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将纳米颗粒尺寸与膜孔隙率集成,以提高夹心免疫层析分析中的分析性能。

Integrated nanoparticle size with membrane porosity for improved analytical performance in sandwich immunochromatographic assay.

机构信息

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

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

出版信息

Anal Chim Acta. 2021 Jan 2;1141:136-143. doi: 10.1016/j.aca.2020.10.041. Epub 2020 Oct 22.

DOI:10.1016/j.aca.2020.10.041
PMID:33248647
Abstract

The use of luminescent nanobeads to improve the sensitivity of sandwich immunochromatographic assay (ICA) has obtained increasing concern. Illustrating the relationship among luminescent intensity, nanobead size, nitrocellulose membrane aperture, and ICA sensitivity is important for achieving the optimal target detection. Thus, we synthesized six differently sized quantum dot beads (QBs) (95, 140, 180, 235, 325, and 405 nm) as ICA labels and applied them in three aperture membranes (10, 15, and 25 μm). Results indicate that increasing the QB size to less than an appropriate size of 235 nm is beneficial for ICA sensitivity because of the increased fluorescence. However, oversized QBs result in reduced sensitivity due to the decreased diffusion or settlement of the QB on the membrane that causes obvious background signal. The small aperture membrane perfectly matching the QB size contributes to ICA sensitivity by decreasing the migration velocity of the QB probe for increased binding of the QB@analyte complex at the T zone. Consequently, the best detection of hepatitis B surface antigen with a sensitivity of 0.156 ng/mL is achieved using 235 nm QBs in 15 μm membrane. Further performance evaluation of our QB-ICA demonstrates excellent accuracy, selectivity, and practicability. This work provides a new idea to manipulate the sensitivity of sandwich ICA by tuning the QB size and the membrane aperture, and a theoretical guidance for selecting the probe and membrane to achieve the best detection of target analytes.

摘要

使用发光纳米珠来提高夹心免疫层析分析(ICA)的灵敏度已引起越来越多的关注。阐明发光强度、纳米珠尺寸、硝酸纤维素膜孔径和 ICA 灵敏度之间的关系对于实现最佳的目标检测非常重要。因此,我们合成了六种不同尺寸的量子点珠(QBs)(95、140、180、235、325 和 405nm)作为 ICA 标记,并将它们应用于三种孔径的膜(10、15 和 25μm)中。结果表明,将 QB 尺寸增加到小于 235nm 的适当尺寸有利于 ICA 灵敏度,因为荧光增加。然而,过大的 QBs 会导致灵敏度降低,这是由于 QB 在膜上的扩散或沉降减少,导致明显的背景信号。与 QB 尺寸完美匹配的小孔径膜通过降低 QB 探针的迁移速度来提高 T 区 QB@分析物复合物的结合,从而有助于提高 ICA 灵敏度。因此,使用 15μm 膜中的 235nm QB 可实现乙型肝炎表面抗原的最佳检测,灵敏度为 0.156ng/mL。我们的 QB-ICA 的进一步性能评估表明其具有出色的准确性、选择性和实用性。这项工作通过调整 QB 尺寸和膜孔径为操纵夹心 ICA 的灵敏度提供了新的思路,并为选择探针和膜以实现目标分析物的最佳检测提供了理论指导。

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