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Expression purification and crystallization of VP4 protease from Tellina virus 1

机译:Tellina病毒1中VP4蛋白酶的表达纯化和结晶

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摘要

Tellina virus 1 is an aquabirnavirus that was isolated from the sand-dwelling marine bivalve mollusc Tellina tenuis. The self-encoded protease viral protein 4 (VP4) processes its own polyprotein to yield the individual proteins VP2 and VP3 that are required for viral assembly. VP4 protease utilizes a serine–lysine catalytic dyad in its mechanism. A full-length VP4 construct was overexpressed in Escherichia coli and purified to homogeneity using nickel-affinity chromatography. Ion-exchange and size-exclusion chromatographic steps were utilized to isolate a monomeric fraction of the protein. The purified monomeric VP4 was subjected to limited proteolysis to yield crystallizable protein. Crystal growth was performed using the hanging-drop vapour-diffusion method and was carried out at room temperature (∼296 K). Hexagonal crystals grew in the presence of PEG 8000, ammonium sulfate and urea. These crystals diffracted to beyond 2.1 Å resolution and belonged to space group P6422, with unit-cell parameters a = 59.1, b = 59.1, c = 208.1 Å, one molecule in the asymmetric unit and a solvent content of 42%.
机译:Tellina病毒1是一种水生病毒,是从居住在沙地的海洋双壳软体动物Tellina tenuis中分离出的。自我编码的蛋白酶病毒蛋白4(VP4)处理其自身的多蛋白,以产生病毒组装所需的单个蛋白VP2和VP3。 VP4蛋白酶在其机制中利用丝氨酸-赖氨酸催化二聚体。全长VP4构建体在大肠杆菌中过表达,并使用镍亲和层析纯化至同质。离子交换和尺寸排阻色谱步骤用于分离蛋白质的单体级分。对纯化的单体VP4进行有限的蛋白水解以产生可结晶的蛋白质。晶体生长采用悬滴蒸气扩散法进行,并在室温(〜296 K)下进行。六角晶体在PEG 8000,硫酸铵和尿素的存在下生长。这些晶体衍射到超过2.1Å的分辨率,属于空间群P6422,单位晶胞参数a = 59.1,b = 59.1,c = 208.1Å,不对称单元中有一个分子,溶剂含量为42%。

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