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配体诱导的转染了N-甲酰肽受体的淋巴细胞与活化内皮细胞及血管细胞黏附分子-1的黏附。

Ligand-induced adhesion to activated endothelium and to vascular cell adhesion molecule-1 in lymphocytes transfected with the N-formyl peptide receptor.

作者信息

Honda S, Campbell J J, Andrew D P, Engelhardt B, Butcher B A, Warnock R A, Ye R D, Butcher E C

机构信息

Department of Pathology, Stanford University School of Medicine, CA 94305.

出版信息

J Immunol. 1994 Apr 15;152(8):4026-35.

PMID:7511663
Abstract

Binding of FMLP to the neutrophil N-formyl peptide receptor (FPR) transmits signals through pertussis toxin-sensitive G proteins triggering Ca2+ flux, superoxide production, granule exocytosis, and neutrophil aggregation and adhesion involving the beta 2 (CD18) integrins. Expression of the FPR in mouse fibroblasts or human kidney cells has been shown to confer an N-formyl peptide-inducible Ca2+ flux in transfectants. Here we demonstrate that the transfected receptor can also support ligand-induced alterations in cellular adhesion. We established stable transfectants of mouse L1-2 pre-B cells with cDNA for human FPR (L1-2 FPR cells). The transfectants bind N-formyl-Nle-Leu-Phe-Nle-Tyr-Lys-fluorescein with 1.4 x 10(5) sites per cell and a dissociation constant of 3.3 nM. Stimulation with FMLP induces a transient Ca2+ flux. FMLP also triggers adhesion of L1-2 FPR cells to TNF-alpha- or LPS-activated bEnd3 cells (mouse brain-derived endothelial cells) and to purified mouse VCAM-1. Binding is inhibited by Abs to VCAM-1 and to the alpha-chain of its lymphocyte receptor (the alpha 4 beta 1 integrin, VLA-4). Stimulation with FMLP does not induce a change in cell surface expression of alpha 4. Induced adhesion to VCAM-1 is rapid, detectable at the earliest times measurable (30 to 60 s after FMLP addition), and is inhibited by pertussis toxin. We conclude that FPR can mediate integrin activation not only in neutrophils but also in lymphocytes, and can trigger rapid adhesion via lymphocyte alpha 4 beta 1. The adhesion of lymphocytes is critical to their migration and targeting; our results suggest the possibility of manipulating adhesive responses through expression of chemoattractant receptors in lymphoid cells engineered for cellular therapy, allowing targeted adhesion and potentially migration in response to locally administered ligands.

摘要

甲酰甲硫氨酰-亮氨酰-苯丙氨酸(FMLP)与中性粒细胞N-甲酰肽受体(FPR)结合后,通过百日咳毒素敏感的G蛋白传递信号,引发钙离子通量、超氧化物生成、颗粒胞吐作用以及涉及β2(CD18)整合素的中性粒细胞聚集和黏附。FPR在小鼠成纤维细胞或人肾细胞中的表达已被证明能使转染细胞产生N-甲酰肽诱导的钙离子通量。在此,我们证明转染的受体还能支持配体诱导的细胞黏附改变。我们用人类FPR的cDNA建立了小鼠L1-2前B细胞的稳定转染细胞系(L1-2 FPR细胞)。转染细胞以每细胞1.4×10⁵个位点的密度结合N-甲酰-Nle-亮氨酰-苯丙氨酸-Nle-酪氨酸-赖氨酸-荧光素,解离常数为3.3 nM。用FMLP刺激可诱导短暂的钙离子通量。FMLP还能触发L1-2 FPR细胞与肿瘤坏死因子-α或脂多糖激活的bEnd3细胞(小鼠脑源性内皮细胞)以及纯化的小鼠血管细胞黏附分子-1(VCAM-1)的黏附。抗VCAM-1及其淋巴细胞受体α链(α4β1整合素,VLA-4)的抗体可抑制这种黏附。用FMLP刺激不会诱导α4细胞表面表达的改变。诱导的与VCAM-1的黏附迅速,在最早可测量的时间(添加FMLP后30至60秒)即可检测到,并且被百日咳毒素抑制。我们得出结论,FPR不仅能在中性粒细胞中介导整合素激活,还能在淋巴细胞中介导,并且能通过淋巴细胞α4β1触发快速黏附。淋巴细胞的黏附对其迁移和靶向至关重要;我们的结果表明,在为细胞治疗而设计的淋巴细胞中通过表达趋化因子受体来操纵黏附反应是有可能的,这使得在局部给予配体时能够实现靶向黏附并可能实现迁移。

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