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Serendipitous crystallization of E. coli HPII catalase, a sequel to "the tale usually not told".大肠杆菌 HPII 过氧化氢酶的偶然结晶,是“通常不被讲述的故事”的续篇。
Acta Biochim Pol. 2021 Jan 24;68(1):29-31. doi: 10.18388/abp.2020_5501.
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Detecting the nature and solving the crystal structure of a contaminant protein from an opportunistic pathogen.检测机会性病原体中污染物蛋白质的性质并解析其晶体结构。
Acta Crystallogr F Struct Biol Commun. 2020 Sep 1;76(Pt 9):392-397. doi: 10.1107/S2053230X20010626. Epub 2020 Aug 28.
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Using Phaser and ensembles to improve the performance of SIMBAD.使用 Phaser 和 ensembles 来提高 SIMBAD 的性能。
Acta Crystallogr D Struct Biol. 2020 Jan 1;76(Pt 1):1-8. doi: 10.1107/S2059798319015031.
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Making routine native SAD a reality: lessons from beamline X06DA at the Swiss Light Source.实现常规的原生 SAD:来自瑞士光源 X06DA 光束线的经验。
Acta Crystallogr D Struct Biol. 2019 Mar 1;75(Pt 3):262-271. doi: 10.1107/S2059798319003103. Epub 2019 Mar 12.
5
A conformational switch from a closed apo- to an open holo-form equips the acyl carrier protein for acyl chain accommodation.构象开关从封闭的无辅基态到开放的全辅基态,使酰基载体蛋白能够容纳酰基链。
Biochim Biophys Acta Proteins Proteom. 2019 Mar;1867(3):163-174. doi: 10.1016/j.bbapap.2018.12.001. Epub 2018 Dec 10.
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Serendipitous crystallization and structure determination of bacterioferritin from Achromobacter.无色杆菌细菌铁蛋白的偶然结晶及结构测定
Acta Crystallogr F Struct Biol Commun. 2018 Sep 1;74(Pt 9):558-566. doi: 10.1107/S2053230X18009809. Epub 2018 Aug 29.
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SIMBAD: a sequence-independent molecular-replacement pipeline.SIMBAD:一种序列无关的分子置换流水线。
Acta Crystallogr D Struct Biol. 2018 Jul 1;74(Pt 7):595-605. doi: 10.1107/S2059798318005752. Epub 2018 Jun 8.
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Cryo-EM in drug discovery: achievements, limitations and prospects.低温电镜在药物研发中的应用:成就、局限与展望。
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9
Distributed computing for macromolecular crystallography.用于大分子晶体学的分布式计算。
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X-rays in the Cryo-Electron Microscopy Era: Structural Biology's Dynamic Future.冷冻电子显微镜时代的X射线:结构生物学充满活力的未来
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偶然结晶的耻垢分枝杆菌酰基载体蛋白合成酶(AcpS)的鉴定、结构测定和分析。

Identification, structure determination and analysis of Mycobacterium smegmatis acyl-carrier protein synthase (AcpS) crystallized serendipitously.

机构信息

Structural and Functional Biology Laboratory, National Institute of Immunology, Aruna Asaf Ali Marg, New Delhi 110 067, India.

出版信息

Acta Crystallogr F Struct Biol Commun. 2022 Jul 1;78(Pt 7):252-264. doi: 10.1107/S2053230X22005738. Epub 2022 Jun 15.

DOI:10.1107/S2053230X22005738
PMID:35787552
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9254898/
Abstract

The unintended crystallization of proteins which generally originate from the expression host instead of the target recombinant proteins is periodically reported. Despite the massive technological advances in the field, assigning a structural model to the corresponding diffraction data is not a trivial task. Here, the structure of acyl-carrier protein synthase (AcpS) from Mycobacterium smegmatis (msAcpS), which crystallized inadvertently in an experimental setup to grow crystals of a Mycobacterium tuberculosis protein using M. smegmatis as an expression system, is reported. After numerous unsuccessful attempts to solve the structure of the target protein by the molecular-replacement method no convincing solutions were obtained, indicating that the diffraction data may correspond to a crystal of an artifactual protein, which was finally identified by the Sequence-Independent Molecular replacement Based on Available Databases (SIMBAD) server. The msAcpS structure was solved at 2.27 Å resolution and structural analysis showed an overall conserved fold. msAcpS formed a trimeric structure similar to those of other reported structures of AcpS from various organisms; however, the residues involved in trimer formation are not strictly conserved. An unrelated metal ion (Ni), which was possibly incorporated during protein purification, was observed in the proximity of His49 and His116. Structural and sequence differences were observed in the loop connecting the α3 and α4 helices that is responsible for the open and closed conformations of the enzyme. Moreover, the structural analysis of msAcpS augments the current understanding of this enzyme, which plays a crucial role in the functional activation of acyl-carrier proteins in the fatty-acid biosynthesis pathway.

摘要

蛋白质的非预期结晶通常源自表达宿主而非目标重组蛋白,这一现象时有报道。尽管该领域取得了巨大的技术进步,但为相应的衍射数据分配结构模型并不是一项简单的任务。在这里,报道了分枝杆菌酰基载体蛋白合酶(AcpS)的结构,该酶来自耻垢分枝杆菌(msAcpS),它在使用耻垢分枝杆菌作为表达系统来生长分枝杆菌蛋白的晶体的实验方案中意外结晶。通过分子置换法多次尝试解决目标蛋白的结构,但未获得令人信服的解决方案,这表明衍射数据可能对应于一种人工蛋白的晶体,最终通过基于现有数据库的序列独立分子置换(SIMBAD)服务器确定了该晶体。msAcpS 的结构在 2.27Å 的分辨率下得到解决,结构分析表明其整体折叠结构保守。msAcpS 形成了类似于其他来自不同生物体的 AcpS 报道结构的三聚体结构;然而,参与三聚体形成的残基并不严格保守。在 His49 和 His116 附近观察到一个可能在蛋白质纯化过程中掺入的无关金属离子(Ni)。在连接α3 和α4 螺旋的环中观察到结构和序列差异,该环负责酶的开/闭构象。此外,msAcpS 的结构分析增加了对该酶的现有认识,该酶在脂肪酸生物合成途径中酰基载体蛋白的功能激活中起着至关重要的作用。