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利用杆状病毒系统表达的突变体测定人β2-糖蛋白I作为抗心磷脂辅因子的作用。

Human beta2-glycoprotein I as an anticardiolipin cofactor determined using mutants expressed by a baculovirus system.

作者信息

Igarashi M, Matsuura E, Igarashi Y, Nagae H, Ichikawa K, Triplett D A, Koike T

机构信息

Microbiology Laboratory, Yamasa Corp, Choshi, Japan.

出版信息

Blood. 1996 Apr 15;87(8):3262-70.

PMID:8605342
Abstract

beta2-Glycoprotein I (beta2-GPI) consists of five repeats of a homologous domain. We designed a series of human beta2-GPI mutant genes, ie, three mutant genes lacking the domain(s) present in the NH2-terminal region and two of those present in the COOH-terminal region. These mutant genes were expressed in Spodoptera frugiperda insect cells (Sf9) infected with recombinant baculoviruses and the mutant proteins were secreted into the culture medium. The molecular mass of the purified mutant proteins, estimated by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, was fairly consistent with the size calculated from their nucleotide sequences. Binding of beta2-GPI to solid-phase cardiolipin (CL) was diminished by the deletion of the fifth domain (domain V) from its complete structure. Thus, the phospholipid binding site of beta2-GPI is located on its domain V. Monoclonal anti-CL antibodies (aCL) derived either from NZW x BXSB (WB) F1 mice or from patients with antiphospholipid syndrome bound directly to the domain V-deleted mutant protein (DI-IV) absorbed not only on an oxygenated but also on a plain polystyrene surface. We conclude from this study that the epitope for aCL is exposed on a conformationally changed structure of beta2-GPI by interacting with negatively charged phospholipid or on the mutant protein, DI-IV.

摘要

β2-糖蛋白I(β2-GPI)由五个同源结构域重复序列组成。我们设计了一系列人β2-GPI突变基因,即三个缺失NH2末端区域存在的结构域的突变基因,以及两个缺失COOH末端区域存在的结构域的突变基因。这些突变基因在感染重组杆状病毒的草地贪夜蛾昆虫细胞(Sf9)中表达,突变蛋白分泌到培养基中。通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳估计的纯化突变蛋白的分子量与根据其核苷酸序列计算的大小相当一致。从其完整结构中缺失第五个结构域(结构域V)后,β2-GPI与固相心磷脂(CL)的结合减少。因此,β2-GPI的磷脂结合位点位于其结构域V上。源自NZW×BXSB(WB)F1小鼠或抗磷脂综合征患者的单克隆抗CL抗体(aCL)不仅直接结合在氧化的聚苯乙烯表面,而且结合在普通聚苯乙烯表面吸附的缺失结构域V的突变蛋白(DI-IV)上。我们从这项研究得出结论,aCL的表位通过与带负电荷的磷脂相互作用或在突变蛋白DI-IV上暴露于β2-GPI的构象变化结构上。

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