Biosensors Based on Porous Cellulose Nanocrystal-Poly(vinyl Alcohol) Scaffolds

被引:110
|
作者
Schyrr, Bastien [1 ,2 ]
Pasche, Stephanie [1 ]
Voirin, Guy [1 ]
Weder, Christoph [2 ]
Simon, Yoan C. [2 ]
Foster, E. Johan [2 ]
机构
[1] CSEM Ctr Suisse Elect & Microtech SA, CH-2002 Neuchatel, Switzerland
[2] Univ Fribourg, Adolphe Merkle Inst, CH-1723 Marly, Switzerland
基金
瑞士国家科学基金会;
关键词
cellulose nanocrystals; biosensing; nanocomposites; photodetection; porous scaffold; MICHAEL ADDITION-REACTIONS; POLYVINYL-ALCOHOL; POLYMER NANOCOMPOSITES; PROTEASE ACTIVITY; DNA MICROARRAYS; NANOCRYSTALS; THIOL; COPOLYMERS; WHISKERS; IMMOBILIZATION;
D O I
10.1021/am502670u
中图分类号
TB3 [工程材料学];
学科分类号
0805 ; 080502 ;
摘要
Cellulose nanocrystals (CNCs), which offer a high aspect ratio, large specific surface area, and large number of reactive surface groups, are well suited for the facile immobilization of high density biological probes. We here report functional high surface area scaffolds based on cellulose nanocrystals (CNCs) and poly(vinyl alcohol) (PVA) and demonstrate that this platform is useful for fluorescence-based sensing schemes. Porous CNC/PVA nanocomposite films with a thickness of 25-70 nm were deposited on glass substrates by dip-coating with an aqueous mixture of the CNCs and PVA, and the porous nanostructure was fixated by heat treatment. In a subsequent step, a portion of the scaffold's hydroxyl surface groups was reacted with 2-(acryloxy)ethyl (3-isocyanato-4-methylphenyl)carbamate to permit the immobilization of thiolated fluorescein-substituted lysine, which was used as a first sensing motif, via nucleophile-based thiol ene Michael addition. The resulting sensor films exhibit a nearly instantaneous and pronounced change of their fluorescence emission intensity in response to changes in pH. The approach was further extended to the detection of protease activity by immobilizing a Forster-type resonance energy transfer chromophore pair via a labile peptide sequence to the scaffold. This sensing scheme is based on the degradation of the protein linker in the presence of appropriate enzymes, which separate the chromophores and causes a turn-on of the originally quenched fluorescence. Using a standard benchtop spectrometer to monitor the increase in fluorescence intensity, trypsin was detected at a concentration of 250 mu g/mL, i.e., in a concentration that is typical for abnormal proteolytic activity in wound fluids.
引用
收藏
页码:12674 / 12683
页数:10
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