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通过斑点印迹法和聚合酶链反应快速检测和区分家禽样本中重要的弯曲杆菌属菌种。

Rapid detection and differentiation of important Campylobacter spp. in poultry samples by dot blot and PCR.

作者信息

Fontanot Marco, Iacumin Lucilla, Cecchini Francesca, Comi Giuseppe, Manzano Marisa

机构信息

Department of Food Science, University of Udine, Via Sondrio 2/A, 33100 Udine, Italy.

Department of Food Science, University of Udine, Via Sondrio 2/A, 33100 Udine, Italy.

出版信息

Food Microbiol. 2014 Oct;43:28-34. doi: 10.1016/j.fm.2014.05.001. Epub 2014 May 14.

DOI:10.1016/j.fm.2014.05.001
PMID:24929879
Abstract

The detection of Campylobacter, the most commonly reported cause of foodborne gastroenteritis in the European Union, is very important for human health. The most commonly recognised risk factor for infection is the handling and/or consumption of undercooked poultry meat. The methods typically applied to evaluate the presence/absence of Campylobacter in food samples are direct plating and/or enrichment culture based on the Horizontal Method for Detection and Enumeration of Campylobacter spp. (ISO 10272-1B: 2006) and PCR. Molecular methods also allow for the detection of cells that are viable but cannot be cultivated on agar media and that decrease the time required for species identification. The current study proposes the use of two molecular methods for species identification: dot blot and PCR. The dot blot method had a sensitivity of 25 ng for detection of DNA extracted from a pure culture using a digoxigenin-labelled probe for hybridisation; the target DNA was extracted from the enrichment broth at 24 h. PCR was performed using a pair of sensitive and specific primers for the detection of Campylobacter jejuni and Campylobacter coli after 24 h of enrichment in Preston broth. The initial samples were contaminated by 5 × 10 C. jejuni cells/g and 1.5 × 10(2)C. coli cells/g, thus the number of cells present in the enrichment broth at 0 h was 1 or 3 cell/g, respectively.

摘要

弯曲杆菌是欧盟报告中最常见的食源性肠胃炎病因,其检测对人类健康非常重要。最常见的感染风险因素是处理和/或食用未煮熟的禽肉。通常用于评估食品样本中弯曲杆菌存在与否的方法是基于弯曲杆菌属检测和计数水平方法(ISO 10272-1B: 2006)的直接平板接种和/或富集培养以及聚合酶链反应(PCR)。分子方法还能够检测出在琼脂培养基上无法培养但仍存活的细胞,并且缩短了菌种鉴定所需的时间。本研究提出使用两种分子方法进行菌种鉴定:斑点印迹法和PCR。斑点印迹法使用地高辛标记的探针进行杂交,检测从纯培养物中提取的DNA时灵敏度为25纳克;目标DNA在24小时时从富集肉汤中提取。在普雷斯顿肉汤中富集24小时后,使用一对灵敏且特异的引物进行PCR,以检测空肠弯曲杆菌和结肠弯曲杆菌。初始样本被每克5×10个空肠弯曲杆菌细胞和每克1.5×10²个结肠弯曲杆菌细胞污染,因此在0小时时富集肉汤中的细胞数分别为每克1个或3个细胞。

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