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胸膜炎性渗出物诱导培养的大鼠腹膜巨噬细胞中的DNA合成。

Induction of DNA synthesis in rat peritoneal macrophages in culture by a pleural inflammatory exudate.

作者信息

Adolphe M, Fontagné J, Pelletier M, Giroud J P, Timsit J, Lechat P

出版信息

Agents Actions. 1976 Feb;6(1-3):114-22. doi: 10.1007/BF01972194.

Abstract

Peritoneal macrophages in culture are blocked in the G0 phase of the cell cycle, but retain many of their functional characteristics such as phagocytic ability. Peritoneal macrophages have been thought to be a terminal cell type. It has been investigated whether such properties could be modified by a substance released in acute inflammatory exudates. For this purpose a pleural exudate obtained from rats injected with dextran (40,000) 4 hours before, was centrifuged to eliminate cells, sterilized by filtration on Millipore filter 0.22 mum and diluted 50% with 199 medium culture. This medium was used to treat normal and activated peritoneal macrophages in culture. The effects were observed 24, 48, 72, 96 hours after the beginning of treatment. An enhancement of spreading and capacity of phagocytosis was observed 24 hours after the beginning of treatment. After 48 hours, the number of cells incorporating tritiated thymidine increased and became highest 4 days later. These phenomena were also obtained with pleural exudate of inbred rats (Lewis, Wag) treating macrophages of the same strain and with rat pleural exudate treating mouse macrophages. No effects were observed with dextran alone. The chemical nature of the stimulatory factor remains to be elucidated.

摘要

培养中的腹膜巨噬细胞停滞于细胞周期的G0期,但仍保留许多功能特性,如吞噬能力。腹膜巨噬细胞一直被认为是一种终末细胞类型。人们研究了急性炎症渗出物中释放的一种物质是否能改变这些特性。为此,将4小时前注射右旋糖酐(40,000)的大鼠的胸腔渗出液离心以去除细胞,通过0.22μm的微孔滤膜过滤灭菌,并用199培养基培养液稀释50%。该培养基用于处理培养中的正常和活化腹膜巨噬细胞。在处理开始后的24、48、72、96小时观察效果。处理开始24小时后观察到铺展和吞噬能力增强。48小时后,掺入氚标记胸腺嘧啶核苷的细胞数量增加,并在4天后达到最高。用近交系大鼠(刘易斯、瓦格)的胸腔渗出液处理同品系的巨噬细胞以及用大鼠胸腔渗出液处理小鼠巨噬细胞也得到了这些现象。单独使用右旋糖酐未观察到效果。刺激因子的化学性质仍有待阐明。

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