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锚蛋白缺陷型幼红细胞增多症(nb/nb)小鼠红细胞中蛋白质4.2含量降低:锚蛋白增强蛋白质4.2膜结合的证据。

Decreased content of protein 4.2 in ankyrin-deficient normoblastosis (nb/nb) mouse red blood cells: evidence for ankyrin enhancement of protein 4.2 membrane binding.

作者信息

Rybicki A C, Musto S, Schwartz R S

机构信息

Albert Einstein College of Medicine-Montefiore Medical Center, Division of Hematology, Bronx, NY 10467, USA.

出版信息

Blood. 1995 Nov 1;86(9):3583-9.

PMID:7579467
Abstract

Homozygous normoblastosis (nb/nb) mice, whose red blood cell (RBC) membranes are nearly completely deficient in full-length 210-kD ankyrin, were used to study interactions between ankyrin and protein 4.2 (P4.2). Although it is unclear whether or not these proteins interact in the membrane, both ankyrin and P4.2 bind to the cytoplasmic domain of band 3 (cdb3). In addition to the complete deficiency of full-length ankyrin, nb/nb RBC membranes are also partially spectrin deficient, resulting in morphologically spherocytic and mechanically fragile cells. A new finding was that nb/nb RBC membranes are severely (approximately 73%) P4.2 deficient compared with wild type (+/+) or high reticulocyte mouse RBC membranes. Metabolic labeling of nb/nb reticulocytes showed active P4.2 synthesis at levels comparable with high reticulocyte controls suggesting that the nb/nb P4.2 deficiency was not the result of defective P4.2 synthesis. Reconstitution of nb/nb inside-out vesicles (IOVs) with human RBC ankyrin restored ankyrin levels to approximately 80% of +/+ IOV levels and increased binding of exogenously added human RBC P4.2 by approximately 60%. These results suggest that ankyrin is required for normal associations of P4.2 with the RBC membrane.

摘要

纯合性成红细胞增多症(nb/nb)小鼠的红细胞(RBC)膜几乎完全缺乏全长210-kD锚蛋白,被用于研究锚蛋白与蛋白4.2(P4.2)之间的相互作用。尽管尚不清楚这些蛋白在膜中是否相互作用,但锚蛋白和P4.2均与带3的胞质结构域(cdb3)结合。除了完全缺乏全长锚蛋白外,nb/nb RBC膜的血影蛋白也部分缺乏,导致细胞形态呈球形且机械性能脆弱。一项新发现是,与野生型(+/+)或高网织红细胞小鼠RBC膜相比,nb/nb RBC膜严重缺乏(约73%)P4.2。nb/nb网织红细胞的代谢标记显示,P4.2的合成活性水平与高网织红细胞对照相当,这表明nb/nb P4.2缺乏并非P4.2合成缺陷的结果。用人RBC锚蛋白重建nb/nb内翻囊泡(IOV),使锚蛋白水平恢复到+/+ IOV水平的约80%,并使外源添加的人RBC P4.2的结合增加了约60%。这些结果表明,锚蛋白是P4.2与RBC膜正常结合所必需的。

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