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克隆和启动子分析参与骨骼肌细胞成熟的 Palladin 90kDa、140kDa 和 200kDa 同工型。

Cloning and promoter analysis of palladin 90-kDa, 140-kDa, and 200-kDa isoforms involved in skeletal muscle cell maturation.

机构信息

Department of Life Sciences, College of Biosciences and Biotechnology, National Cheng Kung University, No. 1 University Road, East Dist.,, Tainan City, 701, Taiwan (R.O.C.).

Institute of Tropical Plant Sciences, College of Biosciences and Biotechnology, National Cheng Kung University, Tainan, Taiwan (R.O.C.).

出版信息

BMC Res Notes. 2020 Jul 3;13(1):321. doi: 10.1186/s13104-020-05152-9.

Abstract

OBJECTIVE

Palladin is a ubiquitous phosphoprotein expressed in vertebrate cells that works as a scaffolding protein. Several isoforms deriving from alternative splicing are originated from the palladin gene and involved in mesenchymal and muscle cells formation, maturation, migration, and contraction. Recent studies have linked palladin to the invasive spread of cancer and myogenesis. However, since its discovery, the promoter region of the palladin gene has never been studied. The objective of this study was to predict, identify, and measure the activity of the promoter regions of palladin gene.

RESULTS

By using promoter prediction programs, we successfully identified the transcription start sites for the Palld isoforms and revealed the presence of a variety of transcriptional regulatory elements including TATA box, GATA, MyoD, myogenin, MEF, Nkx2-5, and Tcf3 upstream promoter regions. The transcriptome profiling approach confirmed the active role of predicted transcription factors in the mouse genome. This study complements the missing piece in the characterization of palladin gene and certainly contributes to understanding the complexity and enrollment of palladin regulatory factors in gene transcription.

摘要

目的

Palladin 是一种广泛存在于脊椎动物细胞中的磷酸化蛋白,作为一种支架蛋白发挥作用。几种源自选择性剪接的同工型来源于 Palladin 基因,参与间充质和肌肉细胞的形成、成熟、迁移和收缩。最近的研究将 Palladin 与癌症的侵袭性扩散和肌发生联系起来。然而,自从发现 Palladin 以来,其基因的启动子区域从未被研究过。本研究的目的是预测、鉴定和测量 Palladin 基因启动子区域的活性。

结果

通过使用启动子预测程序,我们成功地确定了 Palld 同工型的转录起始位点,并揭示了存在多种转录调控元件,包括 TATA 盒、GATA、MyoD、myogenin、MEF、Nkx2-5 和 Tcf3 上游启动子区域。转录组谱分析方法证实了预测的转录因子在小鼠基因组中的活性作用。这项研究补充了 Palladin 基因特征描述中的缺失部分,肯定有助于理解 Palladin 调控因子在基因转录中的复杂性和募集。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/82a2/7333403/fb229529bfb1/13104_2020_5152_Fig1_HTML.jpg

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