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使用各种烷硫醇单分子层和固定化细胞色素c检测超氧阴离子自由基

Detection of the superoxide radical anion using various alkanethiol monolayers and immobilized cytochrome c.

作者信息

Chen Xiaojun J, West Alan C, Cropek Donald M, Banta Scott

机构信息

Department of Chemical Engineering, Columbia University, New York, New York 10027, USA.

出版信息

Anal Chem. 2008 Dec 15;80(24):9622-9. doi: 10.1021/ac800796b.

Abstract

The superoxide radical anion (SO) is a critical biomarker for monitoring cellular stress responses. Electrochemical SO biosensors are frequently constructed through the covalent immobilization of cytochrome c (Cyt c) onto self-assembled monolayers (SAMs); however, a detailed comparison of these systems as well as configuration influence on SO detection is needed to enable robust applications. Two reaction pathways, oxidation of SO by the SAM-modified gold electrode or electron transfer through a protein and monolayer relay, may be involved during the electrochemical detection of SO with Cyt c, depending on the SAM that is used. Although electrodes with SAMs alone can exhibit a high sensitivity and low limit of detection (LOD) for the SO, they can suffer from a strong response to the presence of interferents such as hydrogen peroxide and ascorbic acid. Electrodes with immobilized Cyt c show decreased sensitivity, but exhibit better selectivity and resistance to fouling in complex media. Considering the trade-offs between sensitivity, selectivity, and LOD for SO detection, a bioelectrode made with Cyt c immobilized on dithiobis(succinimidyl)propionate (DTSP) appears to be the most suitable configuration. In phosphate buffer, the DTSP/Cyt c electrode has a sensitivity of 410 nA microM(-1) cm(-2) and an LOD for SO of 73 nM. Results are also presented for the detection of SO in a complex tissue culture media (MEM) with and without serum, and the sensitivity of the DTSP/Cyt c in MEM in the absence of serum increased to 640 nA microM(-1) cm(-2). By measuring SO with a DTSP/Cyt c electrode before and after the addition of a bolus of the superoxide dismutase (SOD) enzyme, the specificity of the SOD enzyme can be combined with the sensitivity of Cyt c system.

摘要

超氧阴离子自由基(SO)是监测细胞应激反应的关键生物标志物。电化学SO生物传感器通常通过将细胞色素c(Cyt c)共价固定在自组装单分子层(SAMs)上来构建;然而,需要对这些系统进行详细比较以及了解配置对SO检测的影响,以实现可靠的应用。在用Cyt c进行SO的电化学检测过程中,可能涉及两条反应途径,即SAM修饰的金电极对SO的氧化或通过蛋白质和单分子层中继的电子转移,这取决于所使用的SAM。尽管仅具有SAM的电极对SO可表现出高灵敏度和低检测限(LOD),但它们可能会对过氧化氢和抗坏血酸等干扰物的存在产生强烈响应。固定有Cyt c的电极灵敏度降低,但在复杂介质中表现出更好的选择性和抗污染能力。考虑到SO检测在灵敏度、选择性和LOD之间的权衡,用固定在二硫代双(琥珀酰亚胺基)丙酸酯(DTSP)上的Cyt c制成的生物电极似乎是最合适的配置。在磷酸盐缓冲液中,DTSP/Cyt c电极对SO的灵敏度为410 nA μM⁻¹ cm⁻²,检测限为73 nM。还给出了在有血清和无血清的复杂组织培养基(MEM)中检测SO的结果,在无血清的MEM中,DTSP/Cyt c对SO的灵敏度提高到了640 nA μM⁻¹ cm⁻²。通过在添加超氧化物歧化酶(SOD)酶前后用DTSP/Cyt c电极测量SO,可以将SOD酶的特异性与Cyt c系统的灵敏度结合起来。

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