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Capturing Complex Protein Gradients on Biomimetic Hydrogels for Cell-Based Assays

机译:在仿生水凝胶上捕获复杂的蛋白质梯度,用于基于细胞的分析

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摘要

A versatile strategy to rapidly immobilize complex gradients of virtually any desired protein on soft poly(ethylene glycol) (PEG) hydrogel surfaces that are reminiscent of natural extracellular matrices (ECM) is reported. A microfluidic chip is used to generate steady-state gradients of biotinyiated or Fc-tagged fusion proteins that are captured and bound to the surface in less than 5 min by NeutrAvidin or ProteinA, displayed on the surface. The selectivity and orthogonality of the binding schemes enables the formation of parallel and orthogonal overlapping gradients of multiple proteins, which is not possible on conventional cell culture substrates. After patterning, the hydrogels are released from the microfluidic chip and used for cell culture. This novel platform is validated by conducting single-cell migration experiments using time-lapse microscopy. The orientation of cell migration, as well as the migration rate of primary human fibroblasts, depends on the concentration of an immobilized fibronectin fragment. This technique can be readily applied to other proteins to address a wealth of biological questions with different cell types.
机译:据报道,有一种通用的策略可以将几乎任何所需蛋白质的复杂梯度快速固定在柔软的聚乙二醇(PEG)水凝胶表面上,这使人联想到天然细胞外基质(ECM)。微流控芯片用于生成生物素化或Fc标记的融合蛋白的稳态梯度,该融合蛋白在不到5分钟的时间内被NeutrAvidin或ProteinA捕获并结合到表面,并显示在表面上。结合方案的选择性和正交性使得能够形成多种蛋白质的平行和正交重叠梯度,这在常规细胞培养底物上是不可能的。图案化后,水凝胶从微流控芯片中释放出来并用于细胞培养。通过使用延时显微镜进行单细胞迁移实验验证了该新型平台的有效性。细胞迁移的方向以及人类原代成纤维细胞的迁移速率取决于固定的纤连蛋白片段的浓度。这项技术可以很容易地应用于其他蛋白质,以解决具有不同细胞类型的大量生物学问题。

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  • 来源
    《Advanced Functional Materials 》 |2009年第21期| 3411-3419| 共9页
  • 作者单位

    Laboratory of Stem Cell Bioengineering and Institute of Bioengineering Ecole Polytechnique Federale de Lausanne (EPFL) 1015 Lausanne (Switzerland);

    Laboratory of Stem Cell Bioengineering and Institute of Bioengineering Ecole Polytechnique Federale de Lausanne (EPFL) 1015 Lausanne (Switzerland);

    Laboratory of Stem Cell Bioengineering and Institute of Bioengineering Ecole Polytechnique Federale de Lausanne (EPFL) 1015 Lausanne (Switzerland);

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