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2
Human cell-adhesion molecule CD2 binds CD58 (LFA-3) with a very low affinity and an extremely fast dissociation rate but does not bind CD48 or CD59.人类细胞黏附分子CD2以极低的亲和力和极快的解离速率与CD58(淋巴细胞功能相关抗原3)结合,但不与CD48或CD59结合。
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3
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Characterisation of the low affinity interaction between rat cell adhesion molecules CD2 and CD48 by analytical ultracentrifugation.通过分析超速离心法对大鼠细胞黏附分子CD2和CD48之间低亲和力相互作用的表征。
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N-glycosylation is required for human CD2 immunoadhesion functions.人CD2免疫粘附功能需要N-糖基化。
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Expression of soluble recombinant glycoproteins with predefined glycosylation: application to the crystallization of the T-cell glycoprotein CD2.具有预定义糖基化的可溶性重组糖蛋白的表达:应用于T细胞糖蛋白CD2的结晶
Protein Eng. 1993 Feb;6(2):229-32. doi: 10.1093/protein/6.2.229.
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Identification of the T cell surface signal-transducing glycoprotein sgp-60 as CD48, a counter-receptor for mouse CD2.将T细胞表面信号转导糖蛋白sgp-60鉴定为CD48,即小鼠CD2的反受体。
Eur J Immunol. 1993 Jun;23(6):1412-5. doi: 10.1002/eji.1830230638.
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A soluble multimeric recombinant CD2 protein identifies CD48 as a low affinity ligand for human CD2: divergence of CD2 ligands during the evolution of humans and mice.一种可溶性多聚体重组CD2蛋白将CD48鉴定为人CD2的低亲和力配体:人类和小鼠进化过程中CD2配体的差异
J Exp Med. 1993 May 1;177(5):1439-50. doi: 10.1084/jem.177.5.1439.
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SH2 domains exhibit high-affinity binding to tyrosine-phosphorylated peptides yet also exhibit rapid dissociation and exchange.SH2结构域对酪氨酸磷酸化肽段具有高亲和力结合,但也表现出快速解离和交换。
Mol Cell Biol. 1993 Mar;13(3):1449-55. doi: 10.1128/mcb.13.3.1449-1455.1993.
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Human anti-self antibodies with high specificity from phage display libraries.来自噬菌体展示文库的具有高特异性的人抗自身抗体。
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6
Structural analysis of the CD2 T lymphocyte antigen by site-directed mutagenesis to introduce a disulphide bond into domain 1.通过定点诱变对CD2 T淋巴细胞抗原进行结构分析,以在结构域1中引入二硫键。
Protein Eng. 1993 Nov;6(8):965-70. doi: 10.1093/protein/6.8.965.
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The kinetics of antibody binding to membrane antigens in solution and at the cell surface.抗体与溶液中和细胞表面膜抗原结合的动力学。
Biochem J. 1980 Apr 1;187(1):1-20. doi: 10.1042/bj1870001.
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The labelling of proteins to high specific radioactivities by conjugation to a 125I-containing acylating agent.通过与含¹²⁵I的酰化剂结合将蛋白质标记至高比放射性。
Biochem J. 1973 Jul;133(3):529-39. doi: 10.1042/bj1330529.
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The immunoglobulin superfamily--domains for cell surface recognition.免疫球蛋白超家族——细胞表面识别结构域
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The MRC OX-45 antigen of rat leukocytes and endothelium is in a subset of the immunoglobulin superfamily with CD2, LFA-3 and carcinoembryonic antigens.大鼠白细胞和内皮细胞的MRC OX - 45抗原属于免疫球蛋白超家族的一个子集,该超家族还包括CD2、淋巴细胞功能相关抗原3(LFA - 3)和癌胚抗原。
EMBO J. 1988 Oct;7(10):3087-91. doi: 10.1002/j.1460-2075.1988.tb03174.x.

大鼠细胞黏附分子CD2与CD48相互作用的亲和力及动力学分析

Affinity and kinetic analysis of the interaction of the cell adhesion molecules rat CD2 and CD48.

作者信息

van der Merwe P A, Brown M H, Davis S J, Barclay A N

机构信息

MRC Cellular Immunology Unit, Sir William Dunn School of Pathology, University of Oxford, UK.

出版信息

EMBO J. 1993 Dec 15;12(13):4945-54. doi: 10.1002/j.1460-2075.1993.tb06188.x.

DOI:10.1002/j.1460-2075.1993.tb06188.x
PMID:7903240
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC413755/
Abstract

CD2 is a plasma membrane glycoprotein present on T lymphocytes that functions as a cell adhesion molecule (CAM). The CD2 counter-receptor in rodents is the structurally-related CAM CD48. Intercellular adhesion involves the formation of multiple CAM complexes between adhering cells and de-adhesion requires disruption of these complexes. To gain an insight into the initiation and termination of intercellular adhesion, the kinetics and affinity of the rat CD2-CD48 interaction was analysed using a BIAcore instrument, which enables the monitoring of protein binding in real time. A soluble chimeric protein, comprising the extracellular portion of rat CD48 and domains 3 and 4 of rat CD4 (sCD48-CD4), bound to immobilized soluble CD2 (sCD2) with a KD of 90 microM. The affinity was also determined in the reverse orientation and sCD2 was shown to bind immobilized sCD48-CD4 with a comparable KD of 60 microM. sCD48-CD4 bound to immobilized deglycosylated sCD2 with a KD of 125 microM, indicating that glycosylation of sCD2 has little effect on the affinity of the interaction. The low affinity was the result of an extremely rapid off-rate constant (K(off) > or = 6 s-1), whereas the on-rate constant was unremarkable (K(on) > or = 10(5) M-1s-1). The kinetic analysis revealed that small amounts of multimeric aggregates of sCD48-CD4 formed in concentrated preparations. Our experience suggests that even low concentrations (< 2%) of these aggregates may be a cause of artifactually high affinity values when analysing low-affinity protein interactions. In conclusion, this study provides the first detailed analysis of the kinetics and affinity of monomeric CAM interactions and suggests that binding between CAMs may be weaker than anticipated.

摘要

CD2是一种存在于T淋巴细胞上的质膜糖蛋白,起细胞粘附分子(CAM)的作用。啮齿动物中的CD2反受体是结构相关的CAM CD48。细胞间粘附涉及粘附细胞之间多个CAM复合物的形成,而去粘附则需要破坏这些复合物。为了深入了解细胞间粘附的起始和终止,使用BIAcore仪器分析了大鼠CD2-CD48相互作用的动力学和亲和力,该仪器能够实时监测蛋白质结合。一种可溶性嵌合蛋白,由大鼠CD48的细胞外部分和大鼠CD4的结构域3和4组成(sCD48-CD4),以90微摩尔的解离常数(KD)与固定化的可溶性CD2(sCD2)结合。还以相反方向测定了亲和力,结果显示sCD2以60微摩尔的可比KD与固定化的sCD48-CD4结合。sCD48-CD4以125微摩尔的KD与固定化的去糖基化sCD2结合,表明sCD2的糖基化对相互作用的亲和力影响很小。低亲和力是极高的解离速率常数(K(off)≥6 s-1)的结果,而结合速率常数并不显著(K(on)≥10(5) M-1s-1)。动力学分析表明,在浓缩制剂中形成了少量sCD48-CD4的多聚体聚集体。我们的经验表明,在分析低亲和力蛋白质相互作用时,即使是低浓度(<2%)的这些聚集体也可能是导致人为高亲和力值的原因。总之,本研究首次对单体CAM相互作用的动力学和亲和力进行了详细分析,并表明CAM之间的结合可能比预期的弱。