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人乳铁蛋白与大鼠肝脏的相互作用。

Interaction of human lactoferrin with the rat liver.

作者信息

Debanne M T, Regoeczi E, Sweeney G D, Krestynski F

出版信息

Am J Physiol. 1985 Apr;248(4 Pt 1):G463-9. doi: 10.1152/ajpgi.1985.248.4.G463.

DOI:10.1152/ajpgi.1985.248.4.G463
PMID:2984944
Abstract

Binding of human lactoferrin (hLf) by purified rat liver plasma membranes was studied to clarify whether the liver possesses specific hLf receptors. The binding was rapid between 4 degrees and 37 degrees C, with a pH optimum close to 5.0. At 22 degrees C and in glycine-NaOH (5 mM, pH 7.4) containing 150 mM NaCl and 0.5% albumin, 1 microgram of membrane bound a maximum of 11.8 ng hLf. The dissociation constant of the interaction was 1.6 X 10(-7) M. Other proteins of high isoelectric points (lactoperoxidase, lysozyme, and particularly salmine sulfate) and a piperazine derivative inhibited hLf binding in a concentration-dependent manner. In contrast, monosaccharides (galactose, N-acetylgalactosamine, mannose, and fucose) were ineffective. By omitting NaCl from the incubation buffer, binding was increased 3.6-fold. Erythrocyte ghosts bound hLf less firmly and alveolar macrophages more firmly than hepatic plasma membranes. Liver cell fractionations performed after the intravenous injection of labeled hLf showed that approximately 88% of the hepatic radioligand was associated with parenchymal cells. When binding was expressed per unit of cell volume, however, more hLf was present in nonparenchymal than in parenchymal cells, implying that the above value was determined by the relative cell masses rather than affinities alone. It is concluded that the binding of hLf by hepatic plasma membranes is electrostatic, i.e., is mediated by the cationic nature of the ligand, and that it is explicable in terms of a "specific nonreceptor interaction" of the generalized type proposed by Cuatrecasas and Hollenberg (Adv. Protein Chem. 30: 251-451, 1976).

摘要

研究了纯化的大鼠肝细胞膜与人乳铁蛋白(hLf)的结合情况,以阐明肝脏是否具有特异性hLf受体。在4℃至37℃之间结合迅速,最适pH接近5.0。在22℃以及含有150 mM NaCl和0.5%白蛋白的甘氨酸 - NaOH(5 mM,pH 7.4)中,1微克膜最多结合11.8纳克hLf。相互作用的解离常数为1.6×10⁻⁷ M。其他等电点高的蛋白质(乳过氧化物酶、溶菌酶,尤其是硫酸鱼精蛋白)和一种哌嗪衍生物以浓度依赖的方式抑制hLf结合。相比之下,单糖(半乳糖、N - 乙酰半乳糖胺、甘露糖和岩藻糖)无效。通过从孵育缓冲液中省略NaCl,结合增加了3.6倍。红细胞空壳结合hLf的牢固程度低于肝细胞膜,而肺泡巨噬细胞结合得更牢固。静脉注射标记的hLf后进行的肝细胞分级分离显示,约88%的肝脏放射性配体与实质细胞相关。然而,当以每单位细胞体积表示结合时,非实质细胞中的hLf比实质细胞中更多,这意味着上述值是由相对细胞质量而非仅由亲和力决定的。结论是,肝细胞膜对hLf的结合是静电性的,即由配体的阳离子性质介导,并且可以根据Cuatrecasas和Hollenberg提出的广义类型的“特异性非受体相互作用”来解释(《蛋白质化学进展》30: 251 - 451, 1976)。

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