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首页> 美国卫生研究院文献>PLoS Genetics >Tethering of the Conserved piggyBac Transposase Fusion Protein CSB-PGBD3 to Chromosomal AP-1 Proteins Regulates Expression of Nearby Genes in Humans
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Tethering of the Conserved piggyBac Transposase Fusion Protein CSB-PGBD3 to Chromosomal AP-1 Proteins Regulates Expression of Nearby Genes in Humans

机译:保守的piggyBac转座酶融合蛋白CSB-PGBD3与染色体AP-1蛋白的网络连接调节人类附近基因的表达。

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The CSB-PGBD3 fusion protein arose more than 43 million years ago when a 2.5-kb piggyBac 3 (PGBD3) transposon inserted into intron 5 of the Cockayne syndrome Group B (CSB) gene in the common ancestor of all higher primates. As a result, full-length CSB is now coexpressed with an abundant CSB-PGBD3 fusion protein by alternative splicing of CSB exons 1–5 to the PGBD3 transposase. An internal deletion of the piggyBac transposase ORF also gave rise to 889 dispersed, 140-bp MER85 elements that were mobilized in trans by PGBD3 transposase. The CSB-PGBD3 fusion protein binds MER85s in vitro and induces a strong interferon-like innate antiviral immune response when expressed in CSB-null UVSS1KO cells. To explore the connection between DNA binding and gene expression changes induced by CSB-PGBD3, we investigated the genome-wide DNA binding profile of the fusion protein. CSB-PGBD3 binds to 363 MER85 elements in vivo, but these sites do not correlate with gene expression changes induced by the fusion protein. Instead, CSB-PGBD3 is enriched at AP-1, TEAD1, and CTCF motifs, presumably through protein–protein interactions with the cognate transcription factors; moreover, recruitment of CSB-PGBD3 to AP-1 and TEAD1 motifs correlates with nearby genes regulated by CSB-PGBD3 expression in UVSS1KO cells and downregulated by CSB rescue of mutant CS1AN cells. Consistent with these data, the N-terminal CSB domain of the CSB-PGBD3 fusion protein interacts with the AP-1 transcription factor c-Jun and with RNA polymerase II, and a chimeric CSB-LacI construct containing only the N-terminus of CSB upregulates many of the genes induced by CSB-PGBD3. We conclude that the CSB-PGBD3 fusion protein substantially reshapes the transcriptome in CS patient CS1AN and that continued expression of the CSB-PGBD3 fusion protein in the absence of functional CSB may affect the clinical presentation of CS patients by directly altering the transcriptional program.
机译:CSB-PGBD3融合蛋白诞生于4300万年前,当时一个2.5 kb的piggyBac 3(PGBD3)转座子插入了所有高级灵长类动物共同祖先Cockayne综合征B组(CSB)基因的内含子5中。结果,通过将CSB外显子1-5与PGBD3转座酶选择性剪接,全长CSB现在可以与丰富的CSB-PGBD3融合蛋白共表达。 piggyBac转座酶ORF的内部缺失也产生了889个分散的140bp MER85元件,其被PGBD3转座酶反式动员。 CSB-PGBD3融合蛋白在体外结合MER85,并在无CSB的UVSS1KO细胞中表达时诱导强烈的干扰素样先天抗病毒免疫应答。为了探索CSB-PGBD3诱导的DNA结合与基因表达变化之间的联系,我们研究了融合蛋白的全基因组DNA结合谱。 CSB-PGBD3在体内与363个MER85元件结合,但这些位点与融合蛋白诱导的基因表达变化不相关。相反,CSB-PGBD3富含AP-1,TEAD1和CTCF基序,大概是通过蛋白质与同源转录因子的相互作用。此外,CSB-PGBD3募集到AP-1和TEAD1基序与附近基因受UVSS1KO细胞中CSB-PGBD3表达的调控以及CSB拯救突变CS1AN细胞的调控。与这些数据一致,CSB-PGBD3融合蛋白的N末端CSB结构域与AP-1转录因子c-Jun和RNA聚合酶II和仅包含CSB N末端的嵌合CSB-LacI构建体相互作用上调CSB-PGBD3诱导的许多基因。我们得出的结论是,CSB-PGBD3融合蛋白可显着重塑CS患者CS1AN中的转录组,并且在缺少功能性CSB的情况下CSB-PGBD3融合蛋白的持续表达可能会通过直接改变转录程序来影响CS患者的临床表现。

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