FOXF1的父系拷贝的一个小的De Novo CNV缺失,使lncRNA FENDRR保持完整,提供了对其双向启动子区域的深入了解。

IF 3.6 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY Non-Coding RNA Pub Date : 2023-10-09 DOI:10.3390/ncrna9050061
Przemyslaw Szafranski, Paweł Stankiewicz
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引用次数: 0

摘要

涉及FOXF1转录因子基因的致病性单核苷酸变异株(SNV)和拷贝数变异株(CNV)缺失或其远处肺特异性增强子的CNV缺失是肺泡毛细血管发育不良伴肺静脉错位(ACDMPV)的原因,ACDMPV是一种罕见的新生儿致命性肺发育障碍。与FOXF1内的SNV和仅涉及FOXF1增强子的CNV缺失相反,涉及FOXFl和相邻的反向lncRNA基因FENDRR的较大大小的缺失还与发育不良左心综合征和单脐动脉(SUA)相关。在这里,在一个没有任何先天性心脏缺陷或SUA的ACDMPV婴儿中,我们发现了一个小的5kb CNV缺失,该缺失去除了FOXF1及其启动子的父系等位基因,使FENDRR及其启动子保持完整。IMR-90胎儿细胞系中的报告基因分析表明,缺失可能确实没有显著影响FENDRR的表达。它还显示了FOXF1-FENDRR启动子间区的极化,该极化由其增加FENDRR转录但不增加FOXF1转录的能力组成。有趣的是,这种转录刺激活性在FOXF1启动子存在的情况下被抑制。我们的数据进一步阐明了FOXF1-FENDRR的相邻启动子与可能的其他差异转录的信使核糖核酸基因对之间的相互作用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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A Small De Novo CNV Deletion of the Paternal Copy of FOXF1, Leaving lncRNA FENDRR Intact, Provides Insight into Their Bidirectional Promoter Region.

Pathogenic single-nucleotide variants (SNVs) and copy-number variant (CNV) deletions involving the FOXF1 transcription factor gene or CNV deletions of its distant lung-specific enhancer are responsible for alveolar capillary dysplasia with misalignment of pulmonary veins (ACDMPV), a rarely diagnosed lethal lung developmental disorder in neonates. In contrast to SNVs within FOXF1 and CNV deletions involving only the FOXF1 enhancer, larger-sized deletions involving FOXF1 and the adjacent, oppositely oriented lncRNA gene FENDRR have additionally been associated with hypoplastic left heart syndrome and single umbilical artery (SUA). Here, in an ACDMPV infant without any congenital heart defect or SUA, we identified a small 5 kb CNV deletion that removed the paternal allele of FOXF1 and its promoter, leaving FENDRR and its promoter intact. Reporter assay in the IMR-90 fetal cell line implied that the deletion may indeed not have significantly affected FENDRR expression. It also showed a polarization of the FOXF1-FENDRR inter-promoter region consisting of its ability to increase the transcription of FENDRR but not FOXF1. Interestingly, this transcription-stimulating activity was suppressed in the presence of the FOXF1 promoter. Our data shed more light on the interactions between neighboring promoters of FOXF1-FENDRR and possibly other divergently transcribed mRNA-lncRNA gene pairs.

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来源期刊
Non-Coding RNA
Non-Coding RNA Biochemistry, Genetics and Molecular Biology-Genetics
CiteScore
6.70
自引率
4.70%
发文量
74
审稿时长
10 weeks
期刊介绍: Functional studies dealing with identification, structure-function relationships or biological activity of: small regulatory RNAs (miRNAs, siRNAs and piRNAs) associated with the RNA interference pathway small nuclear RNAs, small nucleolar and tRNAs derived small RNAs other types of small RNAs, such as those associated with splice junctions and transcription start sites long non-coding RNAs, including antisense RNAs, long ''intergenic'' RNAs, intronic RNAs and ''enhancer'' RNAs other classes of RNAs such as vault RNAs, scaRNAs, circular RNAs, 7SL RNAs, telomeric and centromeric RNAs regulatory functions of mRNAs and UTR-derived RNAs catalytic and allosteric (riboswitch) RNAs viral, transposon and repeat-derived RNAs bacterial regulatory RNAs, including CRISPR RNAS Analysis of RNA processing, RNA binding proteins, RNA signaling and RNA interaction pathways: DICER AGO, PIWI and PIWI-like proteins other classes of RNA binding and RNA transport proteins RNA interactions with chromatin-modifying complexes RNA interactions with DNA and other RNAs the role of RNA in the formation and function of specialized subnuclear organelles and other aspects of cell biology intercellular and intergenerational RNA signaling RNA processing structure-function relationships in RNA complexes RNA analyses, informatics, tools and technologies: transcriptomic analyses and technologies development of tools and technologies for RNA biology and therapeutics Translational studies involving long and short non-coding RNAs: identification of biomarkers development of new therapies involving microRNAs and other ncRNAs clinical studies involving microRNAs and other ncRNAs.
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