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Trapping of Bead-Based Reagents within Microfluidic Systems: On-Chip Solid-Phase Extraction and Electrochromatography

机译:在微流体系统中捕集基于珠子的试剂:片上固相萃取和电色谱

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A 330-pL chromatographic bed was fabricated on a glass substrate as part of an electroosmotically pumped microfluidic system. Two weirs within a sample channel formed a cavity in which octadecylsilane (ODS) coated silica beads (1.5-4 μm diameter) were trapped. ODS beads were mobilized into and out of the cavity using electroosmotic flow through a bead-introduction channel which accessed the cavity. This procedure allowed the beads in the cavity to be repeatedly exchanged. A 1 nM solution of a nonpolar analyte (BODIPY 493/503) in buffer was loaded onto the beads for different lengths of time using an electroosmotic flow of 1.2 nL/s. The material retained on the ODS phase was then eluted by electroosmotic flow of acetonitrile with a concentration enhancement of up to 500 times. Capillary electro-chromatography was conducted using a similar device. BODIPY and fluorescein were loaded onto a 200-μm-long chromatographic bed and then separated in an isocratic CEC run with an acetonitrile/buffer mobile phase. Complete separation was achieved in less than 20 s with a 2-μm plate height.
机译:作为电泵微流体系统的一部分,在玻璃基板上制备了330 pL色谱床。样品通道中的两个堰形成一个空腔,在该空腔中捕获了十八烷基硅烷(ODS)涂层的二氧化硅珠(直径1.5-4μm)。使用电渗流通过进入空腔的珠子引入通道,将ODS珠子动员进出空腔。该过程允许腔中的珠子被重复交换。使用1.2 nL / s的电渗流将1nM非极性分析物(BODIPY 493/503)在缓冲液中的溶液加载到珠子上不同的时间长度。然后通过乙腈的电渗流将保留在ODS相上的物质洗脱,其浓度最多提高500倍。毛细管电色谱法使用类似的装置进行。将BODIPY和荧光素上样至200μm长的色谱床上,然后在乙腈/缓冲液流动相的等度CEC中分离。在不到20 s的时间内,板高为2μm即可实现完全分离。

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