Hamann K J, Neeley S P, Dowling T L, Grant J A, Leff A R
Department of Medicine, University of Chicago, IL 60637, USA.
Blood. 1996 Nov 1;88(9):3575-82.
We examined the selective effects of interleukin (IL-5) in regulating the maturational expression of surface adhesion molecules on human eosinophils and adhesion to endothelial cells during eosinophiiopolesis in vitro. Expression of the beta 2 integrins (CD11/CD18) and the beta 1 integrin, VLA-4 (CD49d/ CD29), was assessed during development in culture with IL-3, IL-5, and granulocyte-macrophage colony stimulating factor in cultures of human umbilical cord blood-derived eosinophil (CDE) precursor cells. Expression of both CD11b and CD18 subunits of Mac-1 was lower on CDE which were continuously (= chronically) exposed to IL-5 than on CDE which were cultured without IL-5 for the final week of culture. CD11b expression on cells grown without IL-5 was 71.3 +/- 5.92 (mean specific fluorescence value [MSF] as measured by flow cytometry) versus 52.5 +/- 4.48 MSF for Mac-1 alpha (CD11b) on CDE grown in the continued presence of 2 x 10 - 11 mol/L IL-5 (P < .01). Although expression of VLA-4 decreased as CDE matured, expression of CD29 and CD49d were similar regardless of cytokine exposure for the final week of culture. For eosinophils cultured without IL-5, acute stimulation with 10 - 8 mol/L IL-5 increased CD11b surface expression and increased the number of cells adhering to unstimulated human umbilical vein endothelial cells (HUVEC) from 4,570 +/- 780 cells (9.14 +/- 1.56% adhesion) to 8,385 +/- 515 cells (16.8 +/- 1.03% adhesion) (P < .01). Basal adhesion to unstimulated HUVEC of CDE cultured continuously with IL-5 was comparable (8.62 +/- 1.12% adhesion; P = NS), but neither CD11b expression (50.3 +/- 11.8 MSF; P = NS v control) nor adhesion to HUVEC (6.77 +/- 1.35%; P = NS) was enhanced in these eosinophils after acute stimulation with IL-5. Blockade of adhesion to IL-1-stimulated HUVEC caused by the anti-CD49d monoclonal antibody (MoAb), HP2/1, was comparable for cells cultured with IL-5 and without IL-5. However, the anti-CD18 MoAb, R15.7, caused 47.6 +/- 5.08% inhibition of adhesion of eosinophils cultured without IL-5 and only 25.8 +/- 5.20% for cells cultured continuously with IL-5 (P < .01), and failed to block significantly the adhesion of only the latter cells to IL-4-stimulated HUVEC. Our data show that continuous, chronic exposure to low concentrations of IL-5 causes decreased expression of Mac-1 and refractoriness to acute stimulation with IL-5 of adhesion to HUVEC. These data further demonstrate that CDE maturing in the continued presence of IL-5 adhere to HUVEC predominantly through VLA-4 ligation.
我们研究了白细胞介素(IL-5)在体外嗜酸性粒细胞生成过程中对人嗜酸性粒细胞表面黏附分子成熟表达及与内皮细胞黏附的选择性作用。在人脐带血来源的嗜酸性粒细胞(CDE)前体细胞培养物中,用IL-3、IL-5和粒细胞-巨噬细胞集落刺激因子培养时,评估β2整合素(CD11/CD18)和β1整合素VLA-4(CD49d/CD29)的表达。在培养的最后一周,持续(即慢性)暴露于IL-5的CDE上Mac-1的CD11b和CD18亚基的表达低于未用IL-5培养的CDE。未用IL-5培养的细胞上CD11b的表达为71.3±5.92(通过流式细胞术测量的平均特异性荧光值[MSF]),而在持续存在2×10-11mol/L IL-5的情况下培养的CDE上Mac-1α(CD11b)的MSF为52.5±4.48(P<.01)。尽管随着CDE成熟VLA-4的表达降低,但无论培养最后一周的细胞因子暴露情况如何,CD29和CD49d的表达相似。对于未用IL-5培养的嗜酸性粒细胞,用10-8mol/L IL-5急性刺激可增加CD11b表面表达,并使黏附于未刺激的人脐静脉内皮细胞(HUVEC)的细胞数量从4570±780个细胞(黏附率9.14±1.56%)增加到8385±515个细胞(黏附率16.8±1.03%)(P<.01)。持续用IL-5培养的CDE对未刺激的HUVEC的基础黏附率相当(黏附率8.62±1.12%;P=无显著性差异),但在用IL-5急性刺激后,这些嗜酸性粒细胞的CD11b表达(50.3±11.8 MSF;与对照相比P=无显著性差异)和对HUVEC的黏附(6.77±1.35%;P=无显著性差异)均未增强。抗CD49d单克隆抗体(MoAb)HP2/1对IL-1刺激的HUVEC黏附的阻断作用,在用IL-5培养和未用IL-5培养的细胞中相当。然而,抗CD-18 MoAb R15.7对未用IL-5培养的嗜酸性粒细胞黏附的抑制率为47.6±5.08%,而对持续用IL-5培养的细胞仅为25.8±5.20%(P<.01),并且未能显著阻断仅后者细胞对IL-4刺激的HUVEC的黏附。我们的数据表明,持续慢性暴露于低浓度IL-5会导致Mac-1表达降低以及对IL-5急性刺激的HUVEC黏附产生不应性。这些数据进一步证明在持续存在IL-5的情况下成熟的CDE主要通过VLA-4连接黏附于HUVEC。
Zotero 插件