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肿瘤抑制因子 Pten 的缺失促进了果蝇细胞在体外的增殖,并产生了连续的细胞系。

Loss of the tumor suppressor Pten promotes proliferation of Drosophila melanogaster cells in vitro and gives rise to continuous cell lines.

机构信息

Department of Molecular Genetics, Ohio State University, Columbus, Ohio, United States of America.

出版信息

PLoS One. 2012;7(2):e31417. doi: 10.1371/journal.pone.0031417. Epub 2012 Feb 21.

Abstract

In vivo analysis of Drosophila melanogaster has enhanced our understanding of many biological processes, notably the mechanisms of heredity and development. While in vivo analysis of mutants has been a strength of the field, analyzing fly cells in culture is valuable for cell biological, biochemical and whole genome approaches in which large numbers of homogeneous cells are required. An efficient genetic method to derive Drosophila cell lines using expression of an oncogenic form of Ras (Ras(V12)) has been developed. Mutations in tumor suppressors, which are known to cause cell hyperproliferation in vivo, could provide another method for generating Drosophila cell lines. Here we screened Drosophila tumor suppressor mutations to test if they promoted cell proliferation in vitro. We generated primary cultures and determined when patches of proliferating cells first emerged. These cells emerged on average at 37 days in wild-type cultures. Using this assay we found that a Pten mutation had a strong effect. Patches of proliferating cells appeared on average at 11 days and the cultures became confluent in about 3 weeks, which is similar to the timeframe for cultures expressing Ras(V12). Three Pten mutant cell lines were generated and these have now been cultured for between 250 and 630 cell doublings suggesting the life of the mutant cells is likely to be indefinite. We conclude that the use of Pten mutants is a powerful means to derive new Drosophila cell lines.

摘要

活体分析黑腹果蝇增强了我们对许多生物学过程的理解,特别是遗传和发育的机制。虽然对突变体的活体分析是该领域的优势,但分析培养的果蝇细胞对于细胞生物学、生物化学和全基因组方法是有价值的,因为这些方法需要大量同质细胞。已经开发了一种有效的遗传方法,通过表达致癌形式的 Ras(Ras(V12))来衍生果蝇细胞系。已知肿瘤抑制因子的突变会导致体内细胞过度增殖,这为生成果蝇细胞系提供了另一种方法。在这里,我们筛选了果蝇肿瘤抑制因子突变,以测试它们是否促进体外细胞增殖。我们生成了原代培养物,并确定了增殖细胞块首次出现的时间。在野生型培养物中,这些细胞平均在 37 天出现。使用该测定法,我们发现 Pten 突变具有很强的效果。增殖细胞块平均在 11 天出现,培养物在大约 3 周内达到汇合,这与表达 Ras(V12)的培养物的时间框架相似。生成了三个 Pten 突变细胞系,这些细胞系现在已经培养了 250 到 630 个细胞倍增,表明突变细胞的寿命可能是无限的。我们得出结论,使用 Pten 突变是衍生新的果蝇细胞系的有效手段。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8df1/3283623/eeae4fc76c62/pone.0031417.g001.jpg

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