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阿特罗克级别的光诱导抗原抗体结合被限制在微流中。

Attogram-level light-induced antigen-antibody binding confined in microflow.

机构信息

Department of Physical Science, Graduate School of Science, Osaka Prefecture University, 1-2 Gakuencho, Nakaku, Sakai, Osaka, 599-8570, Japan.

Research Institute for Light-induced Acceleration System (RILACS), Osaka Prefecture University, 1-2 Gakuencho, Nakaku, Sakai, Osaka, 599-8570, Japan.

出版信息

Commun Biol. 2022 Oct 6;5(1):1053. doi: 10.1038/s42003-022-03946-0.

Abstract

The analysis of trace amounts of proteins based on immunoassays and other methods is essential for the early diagnosis of various diseases such as cancer, dementia, and microbial infections. Here, we propose a light-induced acceleration of antigen-antibody reaction of attogram-level proteins at the solid-liquid interface by tuning the laser irradiation area comparable to the microscale confinement geometry for enhancing the collisional probability of target molecules and probe particles with optical force and fluidic pressure. This principle was applied to achieve a 10-fold higher sensitivity and ultrafast specific detection in comparison with conventional protein detection methods (a few hours) by omitting any pretreatment procedures; 47-750 ag of target proteins were detected in 300 nL of sample after 3 minutes of laser irradiation. Our findings can promote the development of proteomics and innovative platforms for high-throughput bio-analyses under the control of a variety of biochemical reactions.

摘要

基于免疫测定和其他方法的痕量蛋白质分析对于癌症、痴呆症和微生物感染等各种疾病的早期诊断至关重要。在这里,我们通过调整激光照射面积来提出一种在固液界面处加速阿伏伽德罗级蛋白质的抗原抗体反应的方法,该面积与微尺度约束几何形状相当,以提高目标分子和探针粒子与光学力和流体压力的碰撞概率。通过省略任何预处理程序,与传统的蛋白质检测方法(数小时)相比,该原理实现了 10 倍更高的灵敏度和超快特异性检测;在 3 分钟的激光照射后,在 300 nL 的样品中检测到了 47-750 ag 的目标蛋白。我们的发现可以促进蛋白质组学的发展,并为在各种生化反应控制下的高通量生物分析创新平台提供支持。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0bf6/9537419/413347747af7/42003_2022_3946_Fig1_HTML.jpg

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