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6
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Cell- and gene-specific regulation of primary target genes by the androgen receptor.雄激素受体对初级靶基因的细胞和基因特异性调控。
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A transcription factor of lipid synthesis, sterol regulatory element-binding protein (SREBP)-1a causes G(1) cell-cycle arrest after accumulation of cyclin-dependent kinase (cdk) inhibitors.脂质合成的转录因子固醇调节元件结合蛋白(SREBP)-1a在细胞周期蛋白依赖性激酶(cdk)抑制剂积累后导致G1期细胞周期停滞。
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对小鼠肝脏染色质中SREBP-1结合的全基因组分析揭示了其对启动子近端结合新基序的偏好。

Genome-wide analysis of SREBP-1 binding in mouse liver chromatin reveals a preference for promoter proximal binding to a new motif.

作者信息

Seo Young-Kyo, Chong Hansook Kim, Infante Aniello M, Im Seung-Soon, Xie Xiaohui, Osborne Timothy F

机构信息

Department of Molecular Biology and Biochemistry, University of California, Irvine, CA 92697, USA.

出版信息

Proc Natl Acad Sci U S A. 2009 Aug 18;106(33):13765-9. doi: 10.1073/pnas.0904246106. Epub 2009 Aug 4.

DOI:10.1073/pnas.0904246106
PMID:19666523
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2728968/
Abstract

Lipid homeostasis in vertebrates is regulated by 3 sterol regulatory element binding protein (SREBP) isoforms. Here, we identify targets of SREBP-1 in mammalian liver using chromatin immunoprecipitation-high-throughput DNA sequencing. Antisera to SREBP-1 were used with liver chromatin from mice fed a high-carbohydrate diet after a fast, which leads to superinduction of hepatic SREBP-1c expression. SREBP-1-DNA complexes were subjected to massive parallel DNA sequencing using the Illumina Genome Analyzer II, resulting in 5.7 million sequence reads. Mapping these reads to the mouse reference genome identified 426 peaks of SREBP-1 binding vs. a control antibody. These binding peaks show a striking enrichment in proximal promoter regions, with 52% located within 1 kb upstream of a transcription start site. A previously undescribed sequence motif (5'-ACTACANNTCCC-3') was present in 76% of the total peaks, and we show that it is a functional SREBP-1 response element. Our analysis also reveals that an Sp1 consensus site is present as a "coregulatory" motif in 50% of the SREBP-1 binding peaks, consistent with previous functional studies. SREBP-1 bound not only to many well-characterized SREBP-1 target genes but to several other previously unknown targets in lipid and carbohydrate metabolism as well as many putative target genes in other diverse biological pathways.

摘要

脊椎动物中的脂质稳态由3种固醇调节元件结合蛋白(SREBP)异构体调控。在此,我们利用染色质免疫沉淀-高通量DNA测序技术鉴定了哺乳动物肝脏中SREBP-1的靶标。将针对SREBP-1的抗血清与禁食后喂食高碳水化合物饮食的小鼠肝脏染色质一起使用,这会导致肝脏SREBP-1c表达的超诱导。使用Illumina Genome Analyzer II对SREBP-1-DNA复合物进行大规模平行DNA测序,产生了570万个序列读数。将这些读数映射到小鼠参考基因组,与对照抗体相比,鉴定出426个SREBP-1结合峰。这些结合峰在近端启动子区域表现出显著富集,52%位于转录起始位点上游1 kb内。在76%的总峰中存在一个先前未描述的序列基序(5'-ACTACANNTCCC-3'),我们证明它是一个功能性SREBP-1反应元件。我们的分析还表明,在50%的SREBP-1结合峰中,Sp1共有位点作为“共调节”基序存在,这与先前的功能研究一致。SREBP-1不仅与许多已充分表征的SREBP-1靶基因结合,还与脂质和碳水化合物代谢中的其他几个先前未知的靶标以及其他多种生物学途径中的许多假定靶基因结合。