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硫醇盐化学层对GaAs(100)生物功能化的影响:一种结合原子力显微镜和质谱方法的原创方法。

Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry Methods.

作者信息

Bienaime Alex, Leblois Therese, Gremaud Nicolas, Chaudon Maxime-Jean, Osta Marven El, Pecqueur Delphine, Ducoroy Patrick, Elie-Caille Celine

机构信息

MicroNanoSciences and Systems Department, Franche-Comté Electronique, Mécanique, Thermique et Optique-Sciences et Technologies (FEMTO-ST) Institute, 32 avenue de l'Observatoire, 25044 Besançon Cedex, France.

Clinical and Innovation Proteomic Platform, University of Burgundy, CHU, 21000 Dijon, France.

出版信息

Materials (Basel). 2013 Oct 25;6(11):4946-4966. doi: 10.3390/ma6114946.

Abstract

Widely used in microelectronics and optoelectronics; Gallium Arsenide (GaAs) is a III-V crystal with several interesting properties for microsystem and biosensor applications. Among these; its piezoelectric properties and the ability to directly biofunctionalize the bare surface, offer an opportunity to combine a highly sensitive transducer with a specific bio-interface; which are the two essential parts of a biosensor. To optimize the biorecognition part; it is necessary to control protein coverage and the binding affinity of the protein layer on the GaAs surface. In this paper; we investigate the potential of a specific chemical interface composed of thiolate molecules with different chain lengths; possessing hydroxyl (MUDO; for 11-mercapto-1-undecanol (HS(CH₂)OH)) or carboxyl (MHDA; for mercaptohexadecanoic acid (HS(CH₂)CO₂H)) end groups; to reconstitute a dense and homogeneous albumin (Rat Serum Albumin; RSA) protein layer on the GaAs (100) surface. The protein monolayer formation and the covalent binding existing between RSA proteins and carboxyl end groups were characterized by atomic force microscopy (AFM) analysis. Characterization in terms of topography; protein layer thickness and stability lead us to propose the 10% MHDA/MUDO interface as the optimal chemical layer to efficiently graft proteins. This analysis was coupled with MALDI-TOF mass spectrometry measurements; which proved the presence of a dense and uniform grafted protein layer on the 10% MHDA/MUDO interface. We show in this study that a critical number of carboxylic docking sites (10%) is required to obtain homogeneous and dense protein coverage on GaAs. Such a protein bio-interface is of fundamental importance to ensure a highly specific and sensitive biosensor.

摘要

砷化镓(GaAs)广泛应用于微电子和光电子领域;它是一种III-V族晶体,具有一些对微系统和生物传感器应用而言颇为有趣的特性。其中,其压电特性以及直接对裸露表面进行生物功能化的能力,为将高灵敏度传感器与特定生物界面相结合提供了契机,而这两者正是生物传感器的两个关键部分。为优化生物识别部分,有必要控制蛋白质在GaAs表面的覆盖度以及蛋白质层的结合亲和力。在本文中,我们研究了由具有不同链长、带有羟基(MUDO,即11-巯基-1-十一醇(HS(CH₂)₁₀OH))或羧基(MHDA,即巯基十六烷酸(HS(CH₂)₁₅CO₂H))端基的硫醇盐分子组成的特定化学界面,在GaAs(100)表面重构致密且均匀的白蛋白(大鼠血清白蛋白,RSA)蛋白质层的潜力。通过原子力显微镜(AFM)分析对蛋白质单层的形成以及RSA蛋白质与羧基端基之间存在的共价结合进行了表征。从形貌、蛋白质层厚度和稳定性方面进行的表征使我们提出10% MHDA/MUDO界面作为有效接枝蛋白质的最佳化学层。该分析与基质辅助激光解吸电离飞行时间质谱(MALDI-TOF)测量相结合,证明了在10% MHDA/MUDO界面上存在致密且均匀的接枝蛋白质层。我们在本研究中表明,需要一定数量的关键羧基对接位点(10%)才能在GaAs上获得均匀且致密的蛋白质覆盖。这样的蛋白质生物界面对于确保高特异性和高灵敏度的生物传感器至关重要。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/ac75/5452766/efeed5566d1c/materials-06-04946-g001.jpg

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