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利用微流系统中抗体修饰的微颗粒的光力实现细胞外囊泡的超快灵敏度控制和特异性检测。

Ultrafast sensitivity-controlled and specific detection of extracellular vesicles using optical force with antibody-modified microparticles in a microflow system.

机构信息

Department of Physics, Graduate School of Science, Osaka Metropolitan University, 1-2, Gakuen-cho, Naka-ku, Sakai, Osaka 599-8570, Japan.

Research Institute for Light-induced Acceleration System (RILACS), Osaka Metropolitan University, 1-2, Gakuen-cho, Naka-ku, Sakai, Osaka 599-8570, Japan.

出版信息

Nanoscale Horiz. 2023 Jul 24;8(8):1034-1042. doi: 10.1039/d2nh00576j.

Abstract

Extracellular vesicles (EVs), including nanoscale exosomes and ectosomes, hold promise as biomarkers that provide information about the cell of origin through their cargo of nucleic acids and proteins, both on their surface and within. Here, we develop a detection method of EVs based on light-induced acceleration of specific binding between their surface and antibody-modified microparticles, using a controlled microflow with three-dimensional analysis by confocal microscopy. Our method successfully detected 10-10 nanoscale EVs in liquid samples as small as a 500 nanoliters within 5 minutes, with the ability to distinguish multiple membrane proteins. Remarkably, we achieved the specific detection of EVs secreted from living cancer cell lines with high linearity, without the need for a time-consuming ultracentrifugation process that can take several hours. Furthermore, the detection range can be controlled by adjusting the action range of optical force using a defocused laser, consistent with the theoretical calculations. These findings demonstrate an ultrafast, sensitive, and quantitative approach for measuring biological nanoparticles, enabling innovative analyses of cell-to-cell communication and early diagnosis of various diseases, including cancer.

摘要

细胞外囊泡 (EVs),包括纳米级的外泌体和胞外体,有望成为生物标志物,通过其携带的核酸和蛋白质(包括表面和内部)提供有关其来源细胞的信息。在这里,我们开发了一种基于光诱导的 EVs 表面与抗体修饰的微颗粒之间特异性结合加速的检测方法,使用具有三维分析的受控微流来进行共聚焦显微镜分析。我们的方法成功地在小至 500 纳升的液体样本中检测到 10-10 纳米级的 EVs,并且能够区分多种膜蛋白。值得注意的是,我们实现了对来自活癌细胞系分泌的 EVs 的特异性检测,具有高线性度,无需耗时数小时的超速离心过程。此外,通过使用离焦激光调整光力学作用范围,可以控制检测范围,与理论计算一致。这些发现展示了一种超快速、灵敏和定量的测量生物纳米颗粒的方法,为细胞间通讯的创新分析和各种疾病(包括癌症)的早期诊断提供了可能。

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