Optimal 1TEL-target protein linker character is target protein-dependent.

IF 3.8 4区生物学 Q2 BIOCHEMICAL RESEARCH METHODS

Acta Crystallographica. Section D, Structural Biology Pub Date : 2026-05-01 Epub Date: 2026-04-07 DOI:10.1107/S2059798326002494

Maria J Pedroza Romo, Alihikaua Keliiliki, Jacob C Averett, Joseph F Gonzalez, Ethan Noakes, Elijah W Wilson, Conrad Smith, Blake Averett, Dalton Hansen, Riley Nickles, Miles Bradford, Sara Soleimani, Tobin Smith, Supeshala Nawarathnage, Prasadika Samarwickrama, Ariel Kelsch, Derick Bunn, Cameron Stewart, Wisdom Abiodun, Evan Tsubaki, Seth Brown, Tzanko I Doukov, James D Moody

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引用次数: 0

Abstract

Fusing a variant of the sterile alpha motif domain of the human translocation ETS leukaemia protein (1TEL) to a protein of interest has been shown to significantly enhance its crystallization propensity. 1TEL is a pH-dependent, polymer-forming protein crystallization chaperone which, when covalently fused to a protein of interest, forms a stable, well ordered crystal lattice. However, despite its success, a challenge persists in that crystal quality and diffraction limits appear to be heavily dependent on the choice of linker between 1TEL and the protein of interest, with the identification of a functional linker currently relying on trial-and-error methods. Likewise, previous studies revealed that a ten-histidine tag at the 1TEL N-terminus can either facilitate or hinder the ordered crystallization of target proteins attached via flexible or semi-flexible linkers. To address these challenges, we designed multiple constructs with several types of linkers [rigid (helical fusion), semi-flexible (Pro-Ala and Pro-Ala-Ala) and flexible (Gly-Gly and Gly-Gly-Gly)] of varying lengths to fuse either a designed ankyrin-repeat protein (DARPin) or the thirty-eight-negative kinase-1 ubiquitin-associated (UBA) domain to the 1TEL C-terminus. Semi-flexible and flexible linker constructs were made with and without a ten-histidine tag. Our findings indicate that short semi-flexible and rigid linkers consistently yielded large crystals with a DARPin target protein, but that flexible linkers performed best with a UBA-domain target protein. Removing the ten-histidine tag uniformly enhanced crystallization rates, improved the crystal morphology and increased the crystallization propensity of the semi-flexible and flexible linker constructs. These results suggest that the ideal linker selection primarily depends on the properties of the target protein. Our data support our current recommendation to use a short flexible or semi-flexible linker between 1TEL and the target protein to facilitate protein crystallization and high-resolution structure determination.

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最佳1tel靶蛋白连接体特性依赖于靶蛋白。

将人类易位ETS白血病蛋白（1TEL）的无菌α基序结构域的一种变体与感兴趣的蛋白质融合，已被证明可显著增强其结晶倾向。tel是一种依赖于ph值的聚合物形成的蛋白质结晶伴侣，当它与感兴趣的蛋白质共价融合时，形成一个稳定的、有序的晶格。然而，尽管它取得了成功，但仍然存在一个挑战，即晶体质量和衍射极限似乎严重依赖于1TEL和感兴趣的蛋白质之间的连接体的选择，而功能性连接体的鉴定目前依赖于试错方法。同样，先前的研究表明，1TEL n端的10 -组氨酸标签可以促进或阻碍通过柔性或半柔性连接体连接的靶蛋白的有序结晶。为了解决这些挑战，我们设计了多种结构体，包括几种不同长度的连接体[刚性（螺旋融合），半柔性（Pro-Ala和Pro-Ala- ala）和柔性（Gly-Gly和Gly-Gly- gly）]，以将设计的锚蛋白重复蛋白（DARPin）或38 -负激酶-1泛素相关（UBA）结构域融合到1TEL c端。半柔性和柔性连接体构建有和不带10 -组氨酸标签。我们的研究结果表明，短的半柔性和刚性连接体一致地产生具有DARPin靶蛋白的大晶体，但柔性连接体在uba结构域靶蛋白上表现最好。去除10 -组氨酸标签均匀地提高了结晶速率，改善了晶体形态，增加了半柔性和柔性连接体结构的结晶倾向。这些结果表明，理想的连接体选择主要取决于目标蛋白的性质。我们的数据支持我们目前的建议，即在1TEL和靶蛋白之间使用短柔性或半柔性连接体，以促进蛋白质结晶和高分辨率结构测定。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Acta Crystallographica. Section D, Structural Biology BIOCHEMICAL RESEARCH METHODSBIOCHEMISTRY &-BIOCHEMISTRY & MOLECULAR BIOLOGY

CiteScore

4.50

自引率

13.60%

发文量

216

期刊介绍： Acta Crystallographica Section D welcomes the submission of articles covering any aspect of structural biology, with a particular emphasis on the structures of biological macromolecules or the methods used to determine them. Reports on new structures of biological importance may address the smallest macromolecules to the largest complex molecular machines. These structures may have been determined using any structural biology technique including crystallography, NMR, cryoEM and/or other techniques. The key criterion is that such articles must present significant new insights into biological, chemical or medical sciences. The inclusion of complementary data that support the conclusions drawn from the structural studies (such as binding studies, mass spectrometry, enzyme assays, or analysis of mutants or other modified forms of biological macromolecule) is encouraged. Methods articles may include new approaches to any aspect of biological structure determination or structure analysis but will only be accepted where they focus on new methods that are demonstrated to be of general applicability and importance to structural biology. Articles describing particularly difficult problems in structural biology are also welcomed, if the analysis would provide useful insights to others facing similar problems.