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蛋白质从具有对比性水凝胶结构域的微孔中扩散。

Protein diffusion from microwells with contrasting hydrogel domains.

作者信息

Su Elaine J, Jeeawoody Shaheen, Herr Amy E

出版信息

APL Bioeng. 2019 Apr 19;3(2):026101. doi: 10.1063/1.5078650. eCollection 2019 Jun.

DOI:10.1063/1.5078650
PMID:31069338
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6481738/
Abstract

Understanding and controlling molecular transport in hydrogel materials is important for biomedical tools, including engineered tissues and drug delivery, as well as life sciences tools for single-cell analysis. Here, we scrutinize the ability of microwells-micromolded in hydrogel slabs-to compartmentalize lysate from single cells. We consider both (i) microwells that are "open" to a large fluid (i.e., liquid) reservoir and (ii) microwells that are "closed," having been capped with either a slab of high-density polyacrylamide gel or an impermeable glass slide. We use numerical modeling to gain insight into the sensitivity of time-dependent protein concentration distributions on hydrogel partition and protein diffusion coefficients and open and closed microwell configurations. We are primarily concerned with diffusion-driven protein loss from the microwell cavity. Even for closed microwells, confocal fluorescence microscopy reports that a fluid (i.e., liquid) film forms between the hydrogel slabs (median thickness of 1.7 m). Proteins diffuse from the microwells and into the fluid (i.e., liquid) layer, yet concentration distributions are sensitive to the lid layer partition coefficients and the protein diffusion coefficient. The application of a glass lid or a dense hydrogel retains protein in the microwell, increasing the protein solute concentration in the microwell by ∼7-fold for the first 15 s. Using triggered release of Protein G from microparticles, we validate our simulations by characterizing protein diffusion in a microwell capped with a high-density polyacrylamide gel lid (p > 0.05, Kolmogorov-Smirnov test). Here, we establish and validate a numerical model useful for understanding protein transport in and losses from a hydrogel microwell across a range of boundary conditions.

摘要

理解和控制水凝胶材料中的分子传输对于生物医学工具(包括工程组织和药物递送)以及单细胞分析的生命科学工具而言至关重要。在此,我们仔细研究了水凝胶平板中微模塑微阱对单细胞裂解液进行分隔的能力。我们考虑了两种情况:(i)对大型流体(即液体)储库“开放”的微阱,以及(ii)已用高密度聚丙烯酰胺凝胶平板或不透水玻璃载玻片覆盖的“封闭”微阱。我们使用数值模型来深入了解随时间变化的蛋白质浓度分布对水凝胶分配、蛋白质扩散系数以及开放和封闭微阱配置的敏感性。我们主要关注微阱腔内由扩散驱动的蛋白质损失。即使对于封闭的微阱,共聚焦荧光显微镜报告显示在水凝胶平板之间形成了一层流体(即液体)膜(中位厚度为1.7μm)。蛋白质从微阱扩散到流体(即液体)层中,但浓度分布对盖层分配系数和蛋白质扩散系数敏感。使用玻璃盖或致密水凝胶可将蛋白质保留在微阱中,在最初的15秒内,微阱中的蛋白质溶质浓度增加约7倍。通过从微粒触发释放蛋白G,我们通过表征在高密度聚丙烯酰胺凝胶盖封闭的微阱中的蛋白质扩散来验证我们的模拟(p>0.05,柯尔莫哥洛夫-斯米尔诺夫检验)。在此,我们建立并验证了一个数值模型,该模型有助于理解在一系列边界条件下水凝胶微阱中蛋白质的传输和损失情况。

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本文引用的文献

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A rapid method for determining protein diffusion through hydrogels for regenerative medicine applications.一种用于再生医学应用中测定蛋白质通过水凝胶扩散的快速方法。
APL Bioeng. 2018 Jun 12;2(2):026110. doi: 10.1063/1.4999925. eCollection 2018 Jun.
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Microparticle Delivery of Protein Markers for Single-Cell Western Blotting from Microwells.微液滴包载蛋白标志物用于微井中的单细胞免疫印迹分析
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Electrophoretic cytometry of adherent cells.贴壁细胞电泳细胞术。
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Photoactivatable fluorescent probes reveal heterogeneous nanoparticle permeation through biological gels at multiple scales.光活化荧光探针揭示了纳米颗粒在多个尺度上通过生物凝胶的异质性渗透。
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