Runx1:神经纤维生成的新驱动因子

Jianqiang Wu, Gang Huang, N. Ratner
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These modifications control various aspects of transcriptional factors' activities such as auto inhibition, dimerization and ubiquitin-mediated degradation [3]. \n \nBesides its developmental determination role, RUNX1 is involved in malignant tumor formation. Reports have shown that RUNX1 is frequently de-regulated and has paradoxical effects in human cancers, in which it can function either as a tumor suppressor or oncogene [3, 4]. RUNX1 has been implicated as a tumor suppressor in several solid tumors including breast cancer, esophageal adenocarcinoma, colon cancer and possibly prostate cancer but acts as an oncogene in head/neck squamous cell carcinomas, endometrial cancer, and epithelial cancer [3, 4]. Because Runx1 is a sequence specific DNA-binding transcription factor, whether it functions as oncogene or tumor suppressor is dependent on its interaction with specific co-regulatory proteins. \n \nWe recently showed that RUNX1 acts as an oncogene in the context of loss of neurofibromatosis type 1 (Nf1). Instead of chromosomal translocation and mutation frequently detected in other cancers, Runx1 is overexpressed in human and mouse neurofibroma-initiating cells, both at the messenger RNA and protein levels. Specifically, loss of Nf1 increases number of embryonic day 12.5 Runx1+/Blbp+ Schwann cell progenitors that enable neurofibroma formation in a mouse model (Figure ​(Figure1).1). Targeted genetic deletion of RUNX1 in Schwann cells and Schwann cell progenitors delays mouse neurofibroma formation in vivo (5). \n \n \n \nFigure 1 \n \nModel of neurofibromagenesis \n \n \n \nIt is not clear how loss of Nf1 induces Runx1 overexpression and serves as an oncogene. There are several potential possibilities: 1) NF1 is known to encode a Ras-GTPase activating protein (Ras-GAP) and the Ras-MEK-ERK pathway is important for Nf1 neurofibroma formation [6]. Runx1 may be phosphorylated by the elevated MEK signaling to initiate the tumor formation process. 2) Elevated Wnt or Notch signaling can directly or indirectly activate Runx1, which can accelerate G1-S transition and stimulates cell proliferation. Consistently, our results show that loss of Runx1 in Schwann cells decreased cell proliferation by activating Trp53-p21 or increased cell apoptosis by inhibiting anti-apoptotic gene Bcl-2 in the context of Nf1−/− Schwann cell environment. It is possible that the elevated Runx1 within the neurofibroma cell alters cell fate (i.e. proliferation or differentiation) through Trp53-p21. Further experiments are needed to determine how p21 and Trp53 were activated or Bcl-2 was inactivated in the Runx1fl/fl;Nf1fl/fl; Dhhre tumors. 3) Runx1 might interact with epigenetic regulators such as the chromatin remodeling complexes, SWI/SNF, or polycomb repressive complexes to affect Runx1 activity by post-translational modification [7]. \n \nOverall, our study supports an oncogenic role of Runx1 in neurofibroma initiation and/or maintenance, but the underlying mechanism(s) are not clear. 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引用次数: 3

摘要

runt相关转录因子-1 (RUNX1或AML1)编码一种转录因子,作为主要的发育调节因子。它对造血、血管生成、巨核细胞成熟以及T细胞和B细胞分化具有重要作用[1]。Runx1在神经元发育和胶质细胞分化中也很重要[2]。Runx1被整合到一个复杂的调控网络中,该网络在转录和转录后水平上都起作用。Runx1的活性可以通过多种翻译后修饰来调节,包括磷酸化、去磷酸化、SUMOylation、乙酰化、甲基化和泛素化。这些修饰控制转录因子活性的各个方面,如自抑制、二聚化和泛素介导的降解[3]。RUNX1除了具有发育决定作用外,还参与恶性肿瘤的形成。有报道表明,RUNX1经常被去调控,并在人类癌症中具有矛盾的作用,在这种作用中,它既可以作为肿瘤抑制因子,也可以作为致癌基因[3,4]。RUNX1在包括乳腺癌、食管癌、结肠癌和可能的前列腺癌在内的几种实体肿瘤中被认为是肿瘤抑制因子,但在头颈部鳞状细胞癌、子宫内膜癌和上皮癌中作为癌基因[3,4]。由于Runx1是一种序列特异性的dna结合转录因子,所以它是作为致癌基因还是肿瘤抑制因子,取决于它与特异性共调控蛋白的相互作用。我们最近发现RUNX1在1型神经纤维瘤病(Nf1)缺失的情况下作为致癌基因。与在其他癌症中经常检测到的染色体易位和突变不同,Runx1在人和小鼠神经纤维瘤起始细胞中在信使RNA和蛋白质水平上都过表达。具体来说,Nf1的缺失增加了小鼠模型中能够形成神经纤维瘤的Runx1+/Blbp+雪旺细胞祖细胞的胚胎天数12.5天(图1)。雪旺细胞和雪旺细胞祖细胞中RUNX1基因的靶向缺失延缓了小鼠体内神经纤维瘤的形成(5)。图1神经纤维增生模型。目前尚不清楚Nf1缺失如何诱导RUNX1过表达并作为致癌基因。有几种潜在的可能性:1)已知NF1编码Ras-GTPase激活蛋白(Ras-GAP), Ras-MEK-ERK通路对NF1神经纤维瘤的形成很重要[6]。Runx1可能通过MEK信号的升高而磷酸化,从而启动肿瘤的形成过程。2) Wnt或Notch信号升高可直接或间接激活Runx1,加速G1-S转变,刺激细胞增殖。同样,我们的研究结果表明,在Nf1−/−雪旺细胞环境下,Runx1在雪旺细胞中的缺失通过激活Trp53-p21来降低细胞增殖,或者通过抑制抗凋亡基因Bcl-2来增加细胞凋亡。神经纤维瘤细胞内Runx1的升高可能通过Trp53-p21改变细胞命运(即增殖或分化)。需要进一步的实验来确定Runx1fl/fl、Nf1fl/fl、Bcl-2如何被激活或失活。Dhhre肿瘤。3) Runx1可能与染色质重塑复合体、SWI/SNF或多梳抑制复合体等表观遗传调控因子相互作用,通过翻译后修饰影响Runx1活性[7]。总的来说,我们的研究支持Runx1在神经纤维瘤发生和/或维持中的致癌作用,但其潜在机制尚不清楚。随着对RUNX1生物学认识的不断增加,靶向转录因子RUNX1或RUNX1通路可能为神经纤维瘤及其他RUNX1过表达肿瘤提供新的治疗方法。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Runx1: a new driver in neurofibromagenesis
The Runt-related transcription factor-1 (RUNX1 or AML1) encodes a transcription factor that serves as a master developmental regulator. It is important for hematopoiesis, angiogenesis, maturation of megakaryocytes, and differentiation of T and B cells [1]. Runx1 is also important for neuronal development and glial cell differentiation [2]. Runx1 is integrated into a complex regulatory network which acts both at the transcriptional and post-transcriptional levels. Runx1 activity can be regulated by several posttranslational modifications, including phosphorylation, de-phosphorylation, SUMOylation, acetylation, methylation and ubiquitination. These modifications control various aspects of transcriptional factors' activities such as auto inhibition, dimerization and ubiquitin-mediated degradation [3]. Besides its developmental determination role, RUNX1 is involved in malignant tumor formation. Reports have shown that RUNX1 is frequently de-regulated and has paradoxical effects in human cancers, in which it can function either as a tumor suppressor or oncogene [3, 4]. RUNX1 has been implicated as a tumor suppressor in several solid tumors including breast cancer, esophageal adenocarcinoma, colon cancer and possibly prostate cancer but acts as an oncogene in head/neck squamous cell carcinomas, endometrial cancer, and epithelial cancer [3, 4]. Because Runx1 is a sequence specific DNA-binding transcription factor, whether it functions as oncogene or tumor suppressor is dependent on its interaction with specific co-regulatory proteins. We recently showed that RUNX1 acts as an oncogene in the context of loss of neurofibromatosis type 1 (Nf1). Instead of chromosomal translocation and mutation frequently detected in other cancers, Runx1 is overexpressed in human and mouse neurofibroma-initiating cells, both at the messenger RNA and protein levels. Specifically, loss of Nf1 increases number of embryonic day 12.5 Runx1+/Blbp+ Schwann cell progenitors that enable neurofibroma formation in a mouse model (Figure ​(Figure1).1). Targeted genetic deletion of RUNX1 in Schwann cells and Schwann cell progenitors delays mouse neurofibroma formation in vivo (5). Figure 1 Model of neurofibromagenesis It is not clear how loss of Nf1 induces Runx1 overexpression and serves as an oncogene. There are several potential possibilities: 1) NF1 is known to encode a Ras-GTPase activating protein (Ras-GAP) and the Ras-MEK-ERK pathway is important for Nf1 neurofibroma formation [6]. Runx1 may be phosphorylated by the elevated MEK signaling to initiate the tumor formation process. 2) Elevated Wnt or Notch signaling can directly or indirectly activate Runx1, which can accelerate G1-S transition and stimulates cell proliferation. Consistently, our results show that loss of Runx1 in Schwann cells decreased cell proliferation by activating Trp53-p21 or increased cell apoptosis by inhibiting anti-apoptotic gene Bcl-2 in the context of Nf1−/− Schwann cell environment. It is possible that the elevated Runx1 within the neurofibroma cell alters cell fate (i.e. proliferation or differentiation) through Trp53-p21. Further experiments are needed to determine how p21 and Trp53 were activated or Bcl-2 was inactivated in the Runx1fl/fl;Nf1fl/fl; Dhhre tumors. 3) Runx1 might interact with epigenetic regulators such as the chromatin remodeling complexes, SWI/SNF, or polycomb repressive complexes to affect Runx1 activity by post-translational modification [7]. Overall, our study supports an oncogenic role of Runx1 in neurofibroma initiation and/or maintenance, but the underlying mechanism(s) are not clear. With increasing knowledge of RUNX1 biology, targeting the transcription factor RUNX1 or RUNX1 pathway might provide a novel therapy for neurofibroma as well as other tumors which overexpress RUNX1.
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