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两种食源性病原体媒介昆虫(属于“肮脏 22 种”的第 II 组)的多位点遗传特征,这两种昆虫已知会污染食物和食品,并传播食源性致病菌。

Multilocus genetic characterization of two ant vectors (Group II "Dirty 22" species) known to contaminate food and food products and spread foodborne pathogens.

机构信息

U.S. Food and Drug Administration, Southeast Regional Laboratory, 60 Eighth Street, Atlanta, GA 30309, USA.

出版信息

J Food Prot. 2012 Aug;75(8):1447-52. doi: 10.4315/0362-028X.JFP-12-098.

Abstract

The U.S. Food and Drug Administration utilizes the presence of filth and extraneous materials as one of the criteria for implementing regulatory actions and assessing adulteration of food products of public health importance. Twenty-two prevalent pest species (also known as the ''Dirty 22'' species) have been considered by this agency as possible vehicles for the spread of foodborne diseases, and the presence of these species is considered an indicator of unsanitary conditions in food processing and storage facilities. In a previous study, we further categorized the Dirty 22 species into four groups: group I includes four cockroach species, group II includes two ant species, group III includes 12 fly species, and group IV includes four rodent species. Here, we describe the development of three nested PCR primer sets and multilocus genetic characterization by amplifying the small subunit rRNA, elongation factor 1-alpha, and wingless (WNT-1) genes of group II Dirty 22 ant species Monomorium pharaonis and Solenopsis molesta. These novel group II Dirty 22 species-specific nested PCR primer sets can be used when the specimens cannot be identified using conventional microscopic methods. These newly developed assays will provide correct identification of group II Dirty 22 ant species, and the information can be used in the control of foodborne pathogens.

摘要

美国食品和药物管理局将污秽物和杂质的存在作为实施监管行动和评估对公众健康重要的食品产品掺假的标准之一。该机构已经考虑了 22 种常见的害虫物种(也称为“肮脏 22 种”物种),它们可能是食源性疾病传播的媒介,这些物种的存在被认为是食品加工和储存设施卫生条件不佳的指标。在之前的一项研究中,我们进一步将肮脏 22 种物种分为四组:第一组包括四种蟑螂物种,第二组包括两种蚂蚁物种,第三组包括 12 种苍蝇物种,第四组包括四种啮齿动物物种。在这里,我们描述了三种嵌套 PCR 引物组的开发和通过扩增小亚基 rRNA、延伸因子 1-α 和无翅(WNT-1)基因对第二组肮脏 22 种蚂蚁物种法老蚁和红火蚁的多基因特征分析。当使用常规显微镜方法无法识别标本时,可以使用这些新型的第二组肮脏 22 种物种特异性嵌套 PCR 引物组。这些新开发的检测方法将提供对第二组肮脏 22 种蚂蚁物种的正确鉴定,并且可以用于控制食源性病原体。

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