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在 lin-12/Notch 依赖性细胞命运特化过程中,lag-1/CSL 中的簇状 LAG-1 结合位点参与调节 lag-1 的表达。

Clustered LAG-1 binding sites in lag-1/CSL are involved in regulating lag-1 expression during lin-12/Notch-dependent cell-fate specification.

机构信息

Department of Molecular Bioscience, College of Biomedical Science, Kangwon National University, Chuncheon 200-701, Korea.

出版信息

BMB Rep. 2013 Apr;46(4):219-24. doi: 10.5483/bmbrep.2013.46.4.269.

Abstract

The cell-fate specification of the anchor cell (AC) and a ventral uterine precursor cell (VU) in Caenorhabditis elegans is initiated by a stochastic interaction between LIN-12/Notch receptor and LAG-2/Delta ligand in two neighboring Z1.ppp and Z4.aaa cells. Both cells express lin-12 and lag-2 before specification, and a small difference in LIN-12 activity leads to the exclusive expressions of lin-12 in VU and lag-2 in the AC, through a feedback mechanism of unknown nature. Here we show that the expression pattern of lag-1/CSL, a transcriptional repressor itself that turns into an activator upon binding of the intracellular domain of Notch, overlaps with that of lin-12. Site-directed mutagenesis of LAG-1 binding sites in lag-1 maintains its expression in the AC, and eliminates it in the VU. Thus, AC/VU cell-fate specification appears to involve direct regulation of lag-1 expression by the LAG-1 protein, activating its transcription in VU cells, but repressing it in the AC.

摘要

线虫中锚细胞 (AC) 和一个腹侧子宫前体细胞 (VU) 的命运决定,是由两个相邻的 Z1.ppp 和 Z4.aaa 细胞中 LIN-12/Notch 受体和 LAG-2/Delta 配体之间的随机相互作用启动的。在决定命运之前,这两个细胞都表达 lin-12 和 lag-2,而 LIN-12 活性的微小差异导致 VU 中 lin-12 的特异性表达和 AC 中 lag-2 的特异性表达,其通过未知性质的反馈机制实现。在这里,我们发现转录抑制因子 lag-1/CSL 的表达模式与其自身的配体 LAG-2 重叠,lag-1/CSL 是一种转录抑制因子,在结合 Notch 细胞内结构域后会转化为激活剂。通过对 lag-1 结合位点的定点突变,维持了其在 AC 中的表达,并消除了其在 VU 中的表达。因此,AC/VU 细胞命运的决定似乎涉及 LAG-1 蛋白对 lag-1 表达的直接调控,在 VU 细胞中激活其转录,而在 AC 中抑制其转录。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b7ad/4133882/17381baac9d3/BMB-46-219-g0001.jpg

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