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Protein crystallization by design: Chymotrypsinogen without precipitants

机译:通过设计使蛋白质结晶:没有沉淀的胰凝乳蛋白酶原

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Protein crystals are usually obtained by an empirical approach based on extensive screening to identify suitable crystallization conditions. In contrast, we have used a systematic predictive procedure to produce data-quality crystals of bovine chymotrypsinogen A and used them to obtain a refined X-ray structure to 3 Angstrom resolution. Measurements of the osmotic second virial coefficient of chymotrypsinogen solutions were used to identify suitable solvent conditions, following which crystals were grown for approximately 30 hours by ultracentrifugal crystallization, without the use of any precipitants. Existing structures of chymotrypsinogen were obtained in solutions including 10-30% ethanol, whereas simple buffered NaCl solutions were used here. The protein crystallized in the tetragonal space group P4(1)2(1)2, with one molecule per asymmetric unit. The quality of the refined map was very high throughout, with the main-chain atoms of all but four residues clearly defined and with nearly all side-chains also defined. Although only minor differences are seen compared to the structures previously reported, they indicate the possibility of structural changes due to the crystallization conditions used in those studies. Our results show that more systematic crystallization of proteins is possible, and that the procedure can expand the range of conditions under which crystals can be grown successfully and can make new crystal forms available. (C) 2000 Academic Press. [References: 26]
机译:通常通过基于广泛筛选以鉴定合适的结晶条件的经验方法获得蛋白质晶体。相比之下,我们已使用系统的预测程序来生产牛胰凝乳蛋白酶原A的数据质量的晶体,并使用它们获得了3埃分辨率的精确X射线结构。胰凝乳蛋白酶原溶液的渗透第二病毒系数的测量用于确定合适的溶剂条件,此后通过超离心结晶使晶体生长约30小时,而无需使用任何沉淀剂。在包含10-30%乙醇的溶液中获得了胰凝乳蛋白酶原的现有结构,而此处使用了简单的缓冲NaCl溶液。该蛋白质在四边形空间群P4(1)2(1)2中结晶,每个不对称单元具有一个分子。整个过程中,精制图的质量非常高,除了四个残基外,所有主链原子都清晰定义,几乎所有侧链也都定义了。尽管与以前报道的结构相比只有很小的差异,但它们表明由于这些研究中使用的结晶条件,可能会发生结构变化。我们的结果表明,蛋白质的更系统的结晶是可能的,并且该程序可以扩大晶体可以成功生长的条件范围,并可以提供新的晶体形式。 (C)2000学术出版社。 [参考:26]

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