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用于一步法无试剂固定DNA和蛋白质的微板的等离子体活化优化

Plasma Activation of Microplates Optimized for One-Step Reagent-Free Immobilization of DNA and Protein.

作者信息

Coffi Dit Gleize Kanako, Tran Clara T H, Waterhouse Anna, Bilek Marcela M M, Wickham Shelley F J

机构信息

School of Chemistry, The University of Sydney, Sydney, NSW 2006, Australia.

School of Physics, The University of Sydney, Sydney, NSW 2006, Australia.

出版信息

Langmuir. 2023 Jan 10;39(1):343-356. doi: 10.1021/acs.langmuir.2c02573. Epub 2022 Dec 22.

Abstract

Activated microplates are widely used in biological assays and cell culture to immobilize biomolecules, either through passive physical adsorption or covalent cross-linking. Covalent attachment gives greater stability in complex biological mixtures. However, current multistep chemical activation methods add complexity and cost, require specific functional groups, and can introduce cytotoxic chemicals that affect downstream cellular applications. Here, we show a method for one-step linker-free activation of microplates by energetic ions from plasma for covalent immobilization of DNA and protein. Two types of energetic ion plasma treatment were shown to be effective: plasma immersion ion implantation (PIII) and plasma-activated coating (PAC). This is the first time that PIII and PAC have been reported in microwell plates with nonflat geometry. We confirm that the plasma treatment generates radical-activated surfaces at the bottom of wells despite potential shadowing from the walls. Comprehensive surface characterization studies were used to compare the PIII and PAC microplate surface composition, wettability, radical density, optical properties, stability, and biomolecule immobilization density. PAC plates were found to have more nitrogen and lower radical density and were more hydrophobic and more stable over 3 months than PIII plates. Optimal conditions were obtained for high-density DNA (PAC, 0 or 21% nitrogen, pH 3-4) and streptavidin (PAC, 21% nitrogen, pH 5-7) binding while retaining optical properties required for typical high-throughput biochemical microplate assays, such as low autofluorescence and high transparency. DNA hybridization and protein activity of immobilized molecules were confirmed. We show that PAC activation allows for high-density covalent immobilization of functional DNA and protein in a single step on both 96- and 384-well plates without specific linker chemistry. These microplates could be used in the future to bind other user-selected ligands in a wide range of applications, for example, for solid phase polymerase chain reaction and stem cell culture and differentiation.

摘要

活化微孔板广泛应用于生物分析和细胞培养中,通过被动物理吸附或共价交联来固定生物分子。共价连接在复杂的生物混合物中具有更高的稳定性。然而,目前的多步化学活化方法增加了复杂性和成本,需要特定的官能团,并且可能引入影响下游细胞应用的细胞毒性化学物质。在这里,我们展示了一种通过等离子体中的高能离子对微孔板进行一步无连接子活化的方法,用于DNA和蛋白质的共价固定。两种类型的高能离子等离子体处理被证明是有效的:等离子体浸没离子注入(PIII)和等离子体活化涂层(PAC)。这是首次在具有非平面几何形状的微孔板中报道PIII和PAC。我们证实,尽管孔壁可能存在阴影,但等离子体处理仍能在孔底部产生自由基活化表面。通过全面的表面表征研究来比较PIII和PAC微孔板的表面组成、润湿性、自由基密度、光学性质、稳定性和生物分子固定密度。发现PAC板比PIII板含有更多的氮且自由基密度更低,在3个月内更疏水且更稳定。获得了高密度DNA(PAC,0或21%氮,pH 3 - 4)和链霉亲和素(PAC,21%氮,pH 5 - 7)结合的最佳条件,同时保留了典型高通量生化微孔板分析所需的光学性质,如低自发荧光和高透明度。证实了固定分子的DNA杂交和蛋白质活性。我们表明,PAC活化允许在96孔和384孔板上一步实现功能DNA和蛋白质的高密度共价固定,无需特定的连接子化学。这些微孔板未来可用于在广泛的应用中结合其他用户选择的配体,例如用于固相聚合酶链反应以及干细胞培养和分化。

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