cell function, as defined by neutral red uptake and MTT-dehydrogenase activity, was only reduced by high OTalpha concentrations (1 mM). Addition of 0.1 microM OTA increased ochracin cytotoxicity as defined by latter parameters. No effects on cell culture NF68kD content could be detected. The results are discussed with regard to the existence of an OTA target interaction binding site.

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赭曲霉毒素A、赭曲霉毒素和赭曲霉毒素α体外神经毒性作用的差异。
赭曲霉毒素A (OTA)是一种氯化的二氢异香豆素衍生物,通过酰胺键与l -苯丙氨酸相连。在先前的研究中,我们可以证明与l -苯丙氨酸依赖过程的竞争在OTA神经毒性中不起作用。为了测试异香豆素部分是否对神经毒性作用负责,我们在本研究中确定了OTA,赭曲霉毒素- α (OTalpha)和赭曲霉素的水解产物对胚胎鸡脑细胞培养的影响。此外,我们还研究了OTA与ochracin在神经毒性作用方面的相互作用。我们在此报告OTalpha在浓度高达15微米时不影响脑细胞培养。除了细胞培养中少量(20%)但显著减少外,在浓度高于0.3微米时,细胞蛋白在我们的细胞培养中的细胞功能(由中性红色摄取和mtt脱氢酶活性定义)仅在高OTalpha浓度(1毫米)下降低。0.1 μ m OTA的加入增加了ochracin的细胞毒性。未检测到对细胞培养NF68kD含量的影响。讨论了OTA靶相互作用结合位点的存在性。
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Erratum: Alfonso D, Johnson HA, Colman-Saizarbitoria T, Presley CP, McCabe GP, McLaughlin JL (1996): SARs of annonaceous acetogenins in rat liver mitochondria. Nat Toxins 4:181-188. Advances in detection methods for fungal and algal toxins. HPLC/MS analysis of fusarium mycotoxins, fumonisins and deoxynivalenol. Neuronal binding of tetanus toxin compared to its ganglioside binding fragment (H(c)). A new type sandwich immunoassay for microcystin: production of monoclonal antibodies specific to the immune complex formed by microcystin and an anti-microcystin monoclonal antibody.
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