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Rapid Multiplexed Flow Cytometric Assay for Botulinum Neurotoxin Detection Using an Automated Fluidic Microbead-Trapping Flow Cell for Enhanced Sensitivity

机译:快速多路流式细胞术检测肉毒杆菌神经毒素,使用自动流体微珠捕获流动池增强灵敏度

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摘要

A bead-based sandwich immunoassay for botulinum neurotoxin serotype A (BoNT/A) has been developed and demonstrated using a recombinant 50 kDa fragment (BoNT/A-HC-fragment) of the BoNT/A heavy chain (BoNT/A-HC) as a structurally valid simulant. Three different anti-BoNT/A antibodies were attached to three different fluorescent dye encoded flow cytometry beads for multiplexing. The assay was conducted in two formats: a manual microcentrifuge tube format and an automated fluidic system format. Flow cytometry detection was used for both formats. The fluidic system used a novel microbead-trapping flow cell to capture antibody-coupled beads with subsequent sequential perfusion of sample, wash, dye-labeled reporter antibody, and final wash solutions. After the reaction period, the beads were collected for analysis by flow cytometry. Sandwich assays performed on the fluidic system gave median fluorescence intensity signals on the flow cytometer that were 2-4 times higher than assays performed manually in the same amount of time. Limits of detection were estimated at 1 pM (approx50 pg/mL for BoNT/A-HC-fragment) for the 15 min fluidic assay in buffer.
机译:已开发出基于珠子的肉毒杆菌神经毒素血清型A(BoNT / A)夹心免疫测定法,并使用BoNT / A重链(BoNT / A-HC)的50 kDa重组片段(BoNT / A-HC片段)进行了证明作为结构上有效的模拟物。将三种不同的抗BoNT / A抗体连接到三种不同的荧光染料编码的流式细胞仪珠子上进行多重化。该测定以两种形式进行:手动微量离心管形式和自动流体系统形式。流式细胞术检测用于两种形式。流体系统使用了新型的捕获微珠的流通池来捕获抗体偶联的微珠,随后依次进行样品,洗涤液,染料标记的报告抗体和最终洗涤液的灌注。反应期后,收集珠子用于流式细胞仪分析。在流体系统上进行的夹心测定在流式细胞仪上给出的中值荧光强度信号比在相同时间内手动进行的测定高2-4倍。在缓冲液中进行15分钟的流体分析时,检测限估计为1 pM(BoNT / A-HC片段约为50 pg / mL)。

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