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基于杂交链式反应和氧化石墨烯荧光平台的牛奶中沙门氏菌的快速灵敏检测。

Rapid and sensitive detection of Salmonella in milk based on hybridization chain reaction and graphene oxide fluorescence platform.

机构信息

State Key Laboratory of Food Science and Technology, Nanchang University, Nanchang 330047, PR China.

Zystein LLC, Fayetteville, AR 72703.

出版信息

J Dairy Sci. 2021 Dec;104(12):12295-12302. doi: 10.3168/jds.2021-20713. Epub 2021 Sep 16.

Abstract

Salmonella is a foodborne pathogen that has contributed to numerous food safety accidents worldwide, making it necessary to detect contamination at an early stage. A pair of specific primers based on the invA gene of Salmonella was designed for PCR. Target double-stranded DNA (dsDNA) from PCR was purified and denatured at high temperature to obtain target single-stranded DNA (ssDNA). Two carboxyfluorescein-labeled hairpin probes (H1-FAM and H2-FAM) were designed with complementary portions to the ssDNA sequence so that binding could trigger H1-FAM and H2-FAM hybridization chain reaction (HCR) to produce a long dsDNA complex. In this study, graphene oxide (GO) was used in the development of a homogeneous fluorescence detection platform for Salmonella. Using this HCR-GO assay platform, Salmonella detection was completed in 3.5 h. Salmonella was reliably and specifically detected with a limit of detection (LOD) of 4.2 × 10 cfu/mL in pure culture. Moreover, this new HCR-GO assay platform was successfully applied to the detection of Salmonella in artificially contaminated milk with a LOD of 4.2 × 10 cfu/mL.

摘要

沙门氏菌是一种食源性病原体,已导致全球多起食品安全事故,因此有必要尽早发现污染情况。本研究设计了一对基于沙门氏菌 invA 基因的特异性引物,用于 PCR。从 PCR 中提取并纯化目标双链 DNA(dsDNA),然后在高温下变性以获得目标单链 DNA(ssDNA)。设计了两条带有互补部分的羧基荧光素标记发夹探针(H1-FAM 和 H2-FAM),与 ssDNA 序列结合可以触发 H1-FAM 和 H2-FAM 杂交链式反应(HCR),从而产生长 dsDNA 复合物。本研究将氧化石墨烯(GO)用于开发用于沙门氏菌的均相荧光检测平台。使用这种 HCR-GO 分析平台,在纯培养物中可以可靠且特异地检测到沙门氏菌,检测限(LOD)为 4.2×10 cfu/mL。此外,该新的 HCR-GO 分析平台成功应用于人工污染牛奶中沙门氏菌的检测,检测限为 4.2×10 cfu/mL。

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