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

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

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 opportunit...

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Main Authors: Alex Bienaime, Therese Leblois, Nicolas Gremaud, Maxime-Jean Chaudon, Marven El Osta, Delphine Pecqueur, Patrick Ducoroy, Celine Elie-Caille
Format: Article
Language:English
Published: MDPI AG 2013-10-01
Series:Materials
Subjects:
GaAs
self-assembled thiolate monolayers
proteins grafting
AFM
MALDI-TOF MS
Online Access:http://www.mdpi.com/1996-1944/6/11/4946
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spelling doaj-3748d53c017b4a118ffef88ac18d15ba2020-11-24T22:42:39ZengMDPI AGMaterials1996-19442013-10-016114946496610.3390/ma6114946Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry MethodsAlex BienaimeTherese LebloisNicolas GremaudMaxime-Jean ChaudonMarven El OstaDelphine PecqueurPatrick DucoroyCeline Elie-CailleWidely 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)11OH)) or carboxyl (MHDA; for mercaptohexadecanoic acid (HS(CH2)15CO2H)) 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 in situ 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.http://www.mdpi.com/1996-1944/6/11/4946GaAsself-assembled thiolate monolayersproteins graftingAFMMALDI-TOF MS
collection DOAJ
language English
format Article
sources DOAJ
author Alex Bienaime
Therese Leblois
Nicolas Gremaud
Maxime-Jean Chaudon
Marven El Osta
Delphine Pecqueur
Patrick Ducoroy
Celine Elie-Caille
spellingShingle Alex Bienaime
Therese Leblois
Nicolas Gremaud
Maxime-Jean Chaudon
Marven El Osta
Delphine Pecqueur
Patrick Ducoroy
Celine Elie-Caille
Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry Methods
Materials
GaAs
self-assembled thiolate monolayers
proteins grafting
AFM
MALDI-TOF MS
author_facet Alex Bienaime
Therese Leblois
Nicolas Gremaud
Maxime-Jean Chaudon
Marven El Osta
Delphine Pecqueur
Patrick Ducoroy
Celine Elie-Caille
author_sort Alex Bienaime
title Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry Methods
title_short Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry Methods
title_full Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry Methods
title_fullStr Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry Methods
title_full_unstemmed Influence of a Thiolate Chemical Layer on GaAs (100) Biofunctionalization: An Original Approach Coupling Atomic Force Microscopy and Mass Spectrometry Methods
title_sort influence of a thiolate chemical layer on gaas (100) biofunctionalization: an original approach coupling atomic force microscopy and mass spectrometry methods
publisher MDPI AG
series Materials
issn 1996-1944
publishDate 2013-10-01
description 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)11OH)) or carboxyl (MHDA; for mercaptohexadecanoic acid (HS(CH2)15CO2H)) 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 in situ 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.
topic GaAs
self-assembled thiolate monolayers
proteins grafting
AFM
MALDI-TOF MS
url http://www.mdpi.com/1996-1944/6/11/4946
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