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喷墨打印酶抑制分析基于喷射体积的测定。

Inkjet-Printing Enzyme Inhibitory Assay Based on Determination of Ejection Volume.

机构信息

College of Pharmacy, Seoul National University , Seoul 151-742, South Korea.

出版信息

Anal Chem. 2017 Feb 7;89(3):2009-2016. doi: 10.1021/acs.analchem.6b04585. Epub 2017 Jan 11.

DOI:10.1021/acs.analchem.6b04585
PMID:28029031
Abstract

An accurate, rapid, and cost-effective methodology for enzyme inhibitor assays is highly needed for large-scale screening to evaluate the efficacy of drugs at the molecular level. For the first time, we have developed an inkjet printing-based enzyme inhibition assay for the assessment of drug activity using a conventional inkjet printer composed of four cartridges. The methodology is based on the determination of the number of moles of the drug on the printed surface. The number of moles was quantified through the volume of substance ejected onto the printed surface. The volume ejected on the reaction spot was determined from the density of reagent ink solution and its weight loss after printing. A xanthine oxidase (XOD) inhibition assay was executed to quantitatively evaluate antioxidant activities of the drug based on the determination of the number of moles of the drug ejected by inkjet printing. The assay components of xanthine, nitro blue tetrazolium (NBT), superoxide dismutase (SOD)/drug, and XOD were printed systematically on A4 paper. A gradient range of the number of moles of SOD/drug printed on A4 paper could be successfully obtained. Because of the effect of enzyme activity inhibition, incrementally reduced NBT formazan colors appeared on the paper in a number-of-moles-dependent manner. The observed inhibitory mole (IM) values of tested compounds exhibited a similar tendency in their activity order, compared to the IC values observed through absorption assay in well plates. Inkjet printing-based IM50 assessment consumed a significantly smaller reaction volume (by 2-3 orders of magnitude) and more rapid reaction time, compared to the well-plate-based absorption assay.

摘要

需要一种准确、快速且具有成本效益的酶抑制剂测定方法,以便在大规模筛选中评估药物在分子水平上的疗效。我们首次开发了一种基于喷墨打印的酶抑制测定方法,该方法使用由四个墨盒组成的常规喷墨打印机进行药物活性评估。该方法基于测定打印表面上药物的摩尔数。通过喷射到打印表面上的物质的体积来定量摩尔数。从试剂墨溶液的密度及其打印后的重量损失来确定在反应点上喷出的体积。通过黄嘌呤氧化酶(XOD)抑制测定来定量评估药物的抗氧化活性,该测定基于通过喷墨打印喷射的药物摩尔数的测定。黄嘌呤、硝基蓝四唑(NBT)、超氧化物歧化酶(SOD)/药物和 XOD 的测定组件系统地打印在 A4 纸上。可以成功地在 A4 纸上获得打印的 SOD/药物摩尔数的梯度范围。由于酶活性抑制的影响,NBT 甲臜颜色以摩尔数依赖的方式逐渐出现在纸上。与在平底孔板中观察到的吸收测定的 IC 值相比,测试化合物的观察到的抑制摩尔(IM)值在其活性顺序中表现出相似的趋势。与基于平底孔板的吸收测定相比,基于喷墨打印的 IM50 评估消耗的反应体积(小 2-3 个数量级)更小,反应时间更快。

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Inkjet Bioprinting on Parchment Paper for Hit Identification from Small Molecule Libraries.用于从小分子文库中进行命中物识别的羊皮纸上的喷墨生物打印
ACS Omega. 2019 Dec 27;5(1):588-596. doi: 10.1021/acsomega.9b03169. eCollection 2020 Jan 14.
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A FRET assay for the quantitation of inhibitors of exonuclease EcoRV by using parchment paper inkjet-printed with graphene oxide and FAM-labelled DNA.使用石墨烯氧化物和 FAM 标记的 DNA 喷墨打印在羊皮纸上的 FRET 测定法,定量测定外切酶 EcoRV 的抑制剂。
Mikrochim Acta. 2019 Mar 4;186(4):211. doi: 10.1007/s00604-019-3317-9.
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