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Soft nanotube hydrogels functioning as artificial chaperones

机译:软纳米管水凝胶起人工伴侣的作用

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Figure Persented: Self-assembly of rationally designed asymmetric amphiphilic monomers in water produced nanotube hydrogels in the presence of chemically denatured proteins (green fluorescent protein, carbonic anhydrase, and citrate synthase) at room temperature, which were able to encapsulate the proteins in the one-dimensional channel of the nanotube consisting of a monolayer membrane. Decreasing the concentrations of the denaturants induced refolding of part of the encapsulated proteins in the nanotube channel. Changing the pH dramatically reduced electrostatic attraction between the inner surface mainly covered with amino groups of the nanotube channel and the encapsulated proteins. As a result, the refolded proteins were smoothly released into the bulk solution without specific additive agents. This recovery procedure also transformed the encapsulated proteins from an intermediately refolding state to a completely refolded state. Thus, the nanotube hydrogels assisted the refolding of the denatured proteins and acted as artificial chaperones. Introduction of hydrophobic sites such as a benzyloxycarbony group and a tert-butoxycarbonyl group onto the inner surface of the nanotube channels remarkably enhanced the encapsulation and refolding efficiencies based on the hydrophobic interactions between the groups and the surface-exposed hydrophobic amino acid residues of the intermediates in the refolding process. Refolding was strongly dependent on the inner diameters of the nanotube channels. Supramolecular nanotechnology allowed us to not only precisely control the diameters of the nanotube channels but also functionalize their surfaces, enabling us to fine-tune the biocompatibility. Hence, these nanotube hydrogel systems should be widely applicable to various target proteins of different molecular weights, charges, and conformations.
机译:图(图):在室温下存在化学变性蛋白质(绿色荧光蛋白质,碳酸酐酶和柠檬酸合酶)的情况下,合理设计的不对称两亲单体在水产生的纳米管水凝胶中的自组装,能够将蛋白质封装在其中由单层膜组成的纳米管的三维通道。降低变性剂的浓度会导致纳米管通道中部分包封的蛋白质重新折叠。改变pH值显着降低了主要被纳米管通道的氨基所覆盖的内表面与包封的蛋白质之间的静电吸引力。结果,重新折叠的蛋白质在没有特定添加剂的情况下顺利释放到本体溶液中。该恢复过程还将包封的蛋白质从中间重折叠状态转变为完全重折叠状态。因此,纳米管水凝胶有助于变性蛋白质的重折叠并充当人工伴侣。基于基团与中间体表面暴露的疏水性氨基酸残基之间的疏水性相互作用,将疏水性位点(例如苄氧基碳基和叔丁氧基羰基)引入纳米管通道的内表面,显着提高了包封和重折叠效率在重新折叠过程中。重新折叠在很大程度上取决于纳米管通道的内径。超分子纳米技术使我们不仅可以精确控制纳米管通道的直径,还可以使它们的表面功能化,从而使我们能够微调生物相容性。因此,这些纳米管水凝胶系统应广泛应用于分子量,电荷和构象不同的各种靶蛋白。

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