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基于量子点-酶偶联物的分析纳米球传感器用于尿素和肌酐的检测。

Analytical nanosphere sensors using quantum dot-enzyme conjugates for urea and creatinine.

机构信息

Institute of Biotechnology, Department of Chemical Engineering and Biotechnology, University of Cambridge, Tennis Court Road, Cambridge CB2 1QT, United Kingdom.

出版信息

Anal Chem. 2010 Nov 1;82(21):9043-9. doi: 10.1021/ac101838n. Epub 2010 Oct 12.

Abstract

An enzyme-linked analytical nanosphere sensor (ANSor) is described, responding to enzyme-substrate turnover in the vicinity of a quantum dot (QD) due to coimmobilized enzyme and pH sensitive ligand. QD capping by mercapto-alkanoic acids were rejected as a pH sensitive ligand, but with the use of a layer-by-layer assembly on mercaptopropionic capped QDs and an intermediate poly(allylamine hydrochloride) layer, anthraquinone sulfonate (calcium red, CaR) was introduced to modify the pKa in the immobilized system > 8. QD-CaR absorption shows spectral overlap with QD530 emission at all pHs and gives a complex pH dependent fluorescence resonance energy transfer (FRET) efficiency, due to excited state proton transfer (λ(ex) = 540 nm; λ(em) = 585 nm). In contrast QD615-CaR with spectral overlap between the QD and CaR gave a strong and reproducible pH response. QD-urease and QD-creatinine deiminase conjugates could be linked with pH changes produced by enzyme degradation of urea and creatinine, respectively. Close coupling between the pH sensitive QD and enzyme conjugate maximized signal compared with solution based assays: QD-urease and QD-CD bioconjugates were tested in model biological media (Dulbecco's modified Eagle's Medium and fetal calf serum) and in urine, showing a response in 3-4 min.

摘要

一种酶联分析纳米球传感器(ANSor)被描述为,由于共固定的酶和 pH 敏感配体,在量子点(QD)附近响应酶底物的转化。巯基烷酸作为 pH 敏感配体被排除在外,但通过在巯基丙酸封端的 QD 上进行层层组装和中间聚(盐酸烯丙胺)层,蒽醌磺酸盐(钙红,CaR)被引入以修饰固定化系统中的 pKa > 8。QD-CaR 吸收在所有 pH 值下都与 QD530 发射光谱重叠,并由于激发态质子转移(λ(ex)= 540nm;λ(em)= 585nm)而产生复杂的 pH 依赖荧光共振能量转移(FRET)效率。相比之下,QD615-CaR 与 QD 和 CaR 之间的光谱重叠,产生了强烈且可重复的 pH 响应。QD-脲酶和 QD-肌氨酸脱氨酶缀合物可以与分别由脲酶和肌氨酸脱氨酶降解产生的 pH 变化相连接。pH 敏感 QD 与酶缀合物的紧密偶联与基于溶液的测定相比最大化了信号:QD-脲酶和 QD-CD 生物缀合物在模型生物介质(Dulbecco 改良 Eagle 培养基和胎牛血清)和尿液中进行了测试,在 3-4 分钟内显示出响应。

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