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伴刀豆球蛋白A刺激的淋巴细胞中固醇合成增强:与磷脂合成和DNA合成的相关性

Enhanced sterol synthesis in concanavalin A-stimulated lymphocytes: correlation with phospholipid synthesis and DNA synthesis.

作者信息

Chen S S

出版信息

J Cell Physiol. 1979 Jul;100(1):147-57. doi: 10.1002/jcp.1041000115.

Abstract

Incorporation of (14C)choline and (3H)myo-inositol into the total lipid fraction, incorporation of (14C)acetate into the sterol fraction and incorporation of (3H)thymidine into DNA were studied in human lymphocyte cultures. Concanavalin A induced an increase in the incorporation of these labels with the following features: (a) Phospholipid synthesis was increased promptly. The lag time for the increase in sterol synthesis and DNA synthesis were 5 hours and 27 hours respectively; (b) The increase in phospholipid synthesis and sterol synthesis was proportional to ConA concentration initially. Cells treated with a high concentration of ConA showed very low levels of DNA synthesis; (c) The increase in phospholipid synthesis could be abolished immediately by alpha-Methyl-Mannoside. alpha-Methyl-Mannoside blunted but did not abolish the increase in sterol synthesis. alpha-Methyl-Mannoside enhanced DNA synthesis of those cells which had been treated by a high concentration of ConA; and (d) Selective inhibition of sterol synthesis with 25-hydroxycholesterol did not prevent the increase in phospholipid synthesis, but it blocked the increase in DNA synthesis. Supplement of LDL, HDL or total lipoproteins to lymphocyte cultures was effective in preventing the inhibition of DNA synthesis by 25-hydroxy-cholesterol. These results suggest that in lymphocyte activation by ConA phospholipid synthesis, sterol synthesis and DNA synthesis were sequentially increased. The rate of cellular commitment to mitogenesis was proportional to ConA concentrations. High concentrations of ConA arrested the cell growth at a postcommitment point in the G1 phase. Enhanced phospholipid synthesis was a precommitment event. Enhanced sterol synthesis was a postcommitment event and reflected the requirement of an increased cholesterol supply for the passage of cell growth through G1.

摘要

在人淋巴细胞培养物中研究了(14C)胆碱和(3H)肌醇掺入总脂质部分、(14C)乙酸盐掺入甾醇部分以及(3H)胸苷掺入DNA的情况。伴刀豆球蛋白A诱导这些标记物掺入增加,具有以下特点:(a)磷脂合成迅速增加。甾醇合成和DNA合成增加的延迟时间分别为5小时和27小时;(b)磷脂合成和甾醇合成的增加最初与伴刀豆球蛋白A浓度成正比。用高浓度伴刀豆球蛋白A处理的细胞显示出非常低水平的DNA合成;(c)α-甲基甘露糖苷可立即消除磷脂合成的增加。α-甲基甘露糖苷使甾醇合成的增加减弱但未消除。α-甲基甘露糖苷增强了用高浓度伴刀豆球蛋白A处理的细胞的DNA合成;并且(d)用25-羟基胆固醇选择性抑制甾醇合成并不能阻止磷脂合成的增加,但它阻止了DNA合成的增加。向淋巴细胞培养物中补充低密度脂蛋白、高密度脂蛋白或总脂蛋白可有效防止25-羟基胆固醇对DNA合成的抑制。这些结果表明,在伴刀豆球蛋白A激活淋巴细胞的过程中,磷脂合成、甾醇合成和DNA合成依次增加。细胞进入有丝分裂的速率与伴刀豆球蛋白A浓度成正比。高浓度的伴刀豆球蛋白A在G1期的承诺后点阻止细胞生长。增强的磷脂合成是一个承诺前事件。增强的甾醇合成是一个承诺后事件,反映了细胞生长通过G1期时对增加胆固醇供应的需求。

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