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培养的人内皮细胞的葡萄糖毒性。复制延迟、细胞周期紊乱和加速死亡。

Glucose toxicity for human endothelial cells in culture. Delayed replication, disturbed cell cycle, and accelerated death.

作者信息

Lorenzi M, Cagliero E, Toledo S

出版信息

Diabetes. 1985 Jul;34(7):621-7. doi: 10.2337/diab.34.7.621.

DOI:10.2337/diab.34.7.621
PMID:3924693
Abstract

Functional and anatomical abnormalities of endothelium may represent a pathway to the increased vascular permeability and accelerated atherosclerosis characteristic of diabetes. To identify whether and how hyperglycemia may compromise the endothelial barrier, we have employed an in vitro system of human endothelial cells obtained from umbilical veins and cultured in elevated glucose concentrations (20 mM). Under these conditions, the achievement of saturation density was substantially delayed, with cell counts throughout most of the growth curve being 70-80% of control (P less than 0.002). More profound suppression of cell number was present in cultures exposed to 40 mM glucose. Similar, albeit slightly lesser, effects were observed in cultures exposed to 20 mM mannitol, mimicking the hypertonicity of the high glucose media. The effect of elevated glucose and mannitol was primarily mediated by a decrease in overall rate of replication of the endothelium as documented by the lower mitotic index (P less than 0.025). Analysis of the distribution of cells along phases of the cell cycle uncovered in the high glucose cultures a decreased proportion of cells in G0-G1 (70.5 +/- 5% versus 73.2 +/- 4% in controls, P less than 0.05) and an increased proportion of cells in S phase (16.5 +/- 2.7% versus 13.5 +/- 2.2% in controls, P less than 0.01), suggesting that the replicative delay is likely to occur between the phase of DNA synthesis and mitosis. Increased cellular death was specifically observed in the cultures exposed to elevated glucose concentrations (P less than 0.05), but it could account for only a minor portion of the deficit in cell number.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

内皮细胞的功能和解剖学异常可能是糖尿病所特有的血管通透性增加和动脉粥样硬化加速的一条途径。为了确定高血糖是否以及如何损害内皮屏障,我们采用了一种体外系统,该系统使用从脐静脉获得的人内皮细胞,并在高葡萄糖浓度(20 mM)下培养。在这些条件下,达到饱和密度的时间显著延迟,在大部分生长曲线期间细胞计数为对照的70 - 80%(P小于0.002)。在暴露于40 mM葡萄糖的培养物中,细胞数量受到更显著的抑制。在暴露于20 mM甘露醇的培养物中观察到类似但稍弱的效应,甘露醇模拟了高糖培养基的高渗性。高糖和甘露醇的作用主要是通过内皮细胞总体复制速率的降低介导的,这由较低的有丝分裂指数所证明(P小于0.025)。对细胞周期各阶段细胞分布的分析发现,在高糖培养物中,处于G0 - G1期的细胞比例降低(70.5±5%对对照组的73.2±4%,P小于0.05),处于S期的细胞比例增加(16.5±2.7%对对照组的13.5±2.2%,P小于0.01),这表明复制延迟可能发生在DNA合成期和有丝分裂期之间。在暴露于高葡萄糖浓度的培养物中特别观察到细胞死亡增加(P小于0.05),但它仅占细胞数量减少的一小部分。(摘要截短于250字)

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