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用于肽预浓缩的玻璃微芯片中显微镜辅助紫外光引发制备明确的多孔聚合物整体栓塞

Microscope-assisted UV-initiated preparation of well-defined porous polymer monolithic plugs in glass microchips for peptide preconcentration.

作者信息

Dziomba Szymon, Araya-Farias Monica, Taverna Myriam, Guerrouache Mohamed, Carbonnier Benjamin, Tran N Thuy

机构信息

Univ. Paris-Est, ICMPE (UMR7182), CNRS, UPEC, 2 Rue Henri Dunant, 94320, Thiais, France.

Institut Galien Paris Sud, UMR8612, Protein and Nanotechnology in Analytical Science (PNAS), CNRS, Univ. Paris-Sud, Univ. Paris-Saclay, 5 rue Jean Baptiste Clément, 92290, Châtenay-Malabry, France.

出版信息

Anal Bioanal Chem. 2017 Mar;409(8):2155-2162. doi: 10.1007/s00216-016-0161-1. Epub 2016 Dec 27.

DOI:10.1007/s00216-016-0161-1
PMID:28028588
Abstract

Herein, highly defined monolithic beds were prepared in glass microchips by photopolymerization of ethylene glycol methacrylate phosphate (EGMP), acrylamide, and N,N'-methylenebisacrylamide (BAA) using an epifluorescence microscope as UV-irradiation source. Such a fast and easy method allowed precise control of (i) the edge shape, (ii) the location along the microchannel, and (iii) the length of the monolithic plugs within glass microchips. The addition of hydroquinone, a polymerization inhibitor, to the prepolymerization mixture was beneficial for achieving local and robust incorporation of monoliths with sharp edges within microchannels. The monolith length was easily tuned from 160 to 400 μm through simple change in the magnification of the objective and was found to be repeatable (relative standard deviation <7.5%). Further application for on-chip monolith-assisted solid - phase extraction is demonstrated for fluorescently labeled peptide. Both binding and subsequent elution behaviors were found to fully agree with a cation-exchange mechanism in concordance with the presence of phosphate groups at the monolith surface. Graphical abstract In-chip microscope-UV-synthesis of monolithic plugs with sharp edges.

摘要

在此,通过使用落射荧光显微镜作为紫外线辐射源,使甲基丙烯酸磷酸乙二醇酯(EGMP)、丙烯酰胺和N,N'-亚甲基双丙烯酰胺(BAA)进行光聚合反应,在玻璃微芯片中制备了高度规整的整体柱床。这种快速简便的方法能够精确控制:(i)边缘形状;(ii)沿微通道的位置;(iii)玻璃微芯片内整体柱塞的长度。向预聚合混合物中添加聚合抑制剂对苯二酚,有利于在微通道内实现具有尖锐边缘的整体柱的局部且稳固的形成。通过简单改变物镜的放大倍数,整体柱长度可轻松从160μm调整至400μm,且发现具有可重复性(相对标准偏差<7.5%)。荧光标记肽的芯片上整体柱辅助固相萃取的进一步应用得到了证明。发现结合和随后的洗脱行为与阳离子交换机制完全一致,这与整体柱表面存在磷酸基团相符。图形摘要:芯片内显微镜紫外合成具有尖锐边缘的整体柱塞。

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