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Evaluation of photochemistry reaction kinetics to pattern bioactive proteins on hydrogels for biological applications

机译:评估光化学反应动力学以在水凝胶上为生物应用图案化生物活性蛋白

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摘要

Bioactive signals play many important roles on cell function and behavior. In most biological studies, soluble biochemical cues such as growth factors or cytokines are added directly into the media to maintain and/or manipulate cell activities in vitro. However, these methods cannot accurately mimic certain in vivo biological signaling motifs, which are often immobilized to extracellular matrix and also display spatial gradients that are critical for tissue morphology. Besides biochemical cues, biophysical properties such as substrate stiffness can influence cell behavior but is not easy to manipulate under conventional cell culturing practices. Recent development in photocrosslinkable hydrogels provides new tools that allow precise control of spatial biochemical and biophysical cues for biological applications, but doing so requires a comprehensive study on various hydrogel photochemistry kinetics to allow thorough photocrosslink reaction while maintain protein bioactivities at the same time. In this paper, we studied several photochemistry reactions and evaluate key photochemical parameters, such as photoinitiators and ultra-violet (UV) exposure times, to understand their unique contributions to undesired protein damage and cell death. Our data illustrates the retention of protein function and minimize of cell health during photoreactions requires careful selection of photoinitiator type and concentration, and UV exposure times. We also developed a robust method based on thiol-norbornene chemistry for independent control of hydrogel stiffness and spatial bioactive patterns. Overall, we highlight a class of bioactive hydrogels to stiffness control and site specific immobilized bioactive proteins/peptides for the study of cellular behavior such as cellular attraction, repulsion and stem cell fate.
机译:生物活性信号在细胞功能和行为中起许多重要作用。在大多数生物学研究中,可溶性生化线索(例如生长因子或细胞因子)被直接添加到培养基中以维持和/或操纵体外细胞活性。但是,这些方法无法准确地模拟某些体内的生物信号基序,这些基序通常固定在细胞外基质上,并且还显示出对于组织形态至关重要的空间梯度。除了生化线索外,诸如底物刚度之类的生物物理特性也会影响细胞行为,但在常规细胞培养实践中不易操作。可光交联水凝胶的最新发展提供了新的工具,可以精确控制用于生物应用的空间生化和生物物理线索,但是这样做需要对各种水凝胶光化学动力学进行全面研究,以允许彻底的光交联反应,同时保持蛋白质的生物活性。在本文中,我们研究了几种光化学反应并评估了关键的光化学参数,例如光引发剂和紫外线(UV)暴露时间,以了解它们对不希望的蛋白质损伤和细胞死亡的独特贡献。我们的数据说明了光反应过程中蛋白质功能的保留和细胞健康的最小化需要仔细选择光引发剂的类型和浓度以及紫外线照射时间。我们还开发了一种基于硫醇-降冰片烯化学的稳健方法,可独立控制水凝胶的硬度和空间生物活性模式。总的来说,我们重点介绍了一类可控制僵硬度的生物活性水凝胶,以及用于研究细胞行为(例如细胞吸引力,排斥力和干细胞命运)的特定位点固定化生物活性蛋白质/肽。

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