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一种用于细胞运动性和增殖的新型体外测定法。

A new in vitro assay for cell motility and proliferation.

作者信息

Benestad H B, Saxholm H J, Siebke E M

出版信息

Cell Tissue Kinet. 1987 Jan;20(1):109-19. doi: 10.1111/j.1365-2184.1987.tb01087.x.

Abstract

We have described and characterized a new micropore membrane assay for migration and proliferation of cells of various tumourigenic potential. The assay was developed to facilitate analysis of some aspects of cancer invasion and metastasis. Tumorigenic and non-tumorigenic C3H/10 T 1/2 cells grow in and migrate out of a culture chamber during a 1-11 day period, the shorter periods are used for chambers with 6 micron thick polycarbonate membranes, the longer ones for 140 micron thick cellulose nitrate membranes. Cell growth within the chambers, in their micropore membranes and on the outside of the membranes, was assessed with microscopy, electronic cell counting, flow cytometry of propidium iodide (PI) stained cells, and 3H-thymidine [( 3H]TdR) incorporation. A complete retrieval of intact cells that have traversed the membraneous chamber wall is possible, and these cells can be recultured or used in other studies. The tumorigenic cells had a steeper growth curve in vitro than the non transformed cells, but the relative sizes of the emigrated subpopulations were not significantly different. The subpopulation of tumorigenic cells that emigrated spontaneously from the chambers was less able than the subpopulation retained to populate secondary chamber cultures, suggesting that the clonogenic (stem) tumour cells are 'slow movers'.

摘要

我们已经描述并表征了一种用于分析具有不同致瘤潜力的细胞迁移和增殖的新型微孔膜测定法。开发该测定法是为了便于分析癌症侵袭和转移的某些方面。致瘤性和非致瘤性C3H/10 T 1/2细胞在1 - 11天内生长并从培养室迁移出来,较短的时间用于配备6微米厚聚碳酸酯膜的培养室,较长的时间用于配备140微米厚硝酸纤维素膜的培养室。通过显微镜检查、电子细胞计数、碘化丙啶(PI)染色细胞的流式细胞术以及3H - 胸腺嘧啶核苷[(3H]TdR)掺入来评估培养室内、微孔膜内以及膜外的细胞生长情况。有可能完整回收穿过膜质室壁的细胞,并且这些细胞可以重新培养或用于其他研究。致瘤细胞在体外的生长曲线比未转化细胞更陡峭,但迁出亚群的相对大小没有显著差异。从培养室中自发迁出的致瘤细胞亚群比保留下来的亚群在接种次级培养室时的能力更弱,这表明克隆性(干细胞)肿瘤细胞是“迁移缓慢者”。

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