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钙离子和离子载体A23187处理的人红细胞中1,2 - 二酰甘油和磷脂酸的产生

Production of 1,2-diacylglycerol and phosphatidate in human erythrocytes treated with calcium ions and ionophore A23187.

作者信息

Allan D, Watts R, Michell R H

出版信息

Biochem J. 1976 May 15;156(2):225-32. doi: 10.1042/bj1560225.

Abstract
  1. When the ionophore A23187 and Ca2+ were added to normal human erythrocytes, the incorporation of 32P into phosphatidate was enhanced within 1 min, but there was only slight labelling of other phospholipids. 2. Labelling of phosphatidate in these cells did not continue to increase after about 20min at 37 degrees C; by this time, radioactivity in phosphatidate was about ten times higher inionophore A23187-treated cells than in controls. A net synthesis of phosphatidate was measured in response to the increase in intracellular Ca2+ concentration; the content of this phospholipid in the cell was increased by approximately 50%. 3. In the presence of 2.5 mM-Ca2+ a maximum effect was seen with about 0.5 mug of ionophore/ml. 4. The concentration of Ca2+ giving half-maximal labelling of phosphatidate in the presence of 10 mug of ionophore A23187/ml was about 10 muM. 5. A rapid decrease of ATP content in the cell occurred in ionophore-treated cells. 6. Labelling of phosphatidate appeared to be secondary to the production of 1,2-diacylglycerol in the cells; accumulation of 1,2-diacylglycerol was only seen after about 15 min. After 60 min, the 1,2-diacylglycerol content of the cells was five to seven times that of untreated control cells. 7. The change in the shape of erythrocytes treated with Ca2+ and ionophore appeared to be related to accumulation of 1,2-diacylglycerol. 8. The source of 1,2-diacylglycerol has not been definitely identified, but its fatty acid compositon was similar to that of phosphatidylcholine. However, it has an unusually high content of hexadecenoic acid, a fatty acid not common in the major erythrocyte phospholipids. 9. Accumulation of 1,2-diacyglycerol also occurred in energy-starved cells, even in the absence of calcium; in this case it appeared to be produced by phosphatidate breakdown.
摘要
  1. 当向正常人红细胞中添加离子载体A23187和Ca2+时,32P掺入磷脂酸的过程在1分钟内增强,但其他磷脂的标记很轻微。2. 在37℃下约20分钟后,这些细胞中磷脂酸的标记不再继续增加;此时,离子载体A23187处理的细胞中磷脂酸的放射性比对照细胞高约十倍。测量到磷脂酸的净合成是对细胞内Ca2+浓度增加的响应;这种磷脂在细胞中的含量增加了约50%。3. 在2.5 mM - Ca2+存在下,约0.5 μg离子载体/毫升时可见最大效应。4. 在10 μg离子载体A23187/毫升存在下,使磷脂酸标记达到最大值一半时的Ca2+浓度约为10 μM。5. 离子载体处理的细胞中细胞内ATP含量迅速下降。6. 磷脂酸的标记似乎继发于细胞中1,2 - 二酰基甘油的产生;1,2 - 二酰基甘油的积累仅在约15分钟后才可见。60分钟后,细胞中1,2 - 二酰基甘油的含量是未处理对照细胞的五到七倍。7. 用Ca2+和离子载体处理的红细胞形状变化似乎与1,2 - 二酰基甘油的积累有关。8. 1,2 - 二酰基甘油的来源尚未明确确定,但其脂肪酸组成与磷脂酰胆碱相似。然而,它含有异常高含量的十六碳烯酸,这是一种在主要红细胞磷脂中不常见的脂肪酸。9. 1,2 - 二酰基甘油的积累也发生在能量缺乏的细胞中,即使在没有钙的情况下也是如此;在这种情况下,它似乎是由磷脂酸分解产生的。

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