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Optimized microscale detection of amino acid decarboxylase for rapid screening of Salmonella in the selective enrichment step

机译:优化的微量氨基酸脱羧酶检测方法,用于在选择性富集步骤中快速筛选沙门氏菌

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摘要

To develop a high-throughput spectrophotometric screen for Salmonella contamination, modified amino acid decarboxylase broths with pH indicators supplemented with selective agents were studied in microwell plates. The goal was to develop a rapid, reliable, and efficient procedure for resource-poor settings or food industry with large sample numbers. Detection depends on the broth changing from neutral to acidic pH due to sugar fermentation reflecting cell growth and then to basic due to decarboxylase generating amines, indicating presence of decarboxylase-positive bacteria. The visible absorption spectra of three pH indicators that change color at neutral pH were compared from pH 4.5 to 9. In the modified decarboxylase broth, phenol red showed the largest 550 nm absorbance changes when the pH was shifted from neutral to acidic and basic compared to bromocresol purple and bromothymol blue. Most of tested Salmonella serovars rapidly and specifically metabolized ornithine and lysine and showed positive decarboxylase activity (red broth turning pink) within 6-8 h. All Salmonella serovars possessed arginine decarboxylase, but arginine metabolism took at least 24 h to attain pink broth. Salmonella Typhi and Salmonella Paratyphi A are void of ornithine and lysine decarboxylases, respectively. Therefore, both ornithine and lysine were used as decarboxylase substrates in the selective enrichment media formulated to detect all Salmonella serovars. Three selective inhibitors: magnesium chloride, novobiocin, and magnesium chloride with malachite green (from Rappaport-Vasilliadis soy broth) were chosen to be included in seven new amino acid decarboxylase broths. They were tested for their ability to screen for Salmonella contamination in the selective enrichment step. Collectively, the broth formulations with different amino acid substrates and selective inhibitors not only identified decarboxylase-positive bacteria, but further distinguished between decarboxylase-positive salmonellae and non-salmonellae. The developed screening method was tested on some naturally- and artificially-contaminated food samples of different matrices; homogeneous liquid (pasteurized milk), solid (cooked chicken), and complex food matrix (ready-to-eat food). With proper sample pre-enrichment, this procedure with its seven newly developed broths could reliably and rapidly identify food samples with Salmonella contamination without risking false negative results. (C) 2016 Elsevier Ltd. All rights reserved.
机译:为了开发高通量沙门氏菌污染的分光光度筛,在微孔板上研究了带有pH指示剂和选择剂的改性氨基酸脱羧酶肉汤。目的是为资源匮乏的环境或具有大量样本的食品工业开发一种快速,可靠和高效的程序。检测取决于肉汤(由于糖的发酵反映了细胞的生长)从中性变为酸性pH,然后由于产生脱羧酶的胺而变为碱性,表明存在脱羧酶阳性细菌。比较了三种pH指示剂在中性pH时的颜色从pH 4.5到9的可见吸收光谱。在改性脱羧酶肉汤中,当pH从中性变为酸性和碱性时,酚红显示最大的550 nm吸光度变化。溴甲酚紫和溴百里酚蓝。大多数测试的沙门氏菌血清会快速且特异地代谢鸟氨酸和赖氨酸,并在6-8小时内显示出正的脱羧酶活性(红色肉汤变成粉红色)。所有沙门氏菌血清型均具有精氨酸脱羧酶,但精氨酸代谢至少需要24小时才能获得粉红色肉汤。伤寒沙门氏菌和副伤寒沙门氏菌A分别不含鸟氨酸和赖氨酸脱羧酶。因此,在配制用于检测所有沙门氏菌血清型的选择性富集培养基中,鸟氨酸和赖氨酸均用作脱羧酶底物。选择了三种选择性抑制剂:氯化镁,新生霉素和带有孔雀石绿的氯化镁(来自Rappaport-Vasilliadis大豆肉汤),包含在七个新的氨基酸脱羧酶肉汤中。测试了他们在选择性富集步骤中筛选沙门氏菌污染的能力。集体地,具有不同氨基酸底物和选择性抑制剂的肉汤制剂不仅鉴定出脱羧酶阳性细菌,而且进一步区分了脱羧酶阳性沙门氏菌和非沙门氏菌。在一些自然和人工污染的不同基质食品样品上测试了开发的筛选方法。均质液体(巴氏杀菌牛奶),固体(熟鸡肉)和复杂的食品基质(即食食品)。通过适当的样品预富集,此程序及其7种新开发的肉汤可以可靠,快速地鉴定出沙门氏菌污染的食物样品,而不会冒假阴性结果的风险。 (C)2016 Elsevier Ltd.保留所有权利。

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