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前列腺素E1对转化的和正常的WI-38成纤维细胞中环磷酸腺苷生成的长期刺激作用。

Prolonged prostaglandin E1 stimulation of cyclic AMP production in transformed and normal WI-38 fibroblasts.

作者信息

Chlapowski F J, Ray K P, Butcher R W

出版信息

In Vitro. 1978 Nov;14(11):924-34. doi: 10.1007/BF02616122.

Abstract

Long-term (48-hr) incubations of either the fibroblast strain WI-38 or its SV40-transformed counterpart, WI-38-VA13-2RA, in growth medium containing 1 micron prostaglandin E1 (PGE1) resulted in a sustained production and release of cyclic AMP from the cells into the medium. Despite the steady production, intracellular levels of the nucleotide decreased, reaching steady-state values within 4 hr of the initial exposure to PGE1. These values were maintained for the remainder of the 48-hr experimental period. The steady-state levels of intracellular cyclic AMP were higher than those observed in unstimulated cells, and cyclic AMP-dependent protein phosphokinase was in a highly activated state as compared to controls. Under these conditions little change in the growth or morphology of either the normal or transformed cells was observed. In contrast, inhibition of growth, apparent cell death, and unusual morphological changes were observed in both normal and transformed cells when high concentrations of either PGE1 (10 micron) or the phosphodiesterase inhibitor 1-methyl, 3-isobutylxanthine (0.5 mM to 2 mM) were used, which was indicative of toxic effects of the drugs. It was concluded that cyclic AMP-mediated activation of protein phosphokinase does not completely inhibit growth in WI-38 cells or restore normal growth and morphology to the SV40-transformed cells.

摘要

将成纤维细胞系WI - 38或其SV40转化的对应细胞系WI - 38 - VA13 - 2RA在含有1微摩尔前列腺素E1(PGE1)的生长培养基中进行长期(48小时)培养,结果导致细胞持续产生并向培养基中释放环磷酸腺苷(cAMP)。尽管cAMP持续产生,但细胞内核苷酸水平下降,在最初接触PGE1后4小时内达到稳态值。在48小时实验期的剩余时间内,这些值保持稳定。细胞内cAMP的稳态水平高于未受刺激的细胞,并且与对照相比,环磷酸腺苷依赖性蛋白磷酸激酶处于高度活化状态。在这些条件下,未观察到正常细胞或转化细胞的生长或形态有明显变化。相反,当使用高浓度的PGE1(10微摩尔)或磷酸二酯酶抑制剂1 - 甲基 - 3 - 异丁基黄嘌呤(0.5毫摩尔至2毫摩尔)时,在正常细胞和转化细胞中均观察到生长抑制、明显的细胞死亡和异常的形态变化,这表明药物具有毒性作用。得出的结论是,环磷酸腺苷介导的蛋白磷酸激酶激活并不能完全抑制WI - 38细胞的生长,也不能使SV40转化细胞恢复正常生长和形态。

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