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钙负载的人红细胞中的膜磷脂组织

Membrane phospholipid organization in calcium-loaded human erythrocytes.

作者信息

Chandra R, Joshi P C, Bajpai V K, Gupta C M

出版信息

Biochim Biophys Acta. 1987 Aug 20;902(2):253-62. doi: 10.1016/0005-2736(87)90303-8.

Abstract

Intracellular Ca2+ levels in human erythrocytes were increased by incubating them with variable concentrations of Ca2+ in the presence of ionophore A23187. Experiments were done to confirm that the Ca2+ loading did induce changes in the cell shape and membrane protein composition. The effect of the increased cytoplasmic Ca2+ levels on the membrane phospholipid organization was analysed using bee venom and pancreatic phospholipases A2, Merocyanine 540 and fluorescamine as the external membrane probes. About 20% phosphatidylethanolamine (PE) and 0% phosphatidylserine (PS) were hydrolysed by the phospholipases in intact control cells, whereas in identical conditions these enzymes readily degraded, 20-30% PE and 7-30% PS, in Ca2+-loaded erythrocytes, depending on the cytoplasmic Ca2+ concentration. Also, Merocyanine 540 failed to stain the fresh or control erythrocytes, but it labeled the cells loaded with Ca2+. Furthermore, fluorescamine labeled approx. 20% PE in fresh or control erythrocytes while in identical conditions, significantly higher amounts of PE were modified in intact Ca2+-loaded cells. These results demonstrate that Ca2+ loading in human erythrocytes leads to loss of the transbilayer phospholipid asymmetry, and suggest that, together with spectrin, polypeptides 2.1 and 4.1 may also play an important role in maintaining the asymmetric distribution of various phospholipids across the erythrocyte membrane bilayer.

摘要

在离子载体A23187存在的情况下,将人红细胞与不同浓度的Ca2+一起孵育,可使细胞内Ca2+水平升高。进行实验以确认Ca2+负载确实会引起细胞形状和膜蛋白组成的变化。使用蜂毒和胰腺磷脂酶A2、部花青540和荧光胺作为外膜探针,分析了细胞质Ca2+水平升高对膜磷脂组织的影响。在完整的对照细胞中,磷脂酶可水解约20%的磷脂酰乙醇胺(PE)和0%的磷脂酰丝氨酸(PS),而在相同条件下,这些酶在Ca2+负载的红细胞中可轻易降解20%-30%的PE和7%-30%的PS,这取决于细胞质Ca2+浓度。此外,部花青540无法对新鲜或对照红细胞进行染色,但它可标记Ca2+负载的细胞。此外,荧光胺可标记新鲜或对照红细胞中约20%的PE,而在相同条件下,完整的Ca2+负载细胞中被修饰的PE量明显更高。这些结果表明,人红细胞中的Ca2+负载会导致跨膜磷脂不对称性的丧失,并表明,与血影蛋白一起,多肽2.1和4.1可能在维持各种磷脂在红细胞膜双层中的不对称分布方面也发挥重要作用。

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