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孕酮和甲羟孕酮在体外对成纤维细胞的生长抑制作用。

Growth inhibition of fibroblasts by progesterone and medroxyprogesterone in vitro.

作者信息

Comini Andrada E, Hoschoian J C, Anton E, Lanari A

出版信息

Int Arch Allergy Appl Immunol. 1985;76(2):97-100. doi: 10.1159/000233673.

DOI:10.1159/000233673
PMID:3967946
Abstract

This study was carried out to evaluate in vitro the beneficial effects observed in various aggressive fibromatoses (mediastinal, retroperitoneal, paraneoplastic fibrosis and desmoid tumors) after treatment with progesterone. Primary cultures of fibroblasts were prepared from fetuses of Swiss strain mice. Continuous fibroblast lines LM and Vero were also used. Moreover, cultures of non-fetal human fibroblast from skin and lung were employed. Epithelial tumor cell line HeLa was used as a control. All cultures were incubated with various doses of progesterone at concentrations from 1.4 X 10(-4) to 1.4 X 10(-3) M. Human cells and monolayers of fetal murine fibroblast were submitted to the action of medroxyprogesterone solution at the same concentrations as used for progesterone. Other steroids (estrone, estriol, testosterone and prednisolone) were used at the identical concentrations in the same vehicles. Progesterone affected all lines of fibroblasts studied and destroyed them within either 2-4 or 24-48 h depending on the steroid concentrations used. Medroxyprogesterone had a comparable effect on human cell lines and monolayers of fetal murine fibroblasts provided that the same ratio between the hormone concentration and the time of exposure was maintained. With higher medium concentrations shorter times of incubation were required for the destruction of fibroblast. However, to observe a degree of lysis similar to that elicited by progesterone, it was necessary to use 4 times higher concentrations of medroxyprogesterone. No effect on HeLa epithelial cells was observed nor were the controls affected by the steroids or diluents used at the appropriate concentrations. Results from incubation studies using monolayers of murine fibroblast and 14C-progesterone suggested that the cells were destroyed by the progesterone and not by a bioproduct of its metabolism.

摘要

本研究旨在体外评估孕酮治疗各种侵袭性纤维瘤病(纵隔、腹膜后、副肿瘤性纤维化和硬纤维瘤)后观察到的有益效果。从瑞士品系小鼠胎儿制备成纤维细胞原代培养物。还使用了连续的成纤维细胞系LM和Vero。此外,采用了来自皮肤和肺的非胎儿人成纤维细胞培养物。上皮肿瘤细胞系HeLa用作对照。所有培养物均用浓度为1.4×10⁻⁴至1.4×10⁻³M的各种剂量孕酮孵育。人细胞和胎儿鼠成纤维细胞单层用与孕酮相同浓度的甲羟孕酮溶液处理。其他类固醇(雌酮、雌三醇、睾酮和泼尼松龙)在相同载体中以相同浓度使用。孕酮对所研究的所有成纤维细胞系均有影响,并根据所用类固醇浓度在2 - 4小时或24 - 48小时内将其破坏。只要保持激素浓度与暴露时间之间的相同比例,甲羟孕酮对人细胞系和胎儿鼠成纤维细胞单层有类似作用。培养基浓度越高,破坏成纤维细胞所需的孵育时间越短。然而,为了观察到与孕酮引起的类似程度的裂解,需要使用高4倍浓度的甲羟孕酮。未观察到对HeLa上皮细胞有影响,适当浓度的类固醇或稀释剂对对照组也无影响。使用鼠成纤维细胞单层和¹⁴C - 孕酮的孵育研究结果表明,细胞是被孕酮破坏的,而不是其代谢生物产物。

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