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Crystallization and preliminary X-ray diffraction analysis of vaccinia virus H1L phosphatase

机译:痘苗病毒H1L磷酸酶的结晶和初步X射线衍射分析

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摘要

The cysteine-based protein phosphatase H1L was the first reported dual-specificity protein phosphatase. H1L is encapsidated within the vaccinia virus and is required for successful host infection and for the production of viable vaccinia progeny. H1L has therefore been proposed as a target candidate for antiviral compounds. Recombinant H1L has been expressed in a catalytically inactive form using an Escherichia coli host, leading to purification and crystallization by the microbatch method. The crystals diffract to 2.1 Å resolution using synchrotron radiation. These crystals belong to space group P422, with unit-cell parameters a = b = 98.31, c = 169.15 Å, and are likely to contain four molecules in the asymmetric unit. A sulfur SAD data set was collected to 2.8 Å resolution on beamline BM14 at the ESRF to facilitate structure determination. Attempts to derivatize these crystals with xenon gas changed the space group to I422, with unit-cell parameters a = b = 63.28, c = 169.68 Å and a single molecule in the asymmetric unit. The relationship between these two crystal forms is discussed.
机译:基于半胱氨​​酸的蛋白磷酸酶H1L是第一个报道的双特异性蛋白磷酸酶。 H1L衣壳化在牛痘病毒内,是成功感染宿主和产生活的牛痘后代所必需的。因此,已经提出将H1L用作抗病毒化合物的目标候选物。重组H1L已通过大肠杆菌宿主以催化失活的形式表达,从而通过微分批法纯化和结晶。晶体通过同步加速器辐射衍射至2.1Å分辨率。这些晶体属于空间群P422,单位晶胞参数a = b = 98.31,c = 169.15Å,并且可能在不对称单元中包含四个分子。在ESRF上的光束线BM14上以2.8?Å的分辨率收集了硫SAD数据集,以便于确定结构。尝试用氙气将这些晶体衍生化,将空间群更改为I422,其晶胞参数a = b = 63.28,c = 169.68Å,并且非对称单元中存在单个分子。讨论了这两种晶体形式之间的关系。

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