Development of molecular approach based on PCR assay for detection of histamine producing bacteria.

IF 2.6 3区 农林科学 Q2 FOOD SCIENCE & TECHNOLOGY Journal of Food Science and Technology-mysore Pub Date : 2016-01-01 Epub Date: 2015-08-13 DOI:10.1007/s13197-015-1982-1
Karn Wongsariya, Nuntavan Bunyapraphatsara, Montri Yasawong, Mullika Traidej Chomnawang
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Abstract

Histamine fish poisoning becomes highly concern not only in public health but also economic aspect. Histamine is produced from histidine in fish muscles by bacterial decarboxylase enzyme. Several techniques have been developed to determine the level of histamine in fish and their products but the effective method for detecting histamine producing bacteria is still required. This study was attempted to detect histamine producing bacteria by newly developed PCR condition. Histamine producing bacteria were isolated from scombroid fish and determined the ability to produce histamine of isolated bacteria by biochemical and TLC assays. PCR method was developed to target the histidine decarboxylase gene (hdc). The result showed that fifteen histamine producing bacterial isolates and three standard strains produced an amplicon at the expected size of 571 bp after amplified by PCR using Hdc_2F/2R primers. Fifteen isolates of histamine producing bacteria were classified as M. morganii, E. aerogenes, and A. baumannii. The lowest detection levels of M. morganii and E. aerogenes were 10(2) and 10(5) Cfu/mL in culture media and 10(3) and 10(6) Cfu/mL in fish homogenates, respectively. The limit of detection by this method was clearly shown to be sensitive because the primers could detect the presence of M. morganii and E. aerogenes before the histamine level reached the regulation level at 50 ppm. Therefore, this PCR method exhibited the potential efficiency for detecting the hdc gene from histamine producing bacteria and could be used to prevent the proliferation of histamine producing bacteria in fish and fish products.

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开发基于 PCR 检测法的分子方法,用于检测组胺产生菌。
组胺鱼类中毒不仅在公共卫生方面受到高度关注,在经济方面也是如此。组胺是通过细菌脱羧酶从鱼类肌肉中的组氨酸产生的。目前已开发出多种技术来确定鱼类及其产品中组胺的含量,但仍需要一种有效的方法来检测产生组胺的细菌。本研究尝试利用新开发的 PCR 条件检测组胺细菌。研究人员从鲭鱼中分离出了产组胺细菌,并通过生化和 TLC 检测法确定了分离细菌产生组胺的能力。针对组氨酸脱羧酶基因(hdc)开发了 PCR 方法。结果表明,15株产生组胺的细菌分离株和3株标准菌株在使用Hdc_2F/2R引物进行PCR扩增后,产生了预期大小为571 bp的扩增片段。15 株产组胺细菌被归类为摩根氏菌、产气荚膜杆菌和鲍曼不动杆菌。摩根氏菌和产气埃希氏菌在培养基中的最低检测水平分别为 10(2) 和 10(5) Cfu/mL,在鱼匀浆中的最低检测水平分别为 10(3) 和 10(6) Cfu/mL。这种方法的检测限显然是灵敏的,因为引物可以在组胺水平达到 50 ppm 的规定水平之前检测到摩根氏菌和产气埃希氏菌的存在。因此,该PCR方法具有检测组胺产生菌hdc基因的潜在效率,可用于防止鱼类和水产品中组胺产生菌的增殖。
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来源期刊
CiteScore
7.70
自引率
0.00%
发文量
274
审稿时长
11 months
期刊介绍: The Journal of Food Science and Technology (JFST) is the official publication of the Association of Food Scientists and Technologists of India (AFSTI). This monthly publishes peer-reviewed research papers and reviews in all branches of science, technology, packaging and engineering of foods and food products. Special emphasis is given to fundamental and applied research findings that have potential for enhancing product quality, extend shelf life of fresh and processed food products and improve process efficiency. Critical reviews on new perspectives in food handling and processing, innovative and emerging technologies and trends and future research in food products and food industry byproducts are also welcome. The journal also publishes book reviews relevant to all aspects of food science, technology and engineering.
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