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采用 aflR-aflJ 基因间隔区 PCR-RFLP 分析技术对纯培养和黄曲霉毒素污染葡萄中黄曲霉和寄生曲霉的鉴别。

Differentiation between Aspergillus flavus and Aspergillus parasiticus from pure culture and aflatoxin-contaminated grapes using PCR-RFLP analysis of aflR-aflJ intergenic spacer.

机构信息

Centre d'analyses et de recherches, Faculté des Sciences, Univ. Saint-Joseph, Beyrouth, Liban.

出版信息

J Food Sci. 2011 May;76(4):M247-53. doi: 10.1111/j.1750-3841.2011.02153.x. Epub 2011 Apr 14.

Abstract

Aflatoxins (AFs) represent the most important single mycotoxin-related food safety problem in developed and developing countries as they have adverse effects on human and animal health. They are produced mainly by Aspergillus flavus and A. parasiticus. Both species have different aflatoxinogenic profile. In order to distinguish between A. flavus and A. parasiticus, gene-specific primers were designed to target the intergenic spacer (IGS) for the AF biosynthesis genes, aflJ and aflR. Polymerase chain reaction (PCR) products were subjected to restriction endonuclease analysis using BglII to look for restriction fragment length polymorphisms (RFLPs). Our result showed that both species displayed different PCR-based RFLP (PCR-RFLP) profile. PCR products from A. flavus cleaved into 3 fragments of 362, 210, and 102 bp. However, there is only one restriction site for this enzyme in the sequence of A. parasiticus that produced only 2 fragments of 363 and 311 bp. The method was successfully applied to contaminated grapes samples. This approach of differentiating these 2 species would be simpler, less costly, and quicker than conventional sequencing of PCR products and/or morphological identification.

摘要

黄曲霉毒素(AFs)是发达国家和发展中国家最重要的与单一致病菌相关的食品安全问题,因为它们对人类和动物健康有不良影响。它们主要由黄曲霉(A. flavus)和寄生曲霉(A. parasiticus)产生。这两个物种的产毒谱不同。为了区分黄曲霉和寄生曲霉,设计了针对黄曲霉生物合成基因 aflJ 和 aflR 的基因间 spacer(IGS)的基因特异性引物。聚合酶链反应(PCR)产物用 BglII 进行限制性内切酶分析,以寻找限制性片段长度多态性(RFLP)。我们的结果表明,这两个物种都显示出不同的基于 PCR 的 RFLP(PCR-RFLP)图谱。黄曲霉的 PCR 产物被切割成 362、210 和 102bp 的 3 个片段。然而,在寄生曲霉的序列中,该酶只有一个限制位点,只能产生 363 和 311bp 的 2 个片段。该方法成功应用于污染的葡萄样本。与传统的 PCR 产物测序和/或形态鉴定相比,这种区分这两个物种的方法更简单、成本更低、速度更快。

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