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AML1, the target of multiple chromosomal translocations in human leukemia, is essential for normal fetal liver hematopoiesis.AML1是人类白血病中多种染色体易位的靶点,对正常胎儿肝脏造血至关重要。
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C/EBP、c-Myb和PU.1协同调节中性粒细胞弹性蛋白酶启动子。

C/EBP, c-Myb, and PU.1 cooperate to regulate the neutrophil elastase promoter.

作者信息

Oelgeschläger M, Nuchprayoon I, Lüscher B, Friedman A D

机构信息

Institut für Molekularbiologie, Medizinische Hochschule Hannover, Germany.

出版信息

Mol Cell Biol. 1996 Sep;16(9):4717-25. doi: 10.1128/MCB.16.9.4717.

DOI:10.1128/MCB.16.9.4717
PMID:8756629
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC231472/
Abstract

The murine neutrophil elastase (NE) gene is expressed specifically in immature myeloid cells. A 91-bp NE promoter region contains three cis elements which are conserved evolutionarily and are essential for activation of the promoter in differentiating 32D cl3 myeloid cells. These elements bound c-Myb (at -49), C/EBPalpha (at -57), and PU.1 (at -82). In NIH 3T3 cells, the NE promoter was activated by c-Myb, C/EBPalpha, and PU.1, via their respective binding sites. Cooperative activation was seen by any combination of c-Myb, C/EBPalpha, and PU.1, including all three together, again via their DNA-binding sites. In CV-1 cells, but not in NIH 3T3 cells, cooperation between Myb and C/EBPalpha depended on the integrity of the PU.1-binding site. In addition to C/EBPalpha, C/EBPdelta strongly activated the NE promoter, alone or with c-Myb, but C/EBPbeta was less active. Either of C/EBPalpha's two transactivation domains cooperatively activated the promoter with c-Myb, in both NIH 3T3 and 32D c13 cells. Synergistic binding to DNA in a gel shift assay between C/EBPalpha, c-Myb, and PU.1 could not be demonstrated. Also, separation of the C/EBP- and c-Myb-binding sites by 5 or 10 bp did not prevent cooperativity. These results suggest that a coactivator protein mediates cooperative activation of the NE promoter by a C/EBP and c-Myb. These factors, together with PU.1, direct restricted expression of the NE promoter to immature myeloid cells.

摘要

小鼠中性粒细胞弹性蛋白酶(NE)基因在未成熟髓样细胞中特异性表达。一个91bp的NE启动子区域包含三个顺式元件,这些元件在进化上保守,并且对于在分化的32D cl3髓样细胞中激活启动子至关重要。这些元件结合c-Myb(位于-49)、C/EBPα(位于-57)和PU.1(位于-82)。在NIH 3T3细胞中,NE启动子通过c-Myb、C/EBPα和PU.1经由它们各自的结合位点被激活。c-Myb、C/EBPα和PU.1的任何组合,包括三者一起,再次经由它们的DNA结合位点,都能观察到协同激活。在CV-1细胞中,但不在NIH 3T3细胞中,Myb和C/EBPα之间的协同作用依赖于PU.1结合位点的完整性。除了C/EBPα,C/EBPδ单独或与c-Myb一起强烈激活NE启动子,但C/EBPβ活性较低。在NIH 3T3和32D c13细胞中,C/EBPα的两个反式激活结构域中的任何一个都能与c-Myb协同激活启动子。在凝胶迁移试验中,无法证明C/EBPα、c-Myb和PU.1之间对DNA的协同结合。此外,C/EBP和c-Myb结合位点之间相隔5或10bp并不妨碍协同作用。这些结果表明,一种共激活蛋白介导了C/EBP和c-Myb对NE启动子的协同激活。这些因子与PU.1一起,将NE启动子的表达定向限制于未成熟髓样细胞。