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基于发光的酶标记噬菌体(Phazyme)检测法用于快速检测产志贺毒素大肠杆菌血清群。

Luminescence based enzyme-labeled phage (Phazyme) assays for rapid detection of Shiga toxin producing Escherichia coli serogroups.

作者信息

Willford John D, Bisha Bledar, Bolenbaugh Kyle E, Goodridge Lawrence D

机构信息

Department of Animal Science; University of Wyoming; Laramie, WY USA.

出版信息

Bacteriophage. 2011 Mar;1(2):101-110. doi: 10.4161/bact.1.2.15666.

Abstract

Most diagnostic approaches for Shiga toxin producing Escherichia coli (STEC) have been designed to detect only serogroup O157 that causes a majority, but not all STEC related outbreaks in the United States. Therefore, there is a need to develop methodology that would enable the detection of other STEC serogroups that cause disease. Three bacteriophages (phages) that infect STEC serogroups O26, O103, O111, O145 and O157 were chemically labeled with horseradish peroxidase (HRP). The enzyme-labeled phages (Phazymes) were individually combined with a sampling device (a swab), STEC serogroup-specific immunomagnetic separation (IMS) beads, bacterial enrichment broth and luminescent HRP substrate, in a self-contained test device, while luminescence was measured in a hand-held luminometer.The O26 and O157 Phazyme assays correctly identified more than 93% of the bacteria tested during this study, the O123 Phazyme assay identified 89.6%, while the O111 and O145 Phazyme assays correctly detected 82.4% and 75.9%, respectively. The decreased specificity of the O111 and O145 assays was related to the broad host ranges of the phages used in both assays. The Phazyme assays were capable of directly detecting between 10(5) and 10(6) CFU/ml in pure culture, depending on the serogroup. In food trials, the O157 Phazyme assay was able to detect E. coli O157:H7 in spinach consistently at levels of 1 CFU/g and occasionally at levels of 0.1 CFU/g. The assay detected 10(0) CFU/100 cm(2) on swabbed meat samples and 10(2) CFU/100 ml in water samples. The Phazyme assay effectively detects most STEC in a simple and rapid manner, with minimal need for instrumentation to interpret the test result.

摘要

大多数针对产志贺毒素大肠杆菌(STEC)的诊断方法仅设计用于检测血清型O157,在美国,该血清型导致了大多数但并非所有与STEC相关的疫情爆发。因此,有必要开发能够检测其他致病STEC血清型的方法。三种感染STEC血清型O26、O103、O111、O145和O157的噬菌体用辣根过氧化物酶(HRP)进行化学标记。酶标记噬菌体(噬菌体酶)分别与采样装置(拭子)、STEC血清型特异性免疫磁珠分离(IMS)、细菌增菌肉汤和发光HRP底物组合在一个独立的测试装置中,同时用手持式发光计测量发光情况。在本研究中,O26和O157噬菌体酶检测法正确鉴定了超过93%的受试细菌,O123噬菌体酶检测法鉴定出89.6%,而O111和O145噬菌体酶检测法分别正确检测出82.4%和75.9%。O111和O145检测法特异性降低与两种检测法中使用的噬菌体宿主范围广泛有关。噬菌体酶检测法能够在纯培养物中直接检测到每毫升10⁵至10⁶个菌落形成单位(CFU),具体取决于血清型。在食品试验中,O157噬菌体酶检测法能够始终检测到菠菜中每克1个CFU的大肠杆菌O157:H7,偶尔能检测到每克0.1个CFU的水平。该检测法在擦拭的肉类样本上检测到每100平方厘米10⁰个CFU,在水样中检测到每100毫升10²个CFU。噬菌体酶检测法以简单快速的方式有效检测大多数STEC,解读检测结果所需仪器最少。

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