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[人卵巢癌细胞系中CA125的产生:与细胞周期的关系]

[Production of CA125 in cell lines derived from human ovarian carcinoma: in relation to the cell cycle].

作者信息

Suzuki M, Ma J, Usui N, Furugen Y, Takada M

机构信息

Department of Obstetrics and Gynecology, Juntendo University School of Medicine, Tokyo.

出版信息

Nihon Sanka Fujinka Gakkai Zasshi. 1992 Jun;44(6):710-6.

PMID:1506733
Abstract

The association of the production of CA125 with the cell cycle was investigated in two cell lines derived from human ovarian cancer, one from a serous cystadenocarcinoma (HTOA) and the other from a mucinous cystadenocarcinoma (RMUG-s). HTOA and RMUG-s cells secreted CA125 at about 50 and 30U/ml/10(5) cell/24hr, respectively, in the logarithmic growth phase and at about 75 and 100U/ml/10(5) cell/24hr in the steady phase. Analysis by FCM revealed that cultures of both cell lines cultured for 7 days contained more cells in the G0/G1 phase and less cells in the S phase than those cultured for 3 days. The positive rate of immunologically stained DNA polymerase alpha was 31% in HTOA cells and 39% in RMUG-s cells after cultivation of the cells for 3 days. The addition of EGF at 0.01, 0.1 or 1.0nM did not affect the production of CA125 in HTOA or RMUG-s cells while the addition of NaBT at 1, 3 and 5mM raised production in both cell lines as the dose rose. With RMUG-s cells, the addition of EGF at 0.01nM to the culture media accelerated both logarithmic and steady phase growth without a significant change in the production of CA125. In contrast, the addition of NaBT at 1mM suppressed growth, but tended to increase the production of CA125 per cell. With the effect of EGF on the cell cycle of both cell lines, cells in the S phase increased by about 20% as compared with the control, 48 hours after its addition at 0.01nM. In contrast, after cultivation for 48 hours in the presence of 1mM NaBT, cells in the S phase were decreased while those in the G0/G1 phase increased. The results presented above suggested the possibility that some factors other than the cell cycle were involved in the production of CA125. There also is close correlation between cells in the G0/G1 phase and the production of CA125 in the culture of human ovarian cancer cells.

摘要

在源自人卵巢癌的两种细胞系中研究了CA125产生与细胞周期的关联,一种来自浆液性囊腺癌(HTOA),另一种来自黏液性囊腺癌(RMUG-s)。HTOA和RMUG-s细胞在对数生长期分别以约50和30U/ml/10⁵细胞/24小时的速率分泌CA125,在稳定期分别以约75和100U/ml/10⁵细胞/24小时的速率分泌。流式细胞术分析显示,两种细胞系培养7天的培养物中处于G0/G1期的细胞比培养3天的更多,处于S期的细胞更少。细胞培养3天后,HTOA细胞中免疫染色的DNA聚合酶α阳性率为31%,RMUG-s细胞中为39%。添加0.01、0.1或1.0nM的表皮生长因子(EGF)对HTOA或RMUG-s细胞中CA125的产生没有影响,而添加1、3和5mM的丁酸钠(NaBT)则随着剂量增加使两种细胞系中的产量提高。对于RMUG-s细胞,向培养基中添加0.01nM的EGF可加速对数期和稳定期生长,而CA125的产生没有显著变化。相反,添加1mM的NaBT会抑制生长,但倾向于增加每个细胞的CA125产量。关于EGF对两种细胞系细胞周期的影响,在添加0.01nM的EGF 48小时后,与对照相比,处于S期的细胞增加了约20%。相反,在1mM NaBT存在下培养48小时后,处于S期的细胞减少,而处于G0/G1期的细胞增加。上述结果表明,除细胞周期外的一些因素可能参与了CA125的产生。在人卵巢癌细胞培养中,G0/G1期的细胞与CA125的产生之间也存在密切相关性。

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