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中性粒细胞胞质颗粒衍生的杀菌/通透性增加蛋白与靶细菌的优先结合。其意义及作为一种纯化手段的用途。

Preferential binding of the neutrophil cytoplasmic granule-derived bactericidal/permeability increasing protein to target bacteria. Implications and use as a means of purification.

作者信息

Mannion B A, Kalatzis E S, Weiss J, Elsbach P

机构信息

Department of Microbiology, New York University School of Medicine, NY 10016.

出版信息

J Immunol. 1989 Apr 15;142(8):2807-12.

PMID:2539411
Abstract

The specificity of the basic bactericidal/permeability increasing protein (BPI) of polymorphonuclear leukocytes (PMN) for gram-negative bacteria is attributable to its strong attraction for the negatively charged envelope LPS. The antibacterial activity of PMN homogenates or extracts toward Escherichia coli corresponds to their BPI content and is blocked by anti-BPI IgG, suggesting that BPI action is unaffected by the presence of other PMN proteins. To test if BPI is preferentially bound to E. coli when other antibacterial proteins are present, we have measured binding in buffered (pH 7.5) balanced salts solution of [125I] human BPI to E. coli J5 in the presence and absence of other human PMN granule proteins. BPI binding is saturable with an apparent K = 23 nM and 2.2 million binding sites/cell. While binding of [125I] human BPI is competitively inhibited by human or rabbit BPI, it is only weakly inhibited by myeloperoxidase, lysozyme, or cathepsin G. In contrast, myeloperoxidase binding to E. coli is strongly inhibited by BPI. Moreover, incubation of E. coli with crude extracts of PMN or CML spleen results in near quantitative binding of BPI, identified by silver staining and immunoblotting after SDS-PAGE of the washed E. coli pellet, without recognizable binding of other leukocyte proteins (greater than 98% of added total protein is recovered in supernatant). After addition of 200 mM MgCl2, approximately 80% of bound BPI is released as fully active and pure protein (as judged by SDS-PAGE and HPLC). Thus the selective and reversible binding of BPI in crude PMN extracts to target bacteria provides a one-step "affinity" purification procedure.

摘要

多形核白细胞(PMN)的碱性杀菌/通透性增加蛋白(BPI)对革兰氏阴性菌的特异性归因于其对带负电荷的包膜脂多糖(LPS)的强烈吸引力。PMN匀浆或提取物对大肠杆菌的抗菌活性与其BPI含量相对应,并被抗BPI IgG阻断,这表明BPI的作用不受其他PMN蛋白的影响。为了测试当存在其他抗菌蛋白时BPI是否优先与大肠杆菌结合,我们在有和没有其他人类PMN颗粒蛋白的情况下,测量了[125I]人BPI在缓冲(pH 7.5)平衡盐溶液中与大肠杆菌J5的结合。BPI结合具有饱和性,表观K = 23 nM,每个细胞有220万个结合位点。虽然[125I]人BPI的结合受到人或兔BPI的竞争性抑制,但仅受到髓过氧化物酶、溶菌酶或组织蛋白酶G的微弱抑制。相反,髓过氧化物酶与大肠杆菌的结合受到BPI的强烈抑制。此外,将大肠杆菌与PMN或慢性粒细胞白血病(CML)脾脏的粗提取物孵育,通过对洗涤后的大肠杆菌沉淀进行SDS-PAGE后的银染和免疫印迹鉴定,结果显示BPI几乎定量结合,而其他白细胞蛋白没有可识别的结合(大于98%的添加总蛋白在上清液中回收)。加入200 mM MgCl2后,约80%结合的BPI以完全活性和纯蛋白形式释放(通过SDS-PAGE和HPLC判断)。因此,粗PMN提取物中BPI与靶细菌的选择性和可逆结合提供了一种一步“亲和”纯化程序。

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