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ABH抗原作为荆豆凝集素I激活红细胞阴离子交换的识别位点。

ABH antigens as recognition sites for the activation of red blood cell anion exchange by the lectin ulex europaeus agglutinin I.

作者信息

Engelmann B

机构信息

Physiologisches Institut, Universität München, Germany.

出版信息

J Cell Physiol. 1993 Nov;157(2):403-7. doi: 10.1002/jcp.1041570224.

DOI:10.1002/jcp.1041570224
PMID:7693725
Abstract

The blood group antigen H (blood group O) and fucose-specific lectin Ulex europaeus agglutinin I (UEA1) (10 micrograms/ml) was found to increase the rate constant of Cl- efflux into 100 mM Na+ oxalate media by about 40% in erythrocytes taken from antigen H donors. In 100 mM K+ oxalate, 150 mM Na+ pyruvate and in 150 mM Na+ acetate media the lectin elevated the rate constant of Cl- efflux by 20-50%. The acceleration of Cl- efflux by UEA1 was completely blocked by 10 microM 4,4'-diisothiocyanato-stilbene-2,2'-disulfonic acid (DIDS) indicating that the effect of the lectin is mediated by the anion exchanger of human erythrocytes (band 3 protein). In antigen A1 erythrocytes no significant stimulation of anion exchange by UEA1 was seen. The activation of Cl- efflux was completely prevented by addition of 1 mM fucose to the medium. These results suggest that the effect of UEA1 is mediated through interaction with the fucose residues of H antigens. Increasing extracellular Ca++ from 0.5 to 5 mM in Na+ pyruvate or Na+ acetate media slightly reduced the acceleration of anion exchange by the lectin. On the other hand, replacing part of extracellular chloride by bicarbonate did not considerably alter the (previously reported) stimulatory effect of UEA1 on red blood cell Ca++ uptake. This suggests that the acceleration of anion exchange and of Ca++ uptake by UEA1, respectively, are mediated by different mechanisms. It is concluded that UEA1 activates anion exchange of human erythrocytes most probably by a direct interaction with H antigens present on extracellular domains of the band 3 protein.

摘要

研究发现,血型抗原H(O血型)和岩藻糖特异性凝集素荆豆凝集素I(UEA1)(10微克/毫升)可使来自H抗原供体的红细胞中氯离子外流至100毫摩尔/升草酸钠培养基中的速率常数提高约40%。在100毫摩尔/升草酸钾、150毫摩尔/升丙酮酸钠和150毫摩尔/升乙酸钠培养基中,该凝集素使氯离子外流的速率常数提高了20% - 50%。10微摩尔/升的4,4'-二异硫氰酸根合芪-2,2'-二磺酸(DIDS)可完全阻断UEA1对氯离子外流的加速作用,这表明该凝集素的作用是由人红细胞的阴离子交换体(带3蛋白)介导的。在A1抗原红细胞中,未观察到UEA1对阴离子交换有明显刺激作用。向培养基中添加1毫摩尔/升岩藻糖可完全阻止氯离子外流的激活。这些结果表明,UEA1的作用是通过与H抗原的岩藻糖残基相互作用介导的。在丙酮酸钠或乙酸钠培养基中,将细胞外钙离子浓度从0.5毫摩尔/升提高到5毫摩尔/升,可略微降低凝集素对阴离子交换的加速作用。另一方面,用碳酸氢根替代部分细胞外氯离子,并未显著改变(先前报道的)UEA1对红细胞钙离子摄取的刺激作用。这表明,UEA1对阴离子交换和钙离子摄取的加速作用分别是由不同机制介导的。研究得出结论,UEA1最有可能通过与带3蛋白细胞外结构域上存在的H抗原直接相互作用来激活人红细胞的阴离子交换。

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