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来自人纤维蛋白原-420的重组αEC结构域的晶体结构。

Crystal structure of a recombinant alphaEC domain from human fibrinogen-420.

作者信息

Spraggon G, Applegate D, Everse S J, Zhang J Z, Veerapandian L, Redman C, Doolittle R F, Grieninger G

机构信息

Center for Molecular Genetics, University of California, San Diego, 9500 Gilman Drive, La Jolla, CA 92093-0634, USA.

出版信息

Proc Natl Acad Sci U S A. 1998 Aug 4;95(16):9099-104. doi: 10.1073/pnas.95.16.9099.

Abstract

The crystal structure of a recombinant alphaEC domain from human fibrinogen-420 has been determined at a resolution of 2.1 A. The protein, which corresponds to the carboxyl domain of the alphaE chain, was expressed in and purified from Pichia pastoris cells. Felicitously, during crystallization an amino-terminal segment was removed, apparently by a contaminating protease, allowing the 201-residue remaining parent body to crystallize. An x-ray structure was determined by molecular replacement. The electron density was clearly defined, partly as a result of averaging made possible by there being eight molecules in the asymmetric unit related by noncrystallographic symmetry (P1 space group). Virtually all of an asparagine-linked sugar cluster is present. Comparison with structures of the beta- and gamma-chain carboxyl domains of human fibrinogen revealed that the binding cleft is essentially neutral and should not bind Gly-Pro-Arg or Gly-His-Arg peptides of the sort bound by those other domains. Nonetheless, the cleft is clearly evident, and the possibility of binding a carbohydrate ligand like sialic acid has been considered.

摘要

已确定来自人纤维蛋白原 - 420的重组αEC结构域的晶体结构,分辨率为2.1埃。该蛋白对应于αE链的羧基结构域,在毕赤酵母细胞中表达并纯化。幸运的是,在结晶过程中,一个氨基末端片段显然被一种污染性蛋白酶切除,使得剩余的201个残基的母体能够结晶。通过分子置换确定了X射线结构。电子密度清晰可辨,部分原因是由于非晶体学对称性(P1空间群)相关的不对称单元中有八个分子,通过平均得以实现。几乎所有的天冬酰胺连接的糖簇都存在。与人纤维蛋白原β链和γ链羧基结构域的结构比较表明,结合裂隙基本呈中性,不应结合其他结构域所结合的那种Gly - Pro - Arg或Gly - His - Arg肽。尽管如此,裂隙明显可见,并且已经考虑了结合像唾液酸这样的碳水化合物配体的可能性。

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