Kuntala Banerjee , K. Rasheeda , Aafiya Tarannum , N. Nishad Fathima
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引用次数: 0
Abstract
Tuning the self-assembly of collagen has broad applications in the biomedical field owing to their desired biological performance as collagenous materials with tunable functionalities can further determine cellular responses. In this work, an attempt has been made to tune the self-assembly of collagen using ionic liquids, viz., imidazolium chloride (IC) and choline dihydrogen phosphate (CDHP) at its physiological pH, followed by probing assembled systems using various characterization methods. Turbidity measurements of fibrillar networks were performed to ascertain the rate of fibril formation in addition of imidazolium chloride and choline dihydrogen phosphate to collagen at physiological pH. Morphological changes were examined using Scanning Electron Microscope (SEM), binding affinities were measured by Microscale Thermophoresis (MST), in addition to, changes in the shear viscosity, mechanical strength of collagen fibrils when interacted with imidazolium and choline based ILs were carried out using rotational rheometer and Quartz Crystal Microbalance (QCM) measurements. Experimental result depicts that CDHP imparts better crosslinking as well as mechanical strength compare to IC, which is already known for destabilizing the triple helix structure is inhibiting the fibril formation. This self-assembled, ionic-liquid treated collagen-fibrillar system would accelerate various force modulated fibrillar network study, for mimicking the ECM and tissue engineering application.
调谐胶原蛋白的自组装在生物医学领域有着广泛的应用,因为具有可调谐功能的胶原蛋白材料可以进一步确定细胞的反应,从而实现理想的生物学性能。在这项工作中,我们尝试使用离子液体,即氯化咪唑(IC)和磷酸胆碱二氢(CDHP),在生理 pH 值下调节胶原蛋白的自组装,然后使用各种表征方法探测组装系统。对纤维网络进行浊度测量,以确定在生理 pH 值下向胶原添加氯化咪唑和磷酸胆碱二氢盐时纤维形成的速度。此外,还使用旋转流变仪和石英晶体微天平(QCM)测量了胶原纤维与咪唑基和胆碱基 IL 相互作用时的剪切粘度和机械强度的变化。实验结果表明,与 IC 相比,CDHP 具有更好的交联性和机械强度,而 IC 则会破坏三螺旋结构的稳定性,从而抑制纤维的形成。这种经离子液体处理的自组装胶原纤维系统将加速各种力调制纤维网络的研究,以模拟 ECM 和组织工程应用。
期刊介绍:
Biophysical Chemistry publishes original work and reviews in the areas of chemistry and physics directly impacting biological phenomena. Quantitative analysis of the properties of biological macromolecules, biologically active molecules, macromolecular assemblies and cell components in terms of kinetics, thermodynamics, spatio-temporal organization, NMR and X-ray structural biology, as well as single-molecule detection represent a major focus of the journal. Theoretical and computational treatments of biomacromolecular systems, macromolecular interactions, regulatory control and systems biology are also of interest to the journal.