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New Surface-Enhanced Raman Sensing Chip Designed for On-Site Detection of Active Ricin in Complex Matrices Based on Specific Depurination

机译:新型表面增强拉曼传感芯片设计用于基于特定脱嘌呤的现场检测复杂基质中的活性蓖麻毒素

摘要

Quick and accurate on-site detection of active ricin has very important realistic significance in view of national security and defense. In this paper, optimized single-stranded oligodeoxynucleotides named poly(21dA), which function as a depurination substrate of active ricin, were screened and chemically attached on gold nanoparticles (AuNPs, similar to 100 nrn) via the Au-S bond [poly(21dA)-AuNPs]. Subsequently, poly(21dA) AuNPs were assembled on a dihydrogen lipoic-acid-modified Si wafer (SH-Si), thus forming the specific surface-enhanced Raman spectroscopy (SERS) chip [poly(21dA)-AuNPs@SH-Si] for depurination of active ricin. Under optimized conditions, active ricin could specifically hydrolyze multiple adenines from poly(21dA) on the chip. This depurination-induced composition change could be conveniently monitored by measuring the distinct attenuation of the SERS signature corresponding to adenine. To improve sensitivity of this method, a silver nanoshell was deposited on post-reacted poly(21dA)-AuNPs, which lowered the limit of detection to 8.9 ng mL(-1). The utility of this well controlled SERS chip was successfully demonstrated in food and biological matrices spiked with different concentrations of active ricin, thus showing to be very promising assay for reliable and rapid on-site detection of active ricin.
机译:鉴于国家安全和国防,快速,准确地现场检测活性蓖麻毒蛋白具有非常重要的现实意义。在本文中,筛选了名为poly(21dA)的优化的单链寡聚脱氧核苷酸,该多肽具有活性蓖麻毒蛋白的净化作用,并通过Au-S键[poly( 21dA)-AuNPs]。随后,将聚(21dA)AuNPs组装在二氢硫辛酸改性的硅晶片(SH-Si)上,从而形成比表面增强拉曼光谱(SERS)芯片[poly(21dA)-AuNPs @ SH-Si]用于活性蓖麻蛋白的纯化。在优化的条件下,活性蓖麻毒蛋白可以从芯片上的poly(21dA)特异性水解多种腺嘌呤。通过测量对应于腺嘌呤的SERS信号的明显衰减,可以方便地监测这种由脱嘌呤引起的成分变化。为了提高此方法的灵敏度,在反应后的聚(21dA)-AuNPs上沉积了银纳米壳,将检测限降低到8.9 ng mL(-1)。在食物和生物基质中掺入不同浓度的活性蓖麻毒蛋白,已成功证明了这种受良好控制的SERS芯片的实用性,因此对于可靠,快速的现场检测活性蓖麻毒蛋白而言,显示出非常有前途的检测方法。

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