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建立一种体外方法预测霉菌毒素在酵母基产品上的结合:以黄曲霉毒素B₁、玉米赤霉烯酮和赭曲霉毒素A为例

Development of an in vitro method for the prediction of mycotoxin binding on yeast-based products: case of aflatoxin B₁, zearalenone and ochratoxin A.

作者信息

Faucet-Marquis Virginie, Joannis-Cassan Claire, Hadjeba-Medjdoub Kheira, Ballet Nathalie, Pfohl-Leszkowicz Annie

机构信息

Laboratory Chemical Engineering, University of Toulouse, UMR-CNRS/INPT/UPS 5503, 1 avenue agrobiopôle, 31320, Auzeville-Tolosane, France.

出版信息

Appl Microbiol Biotechnol. 2014 Sep;98(17):7583-96. doi: 10.1007/s00253-014-5917-y. Epub 2014 Jul 13.

Abstract

To date, no official method is available to accurately define the binding capacity of binders. The goal is to define general in vitro parameters (equilibrium time, pH, mycotoxin/binder ratio) for the determination of binding efficacy, which can be used to calculate the relevant equilibrium adsorption constants. For this purpose, aflatoxin B1 (AFB1), zearalenone (ZEA) or ochratoxin A (OTA) were incubated with one yeast cell wall in pH 3, pH 5 or pH 7 buffers. The percentage of adsorption was recorded by quantitation of remaining mycotoxins in the supernatant and amount of mycotoxin adsorbed on the residue. The incubation of yeast cell wall in the presence of mycotoxins solved in buffer, lead to unexpected high adsorption percentage when the analysis was based only on remaining mycotoxins in the supernatant. The decrease of mycotoxins in the supernatant was not correlated to the amount of mycotoxins found in the residue. For this reason we modified the conditions of incubation. Yeast cell wall (5 mg) was pre-incubated in buffer (990 μl) at 37 °C during 5 min and then 10 μl of an alcoholic solution of mycotoxin (concentration 100 times higher than the final concentration required in the test tube) were added. After incubation, the solution was centrifuged, and the amount of mycotoxins were analysed both in the supernatant and in the residue. A plateau of binding was reached after 15 min of incubation whatever the mycotoxins and the concentrations tested. The adsorption of ZEA was better at pH 5 (75 %), versus 60 % at pH 3 and 7. OTA was only significantly adsorbed at pH 3 (50 %). Depending on the pH, the adsorptions of OTA or ZEA were increased or decreased when they were together, indicative of a cooperative effect.

摘要

迄今为止,尚无官方方法可准确界定结合剂的结合能力。目标是确定用于测定结合效果的通用体外参数(平衡时间、pH值、霉菌毒素/结合剂比例),这些参数可用于计算相关的平衡吸附常数。为此,将黄曲霉毒素B1(AFB1)、玉米赤霉烯酮(ZEA)或赭曲霉毒素A(OTA)与一种酵母细胞壁在pH 3、pH 5或pH 7的缓冲液中孵育。通过对上清液中残留霉菌毒素的定量以及吸附在残渣上的霉菌毒素量来记录吸附百分比。当仅基于上清液中残留的霉菌毒素进行分析时,在缓冲液中溶解的霉菌毒素存在下酵母细胞壁的孵育导致了意外的高吸附百分比。上清液中霉菌毒素的减少与残渣中发现的霉菌毒素量无关。因此,我们修改了孵育条件。将酵母细胞壁(5毫克)在37℃下于缓冲液(990微升)中预孵育5分钟,然后加入10微升霉菌毒素的酒精溶液(浓度比试管中所需的最终浓度高100倍)。孵育后,将溶液离心,并对上清液和残渣中的霉菌毒素量进行分析。无论所测试的霉菌毒素和浓度如何,孵育15分钟后达到结合平台期。ZEA在pH 5时的吸附效果更好(75%),而在pH 3和pH 7时为60%。OTA仅在pH 3时显著吸附(50%)。根据pH值的不同,当OTA和ZEA同时存在时,它们的吸附会增加或减少,表明存在协同效应。

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