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首页> 外文期刊>Journal of Molecular Biology >USE OF ORGANIC COSMOTROPIC SOLUTES TO CRYSTALLIZE FLEXIBLE PROTEINS - APPLICATION TO T7 RNA POLYMERASE AND ITS COMPLEX WITH THE INHIBITOR T7 LYSOZYME
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USE OF ORGANIC COSMOTROPIC SOLUTES TO CRYSTALLIZE FLEXIBLE PROTEINS - APPLICATION TO T7 RNA POLYMERASE AND ITS COMPLEX WITH THE INHIBITOR T7 LYSOZYME

机译:使用有机共溶溶液结晶柔性蛋白质-在T7 RNA聚合酶及其与抑制剂T7溶菌酶的复合物中的应用

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We have crystallized, using several approaches that may be of general interest, T7 RNA polymerase (T7RP) and the T7 RNA polymerase-T7 lysozyme complex (T7RPL) in forms suitable for structure determination by X-ray crystallography. A series of polyhydric alcohols, sugars, amino and methylamino acids, compounds known to stabilize protein structure, were found to be critical for both crystallization and subsequent improvement of the crystal's diffraction resolution. Moreover, optimal crystallogenesis was achieved through an unconventional ''reverse'' vapor diffusion sitting drop method that is suitable for proteins that are insoluble at low ionic strength. T7RP has been crystallized in an orthorhombic form (I), space group P222, with cell parameters a = 220 Angstrom, b = 205 Angstrom, c = 67 Angstrom and a monoclinic form (II), space group P2(1), with cell parameters a = 229 Angstrom, b = 205 Angstrom, c = 70 Angstrom, beta = 106 degrees. Crystal form I diffracts X-rays to 3.5 Angstrom and form II to 6.0 Angstrom. Three and six copies of the polymerase are predicted to be in the asymmetric unit forms I and II, respectively. Three monoclinic crystal forms of the T7RPL complex have been obtained in space group C2. Form I has cell parameters a = 320 Angstrom, b = 93 Angstrom, c = 229 Angstrom, beta = 129 degrees, form II has parameters a = 293 Angstrom, b = 93 Angstrom, c = 68 Angstrom, beta = 93 degrees, and form III has parameters a = 270 Angstrom, b = 93 Angstrom, c = 63 Angstrom; beta = 103 degrees. Crystal form I diffracts synchrotron wiggler radiation to 3.2 Angstrom and form III to 2.8 Angstrom. Calculations of crystal density imply three or four copies of the complex in form I and one copy in the asymmetric unit of forms II and III. (C) 1997 Academic Press Limited. [References: 69]
机译:我们已经使用几种可能普遍感兴趣的方法结晶了T7 RNA聚合酶(T7RP)和T7 RNA聚合酶-T7溶菌酶复合物(T7RPL),其形式适合通过X射线晶体学确定结构。发现一系列已知能稳定蛋白质结构的多元醇,糖,氨基和甲基氨基酸对结晶和随后提高晶体的衍射分辨率都至关重要。此外,通过非常规的“反向”蒸气扩散坐滴法实现了最佳的结晶生成,该方法适用于在低离子强度下不溶的蛋白质。 T7RP已结晶为正交晶型(I),空间群P222,单元参数a = 220埃,b = 205埃,c = 67埃,单斜晶型(II),空间群P2(1),带有单元参数a = 229埃,b = 205埃,c = 70埃,β= 106度。晶型I将X射线衍射到3.5埃,晶型II衍射到6.0埃。预测聚合酶的三个和六个拷贝分别处于不对称单元形式I和II。在空间群C2中已获得T7RPL配合物的三种单斜晶形式。形式I的晶胞参数a = 320埃,b = 93埃,c = 229埃,β= 129度,形式II的参数a = 293埃,b = 93埃,c = 68埃,β= 93度,以及形式III具有参数a = 270埃,b = 93埃,c = 63埃; Beta = 103度。晶型I将同步加速器摆动辐射衍射到3.2埃,晶型III衍射到2.8埃。晶体密度的计算意味着形式I的配合物有3或4个拷贝,形式II和III的不对称单位有1个拷贝。 (C)1997 Academic Press Limited。 [参考:69]

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