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GLI1/GLI2 功能相互作用对于控制 Hedgehog/GLI 靶标基因表达是必需的。

GLI1/GLI2 functional interplay is required to control Hedgehog/GLI targets gene expression.

机构信息

Schulze Center for Novel Therapeutics, Division of Oncology Research, Mayo Clinic, Rochester, MN, U.S.A.

Department of Surgery, Koc University School of Medicine, Istanbul, Turkey.

出版信息

Biochem J. 2020 Sep 18;477(17):3131-3145. doi: 10.1042/BCJ20200335.

DOI:10.1042/BCJ20200335
PMID:32766732
Abstract

The Hedgehog-regulated transcription factors GLI1 and GLI2 play overlapping roles in development and disease; however, the mechanisms underlying their interplay remain elusive. We report for the first time that GLI1 and GLI2 physically and functionally interact in cancer cells. GLI1 and GLI2 were shown to co-immunoprecipitate in PANC1 pancreatic cancer cells and RMS13 rhabdomyosarcoma cells. Mapping analysis demonstrated that the zinc finger domains of both proteins are required for their heteromerization. RNAi knockdown of either GLI1 or GLI2 inhibited expression of many well-characterized GLI target genes (BCL2, MYCN, PTCH2, IL7 and CCND1) in PANC1 cells, whereas PTCH1 expression was only inhibited by GLI1 depletion. qPCR screening of a large set of putative canonical and non-canonical Hedgehog/GLI targets identified further genes (e.g. E2F1, BMP1, CDK2) strongly down-regulated by GLI1 and/or GLI2 depletion in PANC1 cells, and demonstrated that ANO1, AQP1 and SOCS1 are up-regulated by knockdown of either GLI1 or GLI2. Chromatin immunoprecipitation showed that GLI1 and GLI2 occupied the same regions at the BCL2, MYCN and CCND1 promoters. Furthermore, depletion of GLI1 inhibited GLI2 occupancy at these promoters, suggesting that GLI1/GLI2 interaction is required for the recruitment of GLI2 to these sites. Together, these findings indicate that GLI1 and GLI2 co-ordinately regulate the transcription of some genes, and provide mechanistic insight into the roles of GLI proteins in carcinogenesis.

摘要

刺猬调节转录因子 GLI1 和 GLI2 在发育和疾病中发挥重叠作用;然而,它们相互作用的机制仍然难以捉摸。我们首次报道 GLI1 和 GLI2 在癌细胞中物理和功能相互作用。在 PANC1 胰腺癌细胞和 RMS13 横纹肌肉瘤细胞中显示 GLI1 和 GLI2 共免疫沉淀。映射分析表明,两种蛋白质的锌指结构域都需要它们的异二聚化。在 PANC1 细胞中,RNAi 敲低 GLI1 或 GLI2 均抑制许多特征明确的 GLI 靶基因(BCL2、MYCN、PTCH2、IL7 和 CCND1)的表达,而仅 GLI1 耗竭抑制 PTCH1 的表达。对大量推定的经典和非经典 Hedgehog/GLI 靶基因的 qPCR 筛选鉴定了进一步的基因(例如 E2F1、BMP1、CDK2),这些基因在 PANC1 细胞中被 GLI1 和/或 GLI2 耗竭强烈下调,并表明 ANO1、AQP1 和 SOCS1 由 GLI1 或 GLI2 的敲低上调。染色质免疫沉淀显示 GLI1 和 GLI2 占据 BCL2、MYCN 和 CCND1 启动子的相同区域。此外,GLI1 的耗竭抑制了这些启动子处 GLI2 的占据,表明 GLI1/GLI2 相互作用是 GLI2 募集到这些位点所必需的。总之,这些发现表明 GLI1 和 GLI2 协调调节一些基因的转录,并为 GLI 蛋白在致癌作用中的作用提供了机制上的见解。

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