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Local and long-range stability in tandemly arrayed tetratricopeptide repeats

机译:串联排列的四三肽重复序列的局部和远距离稳定性

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摘要

The tetratricopeptide repeat (TPR) is a 34-aa α-helical motif that occurs in tandem arrays in a variety of different proteins. In natural proteins, the number of TPR motifs ranges from 3 to 16 or more. These arrays function as molecular scaffolds and frequently mediate protein-protein interactions. We have shown that correctly folded TPR domain proteins, exhibiting the typical helix-turn-helix fold, can be designed by arraying tandem repeats of an idealized TPR consensus motif. To date, three designed proteins, CTPR1, CTPR2, and CTPR3 (consensus TPR number of repeats) have been characterized. Their high-resolution crystal structures show that the designed proteins indeed adopt the typical TPR fold, which is specified by the correct positioning of key residues. Here, we present a study of the thermodynamic properties and folding kinetics of this set of designed proteins. Chemical denaturation, monitored by CD and fluorescence, was used to assess the folding and global stability of each protein. NMR-detected amide proton exchange was used to investigate the stability of each construct at a residue-specific level. The results of these studies reveal a stable core, which defines the intrinsic stability of an individual TPR motif. The results also show the relationship between the number of tandem repeats and the overall stability and folding of the protein.
机译:四肽重复序列(TPR)是一种34-aaα螺旋基序,它以串联阵列的形式出现在多种不同的蛋白质中。在天然蛋白质中,TPR基序的数量为3至16或更多。这些阵列用作分子支架并经常介导蛋白质-蛋白质相互作用。我们已经显示,可以通过排列理想化TPR共有基序的串联重复序列来设计正确折叠的TPR域蛋白,表现出典型的螺旋-转-螺旋折叠。迄今为止,已表征了三种设计的蛋白CTPR1,CTPR2和CTPR3(重复的共识性TPR数)。它们的高分辨率晶体结构表明,设计的蛋白质确实采用了典型的TPR折叠,这是关键残基的正确定位所指定的。在这里,我们介绍了这组设计蛋白的热力学性质和折叠动力学的研究。通过CD和荧光监测化学变性,以评估每种蛋白质的折叠和整体稳定性。 NMR检测到的酰胺质子交换用于研究每个构建体在残基特异性水平下的稳定性。这些研究的结果揭示了一个稳定的核心,该核心定义了单个TPR基序的固有稳定性。结果还显示了串联重复的数目与蛋白质的整体稳定性和折叠之间的关系。

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