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利用针对细胞表面成分的双标记适体捕获和检测金黄色葡萄球菌。

Capture and detection of Staphylococcus aureus with dual labeled aptamers to cell surface components.

作者信息

Ramlal Shylaja, Mondal Bhairab, Lavu Padma Sudharani, N Bhavanashri, Kingston Joseph

机构信息

Microbiology Division, Defence Food Research Laboratory, Siddarthanagar, Mysore, Karnataka 570011, India.

Microbiology Division, Defence Food Research Laboratory, Siddarthanagar, Mysore, Karnataka 570011, India.

出版信息

Int J Food Microbiol. 2018 Jan 16;265:74-83. doi: 10.1016/j.ijfoodmicro.2017.11.002. Epub 2017 Nov 7.

DOI:10.1016/j.ijfoodmicro.2017.11.002
PMID:29132030
Abstract

In the present study, a high throughput whole cell SELEX method has been applied successfully in selecting specific aptamers against whole cells of Staphylococcus aureus, a potent food poisoning bacterium. A total ten rounds of SELEX and three rounds of intermittent counter SELEX, was performed to obtain specific aptamers. Obtained oligonucleotide pool were cloned, sequenced and then grouped into different families based on their primary sequence homology and secondary structure similarity. FITC labeled sequences from different families were selected for further characterization via flow cytometry analysis. The dissociation constant (K) values of specific and higher binders ranged from 34 to 128nM. Binding assays to assess the selectivity of aptamer RAB10, RAB 20, RAB 28 and RAB 35 demonstrated high affinity against S. aureus and low binding affinity for other bacteria. To demonstrate the potential use of the aptamer a sensitive dual labeled sandwich detection system was developed using aptamer RAB10 and RAB 35 with a detection limit of 10CFU/mL. Furthermore detection from mixed cell population and spiked sample emphasized the robustness as well as applicability of the developed method. Altogether, the established assay could be a reliable detection tool for the routine investigation of Staphylococcus aureus in samples from food and clinical sources.

摘要

在本研究中,一种高通量全细胞SELEX方法已成功应用于筛选针对金黄色葡萄球菌(一种强效食物中毒细菌)全细胞的特异性适体。进行了总共十轮SELEX和三轮间歇反SELEX,以获得特异性适体。将获得的寡核苷酸池进行克隆、测序,然后根据其一级序列同源性和二级结构相似性分为不同家族。从不同家族中选择FITC标记的序列,通过流式细胞术分析进行进一步表征。特异性和高结合力适体的解离常数(K)值范围为34至128nM。评估适体RAB10、RAB20、RAB28和RAB35选择性的结合试验表明,它们对金黄色葡萄球菌具有高亲和力,而对其他细菌的结合亲和力较低。为了证明适体的潜在用途,使用适体RAB10和RAB35开发了一种灵敏的双标记夹心检测系统,检测限为10CFU/mL。此外,从混合细胞群体和加标样品中的检测强调了所开发方法的稳健性和适用性。总之,所建立的检测方法可以成为食品和临床来源样品中金黄色葡萄球菌常规检测的可靠工具。

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