用于高效检测生物液体中人血清白蛋白的荧光探针的分子工程学研究

Raja Chinnappan , Tanveer Ahmad Mir , Shanmugam Easwaramoorthi , Gopika Sunil , Ancy Feba , Balamurugan Kanagasabai , Shadil Ibrahim Wani , Maram N. Sandouka , Alaa Alzhrani , Sandhanasamy Devanesan , Mohamad S. AlSalhi , Naresh Kumar Mani , Wael Al-Kattan , Ahmed Yaqinuddin , Abdullah M. Assiri , Dieter C. Broering
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引用次数: 0

摘要

人血清白蛋白(HSA)由肝脏合成,占脊椎动物血液中血浆蛋白总量的 60%。它是健康人血液中最主要的细胞外血浆蛋白,是外源性和内源性物质的储存器和转运器。人体内白蛋白浓度降低或含量异常,预示着肝脏、肾脏和消化系统相关疾病的发生。因此,准确定量 HSA 对白蛋白相关疾病的诊断检测和常规临床分析具有重要意义。本文合成了一类具有分子内电荷转移(TICT)诱导发射特性的双功能荧光分子--三苯胺罗丹宁-3-乙酸(mRA),并将其用作荧光检测人类白蛋白的新型传感探针。mRA 可通过与血清白蛋白结合分子的位点特异性相互作用而选择性发光,并显示出更强的光物理或生物响应功效。为了从分子水平上理解 mRA 与 HSA 的相互作用,我们采用了对接方法来探索位点特异性相互作用现象。由此产生的荧光策略在 0.01-400 μg/ml 浓度范围内与 HSA 相互作用时产生了剂量依赖性信号响应增强。该传感器探针的检测限低至 10 纳克/毫升,是分析复杂生物液体中 HSA 的一种可行、低成本且有效的方法,可用于白蛋白相关疾病的早期检测和诊断。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Molecular engineering of a fluorescent probe for highly efficient detection of human serum albumin in biological fluid

Molecular engineering of a fluorescent probe for highly efficient detection of human serum albumin in biological fluid
Human serum albumin (HSA) is synthesized by the liver, accounting for 60 % of total plasma protein in vertebrates' blood. It is the most predominant extracellular plasma protein that acts as a repository and transporter of exogenous and endogenous substances in the blood of healthy humans. Decreased albumin concentration in the human body or its abnormal levels indicate the occurrence of hepatic, renal, and digestive-related diseases. Therefore, accurate quantification of HSA is of great significance in diagnostic testing and routine clinical analysis of albumin-linked diseases. Herein, a class of triphenylamine rhodanine-3-acetic acid (mRA)-a bifunctional fluorescent molecule with twisted intramolecular charge transfer (TICT)-induced emission characteristics is synthesized and employed as a novel sensing probe for the fluorescent detection of human albumin. mRA can be selectively lighted up through site-specific interactions with serum albumin-binding moieties and show enhanced photophysical or biological response efficacy. Understanding the interaction of mRA with HSA at the molecular level was carried out using docking methodology to explore the site-specific interaction phenomenon. The resulting fluorescence strategy produced a dose-dependent signal response enhancement upon interaction with HSA in the concentration range of 0.01–400 μg/ml. The sensor probe exhibits a low detection limit of 10 ng/mL and is found to be a feasible, low-cost, and effective approach for HSA analysis in complex biological fluids for early detection and diagnosis of albumin-related diseases.
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