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使用纳米等离子体生物传感器微阵列的多重血清细胞因子免疫测定。

Multiplex serum cytokine immunoassay using nanoplasmonic biosensor microarrays.

作者信息

Chen Pengyu, Chung Meng Ting, McHugh Walker, Nidetz Robert, Li Yuwei, Fu Jianping, Cornell Timothy T, Shanley Thomas P, Kurabayashi Katsuo

机构信息

†Department of Mechanical Engineering, University of Michigan, Ann Arbor, Michigan 48109, United States.

‡Department of Pediatrics and Communicable Diseases, University of Michigan, Ann Arbor, Michigan 48109, United States.

出版信息

ACS Nano. 2015;9(4):4173-81. doi: 10.1021/acsnano.5b00396. Epub 2015 Mar 23.

Abstract

Precise monitoring of the rapidly changing immune status during the course of a disease requires multiplex analysis of cytokines from frequently sampled human blood. However, the current lack of rapid, multiplex, and low volume assays makes immune monitoring for clinical decision-making (e.g., critically ill patients) impractical. Without such assays, immune monitoring is even virtually impossible for infants and neonates with infectious diseases and/or immune mediated disorders as access to their blood in large quantities is prohibited. Localized surface plasmon resonance (LSPR)-based microfluidic optical biosensing is a promising approach to fill this technical gap as it could potentially permit real-time refractometric detection of biomolecular binding on a metallic nanoparticle surface and sensor miniaturization, both leading to rapid and sample-sparing analyte analysis. Despite this promise, practical implementation of such a microfluidic assay for cytokine biomarker detection in serum samples has not been established primarily due to the limited sensitivity of LSPR biosensing. Here, we developed a high-throughput, label-free, multiarrayed LSPR optical biosensor device with 480 nanoplasmonic sensing spots in microfluidic channel arrays and demonstrated parallel multiplex immunoassays of six cytokines in a complex serum matrix on a single device chip while overcoming technical limitations. The device was fabricated using easy-to-implement, one-step microfluidic patterning and antibody conjugation of gold nanorods (AuNRs). When scanning the scattering light intensity across the microarrays of AuNR ensembles with dark-field imaging optics, our LSPR biosensing technique allowed for high-sensitivity quantitative cytokine measurements at concentrations down to 5-20 pg/mL from a 1 μL serum sample. Using the nanoplasmonic biosensor microarray device, we demonstrated the ability to monitor the inflammatory responses of infants following cardiopulmonary bypass (CPB) surgery through tracking the time-course variations of their serum cytokines. The whole parallel on-chip assays, which involved the loading, incubation, and washing of samples and reagents, and 10-fold replicated multianalyte detection for each sample using the entire biosensor arrays, were completed within 40 min.

摘要

在疾病过程中精确监测快速变化的免疫状态需要对频繁采集的人体血液中的细胞因子进行多重分析。然而,目前缺乏快速、多重且低体积的检测方法,使得用于临床决策(如重症患者)的免疫监测不切实际。没有这样的检测方法,对于患有传染病和/或免疫介导疾病的婴儿和新生儿来说,免疫监测几乎是不可能的,因为禁止大量采集他们的血液。基于局域表面等离子体共振(LSPR)的微流控光学生物传感是填补这一技术空白的一种有前途的方法,因为它有可能实现对金属纳米颗粒表面生物分子结合的实时折射检测以及传感器小型化,这两者都能实现快速且节省样品的分析物分析。尽管有这样的前景,但这种用于血清样品中细胞因子生物标志物检测的微流控检测方法尚未实际应用,主要原因是LSPR生物传感的灵敏度有限。在此,我们开发了一种高通量、无标记、多阵列的LSPR光学生物传感器装置,该装置在微流控通道阵列中有480个纳米等离子体传感点,并展示了在单个装置芯片上对复杂血清基质中的六种细胞因子进行平行多重免疫测定,同时克服了技术限制。该装置是使用易于实施的一步微流控图案化和金纳米棒(AuNRs)的抗体偶联制备的。当用暗场成像光学系统扫描AuNR集合的微阵列上的散射光强度时,我们的LSPR生物传感技术能够对1 μL血清样品中低至5 - 20 pg/mL浓度的细胞因子进行高灵敏度定量测量。使用纳米等离子体生物传感器微阵列装置,我们展示了通过跟踪婴儿血清细胞因子的时间进程变化来监测体外循环(CPB)手术后婴儿炎症反应的能力。整个平行芯片检测,包括样品和试剂的加载、孵育和洗涤,以及使用整个生物传感器阵列对每个样品进行10倍重复的多分析物检测,在40分钟内完成。

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