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重组可溶性人CD3分子的表达与特性:天然TCR-CD3复合物上定义的抗原表位的呈现

Expression and characterization of recombinant soluble human CD3 molecules: presentation of antigenic epitopes defined on the native TCR-CD3 complex.

作者信息

Law Che-Leung, Hayden-Ledbetter Martha, Buckwalter Sonya, McNeill Lisa, Nguyen Hieu, Habecker Phil, Thorne Barbara A, Dua Raj, Ledbetter Jeffrey A

机构信息

Xcyte Therapies, Inc., Seattle, WA 98104, USA.

出版信息

Int Immunol. 2002 Apr;14(4):389-400. doi: 10.1093/intimm/14.4.389.

Abstract

The TCR-CD3 complex consists of the clonotypic disulfide-linked TCRalphabeta or TCRdeltagamma heterodimers, and the invariant CD3delta, epsilon, gamma and zeta chains. We generated plasmid constructs expressing the extracellular domains of the CD3delta, epsilon or gamma subunits fused to human IgG1 Fc. Recombinant fusion proteins consisting of individual CD3delta, epsilon or gamma subunits reacted poorly with anti-CD3 mAb including G19-4, BC3, OKT3 and 64.1. Co-expression of the CD3epsilon-Ig with either the CD3delta-Ig (CD3epsilondelta-Ig) or the CD3gamma-Ig (CD3epsilongamma-Ig) resulted in fusion proteins with much increased binding to G19-4. A brief acid treatment of the purified CD3epsilondelta-Ig fusion protein substantially improved its binding to BC3, OKT3 and 64.1. Surface plasmon resonance analysis revealed that the dissociation constants for CD3epsilondelta-Ig and anti-CD3 mAb ranged from 10(-8) to 10(-9) M. Based on these results, a single-chain (sc) construct encoding the CD3delta chain linked to the CD3epsilon chain with a flexible linker followed by human IgG1 Fc was expressed. The sc CD3deltaepsilon-scIg reacted with anti-CD3 mAb without requiring acid treatment. Moreover, anti-CD3 mAb bound CD3epsilondelta-Ig at a higher affinity than CD3epsilongamma-Ig, suggesting potential structural differences between the CD3epsilondelta and CD3epsilongamma subunits. In summary, we report the expression of soluble recombinant CD3 proteins that demonstrate structural characteristics of the native CD3 complex expressed on the T cell surface. These CD3 fusion proteins can be used to further analyze the structure of the TCR-CD3 complex, and to identify molecules that can interfere with TCR-CD3-mediated signal transduction by disrupting the interaction between CD3 and TCR subunits.

摘要

TCR-CD3复合物由克隆型二硫键连接的TCRαβ或TCRδγ异二聚体以及恒定的CD3δ、ε、γ和ζ链组成。我们构建了表达与人IgG1 Fc融合的CD3δ、ε或γ亚基胞外结构域的质粒。由单个CD3δ、ε或γ亚基组成的重组融合蛋白与包括G19-4、BC3、OKT3和64.1在内的抗CD3单克隆抗体反应较差。CD3ε-Ig与CD3δ-Ig(CD3εδ-Ig)或CD3γ-Ig(CD3εγ-Ig)共表达产生的融合蛋白与G19-4的结合力大大增强。对纯化的CD3εδ-Ig融合蛋白进行短暂酸处理可显著改善其与BC3、OKT3和64.1的结合。表面等离子体共振分析表明,CD3εδ-Ig与抗CD3单克隆抗体的解离常数范围为10^(-8)至10^(-9) M。基于这些结果,表达了一种单链(sc)构建体,其编码通过柔性接头连接到CD3ε链的CD3δ链,随后是人IgG1 Fc。sc CD3δε-scIg与抗CD3单克隆抗体反应,无需酸处理。此外,抗CD3单克隆抗体与CD3εδ-Ig的结合亲和力高于CD3εγ-Ig,并表明CD3εδ和CD3εγ亚基之间存在潜在的结构差异。总之,我们报道了可溶性重组CD3蛋白的表达,其展示了T细胞表面表达的天然CD3复合物的结构特征。这些CD3融合蛋白可用于进一步分析TCR-CD3复合物的结构,并鉴定可通过破坏CD3与TCR亚基之间的相互作用来干扰TCR-CD3介导的信号转导的分子。

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