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孵育过程中细胞内蛋白质与红细胞膜的结合:海因茨小体的产生。

Binding of intracellular protein to the erythrocyte membrane during incubation: the production of Heinz bodies.

作者信息

Sears D A, Friedman J M, White D R

出版信息

J Lab Clin Med. 1975 Nov;86(5):722-32.

PMID:810529
Abstract

During sterile incubation of normal human erythrocytes at 37 degrees C., intracellular nonhemoglobin protein is bound to the membrane prior to hemolysis. These studies have characterized this phenomenon further. Protein binding to the membrane began after 12 hours incubation when cellular ATP was depleted and increased to 36 hours incubation. The binding was prevented by adding adenosine or glucose at the start of incubation and was arrested by adding adenosine to regenerate ATP during the course of incubation. However, protein, once bound, was not released by regeneration of ATP. The amount of protein bound was not altered by: (1) addition of Ca++ or EDTA to the medium, (2) blockade of sulfhydryl groups with N-ethylmaleimide, or (3) stabilization of heme-globin bonds by conversion of hemoglobin to cyanmethemoglobin. Conversion of hemoglobin to carboxyhemoglobin by incubations under carbon monoxide inhibited protein binding, but this appeared to be an effect of exclusion of oxygen rather than stabilization of heme-globin bonds since incubation under nitrogen had a similar effect. The morphological counterpart of this chemically-measured membrane-bound protein was visible in red cell ghosts stained with crystal violet as small membrane-associated particles resembling Heinz bodies. Sodium dodecyl sulfate acrylamide gel electrophoresis of membranes of incubated cells revealed a new protein band that was identical to globin monomers. This membrane binding of globin during incubation provides a model for the study of Heinz body formation in clinical disorders.

摘要

在37摄氏度对正常人红细胞进行无菌培养时,细胞内非血红蛋白蛋白在溶血前与细胞膜结合。这些研究进一步描述了这一现象。蛋白与细胞膜的结合在培养12小时后开始,此时细胞内ATP耗尽,至培养36小时时结合增加。在培养开始时加入腺苷或葡萄糖可防止这种结合,在培养过程中加入腺苷使ATP再生可使结合停止。然而,一旦蛋白结合,ATP再生并不能使其释放。结合的蛋白量不受以下因素影响:(1) 向培养基中添加Ca++或乙二胺四乙酸 (EDTA);(2) 用N-乙基马来酰亚胺封闭巯基;(3) 通过将血红蛋白转化为氰化高铁血红蛋白来稳定血红素-珠蛋白键。在一氧化碳环境下培养使血红蛋白转化为羧基血红蛋白会抑制蛋白结合,但这似乎是由于排除了氧气而非稳定了血红素-珠蛋白键,因为在氮气环境下培养也有类似效果。这种化学测量的膜结合蛋白在形态学上的对应物在用结晶紫染色的红细胞影中可见,为类似于海因茨小体的小膜相关颗粒。对培养细胞的细胞膜进行十二烷基硫酸钠聚丙烯酰胺凝胶电泳显示出一条新的蛋白带,它与珠蛋白单体相同。培养过程中珠蛋白的这种膜结合为研究临床疾病中海因茨小体的形成提供了一个模型。

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Binding of intracellular protein to the erythrocyte membrane during incubation: the production of Heinz bodies.孵育过程中细胞内蛋白质与红细胞膜的结合:海因茨小体的产生。
J Lab Clin Med. 1975 Nov;86(5):722-32.
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Altered sulfhydryl reactivity of hemoglobins and red blood cell membranes in congenital Heinz body hemolytic anemia.先天性 Heinz 小体溶血性贫血中血红蛋白和红细胞膜巯基反应性的改变
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Characterization of alpha-soluble N-ethylmaleimide-sensitive fusion attachment protein in alveolar type II cells: implications in lung surfactant secretion.肺泡II型细胞中α-可溶性N-乙基马来酰亚胺敏感融合附着蛋白的特性:对肺表面活性物质分泌的影响
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Complex effects of sulfhydryl reagents on ligand interactions with nucleoside transporters: evidence for multiple populations of ENT1 transporters with differential sensitivities to N-ethylmaleimide.巯基试剂对配体与核苷转运体相互作用的复杂影响:对N-乙基马来酰亚胺敏感性不同的多种ENT1转运体群体的证据
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Metabolic dependence of red cell deformability.红细胞变形性的代谢依赖性。
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Measurement of hemoglobin chains bound to the erythrocyte membrane. Development of a method and studies of incubated normal cells.与红细胞膜结合的血红蛋白链的测定。一种方法的开发及对孵育的正常细胞的研究。
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Effects of Ca2+ on erythrocyte membrane skeleton-bound phosphofructokinase, ATP levels, and hemolysis.钙离子对红细胞膜骨架结合磷酸果糖激酶、ATP水平及溶血的影响。
Mol Genet Metab. 1999 Jan;66(1):56-61. doi: 10.1006/mgme.1998.2773.

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Proc Natl Acad Sci U S A. 1986 Aug;83(16):6137-41. doi: 10.1073/pnas.83.16.6137.
3
An ultrastructural study of the red pulp of the spleen and the liver in unstable hemoglobin hemolytic anemia.
不稳定血红蛋白溶血性贫血时脾脏和肝脏红髓的超微结构研究
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