Division of Biology, California Institute of Technology, MC 139-74, Pasadena, CA 91125 USA.
Dev Biol. 2013 Oct 15;382(2):567-75. doi: 10.1016/j.ydbio.2013.08.009. Epub 2013 Aug 19.
Neural crest cells form diverse derivatives that vary according to their level of origin along the body axis, with only cranial neural crest cells contributing to facial skeleton. Interestingly, the transcription factor Ets-1 is uniquely expressed in cranial but not trunk neural crest, where it functions as a direct input into neural crest specifier genes, Sox10 and FoxD3. We have isolated and interrogated a cis-regulatory element, conserved between birds and mammals, that drives reporter expression in a manner that recapitulates that of endogenous Ets-1 expression in the neural crest. Within a minimal Ets-1 enhancer region, mutation of putative binding sites for SoxE, homeobox, Ets, TFAP2 or Fox proteins results in loss or reduction of neural crest enhancer activity. Morpholino-mediated loss-of-function experiments show that Sox9, Pax7, Msx1/2, Ets-1, TFAP2A and FoxD3, all are required for enhancer activity. In contrast, mutation of a putative cMyc/E-box sequence augments reporter expression, consistent with this being a repressor binding site. Taken together, these results uncover new inputs into Ets-1, revealing critical links in the cranial neural crest gene regulatory network.
神经嵴细胞形成多种衍生物,其来源沿着身体轴而异,只有颅神经嵴细胞有助于面部骨骼的形成。有趣的是,转录因子 Ets-1 仅在颅神经嵴中特异性表达,而不在躯干神经嵴中表达,在那里它作为神经嵴特化基因 Sox10 和 FoxD3 的直接输入发挥作用。我们已经分离并研究了一个顺式调控元件,它在鸟类和哺乳动物之间保守,以类似于内源性 Ets-1 在神经嵴中的表达的方式驱动报告基因的表达。在最小的 Ets-1 增强子区域内,对 SoxE、同源盒、Ets、TFAP2 或 Fox 蛋白的假定结合位点进行突变会导致神经嵴增强子活性的丧失或减少。基于 morpholino 的功能丧失实验表明 Sox9、Pax7、Msx1/2、Ets-1、TFAP2A 和 FoxD3 均对增强子活性是必需的。相比之下,假定的 cMyc/E 盒序列的突变增强了报告基因的表达,这与该序列是一个阻遏物结合位点一致。总之,这些结果揭示了 Ets-1 的新输入,揭示了颅神经嵴基因调控网络中的关键联系。
