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Id1通过提高Deltex1的表达来减弱Notch信号传导并损害T细胞定向分化。

Id1 attenuates Notch signaling and impairs T-cell commitment by elevating Deltex1 expression.

作者信息

Wang Hong-Cheng, Perry S Scott, Sun Xiao-Hong

机构信息

Immunobiology and Cancer Research Program, Oklahoma Medical Research Foundation, Oklahoma City, Oklahoma 73104, USA.

出版信息

Mol Cell Biol. 2009 Sep;29(17):4640-52. doi: 10.1128/MCB.00119-09. Epub 2009 Jun 29.

Abstract

Complete inhibition of E protein transcription factors by Id1 blocks the developmental transition of CD4/CD8 double-negative 1 (DN1; CD44(+) CD25(-)) thymocytes to the DN2 (CD44(+) CD25(+)) stage. To understand the underlying mechanisms, we observed that mRNA levels of Deltex1, as well as Deltex4, were dramatically elevated in Id1-expressing thymocytes, which could result in developmental arrest by attenuating Notch function. In support of this hypothesis, we found that Deltex1 ablation enabled Id1-expressing progenitors to differentiate to the DN3 (CD44(-) CD25(+)) stage, which was accompanied by enhanced Notch1 expression in T-cell progenitors. Consistently, constitutive activation of Notch1 drove the differentiation of Id1-expressing progenitors to the DN3 stage. Furthermore, we showed that Gfi1b levels decreased, whereas GATA3 levels increased in Id1 transgenic thymocytes. When overexpressed, GATA3 was able to upregulate Deltex1 transcription. Thus, T-cell commitment may be controlled by the interplay among E proteins, Gfi1b, and GATA3 transcription regulators, which influence Notch function through the expression of Deltex1.

摘要

Id1对E蛋白转录因子的完全抑制作用会阻断CD4/CD8双阴性1(DN1;CD44(+) CD25(-))胸腺细胞向DN2(CD44(+) CD25(+))阶段的发育转变。为了解其潜在机制,我们观察到在表达Id1的胸腺细胞中,Deltex1以及Deltex4的mRNA水平显著升高,这可能通过减弱Notch功能导致发育停滞。为支持这一假设,我们发现敲除Deltex1能使表达Id1的祖细胞分化至DN3(CD44(-) CD25(+))阶段,同时T细胞祖细胞中的Notch1表达增强。一致地,Notch1的组成性激活促使表达Id1的祖细胞分化至DN3阶段。此外,我们发现Id1转基因胸腺细胞中Gfi1b水平降低,而GATA3水平升高。当GATA3过表达时,它能够上调Deltex1转录。因此,T细胞定向分化可能受E蛋白、Gfi1b和GATA3转录调节因子之间的相互作用控制,这些因子通过Deltex1的表达影响Notch功能。

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