Alma Mater Studiorum, Dipartimento di Patologia Sperimentale, Via S, Giacomo 14, 40126 Bologna, Italy.
BMC Biol. 2010 Apr 7;8:33. doi: 10.1186/1741-7007-8-33.
Neoplastic overgrowth depends on the cooperation of several mutations ultimately leading to major rearrangements in cellular behaviour. Precancerous cells are often removed by cell death from normal tissues in the early steps of the tumourigenic process, but the molecules responsible for such a fundamental safeguard process remain in part elusive. With the aim to investigate the molecular crosstalk occurring between precancerous and normal cells in vivo, we took advantage of the clonal analysis methods that are available in Drosophila for studying the phenotypes due to lethal giant larvae (lgl) neoplastic mutation induced in different backgrounds and tissues.
We observed that lgl mutant cells growing in wild-type imaginal wing discs show poor viability and are eliminated by Jun N-terminal Kinase (JNK)-dependent cell death. Furthermore, they express very low levels of dMyc oncoprotein compared with those found in the surrounding normal tissue. Evidence that this is a cause of lgl mutant cells elimination was obtained by increasing dMyc levels in lgl mutant clones: their overgrowth potential was indeed re-established, with mutant cells overwhelming the neighbouring tissue and forming tumourous masses displaying several cancer hallmarks. Moreover, when lgl mutant clones were induced in backgrounds of slow-dividing cells, they upregulated dMyc, lost apical-basal cell polarity and were able to overgrow. Those phenotypes were abolished by reducing dMyc levels in the mutant clones, thereby confirming its key role in lgl-induced tumourigenesis. Furthermore, we show that the eiger-dependent Intrinsic Tumour Suppressor pathway plays only a minor role in eliminating lgl mutant cells in the wing pouch; lgl-/- clonal death in this region is instead driven mainly by dMyc-induced Cell Competition.
Our results provide the first evidence that dMyc oncoprotein is required in lgl tumour suppressor mutant tissue to promote invasive overgrowth in larval and adult epithelial tissues. Moreover, we show that dMyc abundance inside versus outside the mutant clones plays a key role in driving neoplastic overgrowth.
肿瘤的过度生长依赖于几种突变的协同作用,最终导致细胞行为的重大重排。在肿瘤发生过程的早期,癌变前细胞通常通过细胞死亡从正常组织中被清除,但负责这一基本保护过程的分子在一定程度上仍难以捉摸。为了研究体内癌变前细胞与正常细胞之间发生的分子串扰,我们利用克隆分析方法,在不同背景和组织中研究由于致死性巨幼虫 (lgl) 肿瘤突变引起的表型,该方法可用于研究果蝇中的表型。
我们观察到,在野生型 imaginal 翅膀盘中生长的 lgl 突变细胞活力差,并通过 Jun N-末端激酶 (JNK) 依赖性细胞死亡而被消除。此外,与周围正常组织相比,它们表达的 dMyc 癌蛋白水平非常低。通过增加 lgl 突变克隆中的 dMyc 水平获得了这是消除 lgl 突变细胞的原因的证据:它们的过度生长潜力确实得到了重建,突变细胞压倒了邻近组织并形成了显示出多种癌症特征的肿瘤团块。此外,当 lgl 突变克隆在增殖缓慢的细胞背景中诱导时,它们上调了 dMyc,失去了顶端-基底细胞极性,并能够过度生长。通过降低突变克隆中的 dMyc 水平,可以消除这些表型,从而证实其在 lgl 诱导的肿瘤发生中的关键作用。此外,我们表明 eiger 依赖性内在肿瘤抑制途径在翅膀囊中仅在消除 lgl 突变细胞中起次要作用;该区域中 lgl-/- 克隆死亡主要由 dMyc 诱导的细胞竞争驱动。
我们的研究结果首次证明 dMyc 癌蛋白在 lgl 肿瘤抑制突变组织中是促进幼虫和成年上皮组织侵袭性过度生长所必需的。此外,我们表明突变克隆内外的 dMyc 丰度在驱动肿瘤过度生长方面起着关键作用。
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