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低溶解度蛋白质与单壁碳纳米管的共轭策略作为一种灵敏的蛋白酶活性荧光检测方法

Conjugation Strategies for Low Solubility Proteins to Single-Walled Carbon Nanotubes as a Sensitive Fluorescent Assay to Protease Activity.

作者信息

Hejazi Sepehr, Masud Nabila, Hasib Hasibul Hasan, Bertrand Cole, Sarkar Anwesha, Reuel Nigel F

机构信息

Chemical and Biological Engineering - Iowa State University, 618 Bissell Rd, Ames, IA 50011.

Electrical and Computer Engineering - Iowa State University, 618 Bissell Rd, Ames, IA 50011.

出版信息

Adv Mater Interfaces. 2025 Apr 7;12(7). doi: 10.1002/admi.202400713. Epub 2024 Dec 16.

DOI:10.1002/admi.202400713
PMID:40599679
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12208672/
Abstract

Recently, single-walled carbon nanotube-based optical biosensors have been shown to detect hydrolase activity directly on target substrates such as proteins and peptides. This study presents a metastable protein conjugation approach to immobilize more hydrophobic proteins and enhance the sensitivity of protease detection. The method combines covalent conjugation of substrate proteins via carbodiimide chemistry (EDC/NHS) with non-covalent polymer wrapping of SWCNT, in this case, carboxymethyl cellulose. The formation of protein-SWCNT complexes as a result of multi-site conjugation between the proteins and carboxyl groups, enabled iterative pelleting, washing, and resuspension steps to be applied to the probes which allowed for removal of unbound proteins and residual materials, enhancing the sensor's sensitivity by approximately threefold, reaching an LOD of 6.4 ng/ml in a 5 minute reaction. This immobilization approach is applied to the ECM proteins such as gelatin and collagen and used to detect ECM degrading enzymes' activity. ECM degrading enzymes caused a fluorescent intensity decrease of the SWCNT probes, enabling quantification of enzyme concentration between the range 160 ng/ml to 100 µg/ml within 5 minutes of reaction. This hybrid approach provides a rapid and sensitive platform for detecting extracellular degrading enzymes with potential applications in cancer diagnosis and prognosis, wound healing, high-throughput screening for enzyme inhibitors and drug discovery.

摘要

最近,基于单壁碳纳米管的光学生物传感器已被证明能够直接在蛋白质和肽等目标底物上检测水解酶活性。本研究提出了一种亚稳态蛋白质偶联方法,用于固定更多疏水性蛋白质并提高蛋白酶检测的灵敏度。该方法将通过碳二亚胺化学(EDC/NHS)实现的底物蛋白质共价偶联与单壁碳纳米管的非共价聚合物包裹相结合,在本研究中使用的是羧甲基纤维素。蛋白质与羧基之间的多位点偶联形成了蛋白质 - 单壁碳纳米管复合物,使得能够对探针进行反复的沉淀、洗涤和重悬步骤,从而去除未结合的蛋白质和残留物质,将传感器的灵敏度提高了约三倍,在5分钟的反应中检测限达到6.4 ng/ml。这种固定方法应用于明胶和胶原蛋白等细胞外基质蛋白,并用于检测细胞外基质降解酶的活性。细胞外基质降解酶导致单壁碳纳米管探针的荧光强度降低,从而能够在5分钟的反应时间内对160 ng/ml至100 µg/ml范围内的酶浓度进行定量。这种混合方法为检测细胞外降解酶提供了一个快速且灵敏的平台,在癌症诊断和预后、伤口愈合、酶抑制剂的高通量筛选以及药物发现等方面具有潜在应用。

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本文引用的文献

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