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Pdx1的类泛素化修饰与其核定位及胰岛素基因激活相关。

Sumoylation of Pdx1 is associated with its nuclear localization and insulin gene activation.

作者信息

Kishi Akio, Nakamura Takaaki, Nishio Yoshihiko, Maegawa Hiroshi, Kashiwagi Atsunori

机构信息

Departments of Medicine and Anatomy, Shiga University of Medical Science, Seta, Otsu, Shiga 520-2192 Japan.

出版信息

Am J Physiol Endocrinol Metab. 2003 Apr;284(4):E830-40. doi: 10.1152/ajpendo.00390.2002. Epub 2002 Dec 17.

Abstract

Pancreatic duodenal homeobox-1 (Pdx1) is a transcription factor, and its phosphorylation is thought to be essential for activation of insulin gene expression. This phosphorylation is related to a concomitant shift in molecular mass from 31 to 46 kDa. However, we found that Pdx1 was modified by SUMO-1 (small ubiquitin-related modifier 1) in beta-TC-6 and COS-7 cells, which were transfected with Pdx1 cDNA. This modification contributed to the increase in molecular mass of Pdx1 from 31 to 46 kDa. Additionally, sumoylated Pdx1 localized in the nucleus. The reduction of SUMO-1 protein by use of RNA interference (SUMO-iRNAs) resulted in a significant decrease in Pdx1 protein in the nucleus. A 34-kDa form of Pdx1 was detected by the cells exposed to SUMO-iRNAs in the presence of lactacystin, a proteasome inhibitor. Furthermore, the reduced nuclear sumoylated Pdx1 content was associated with significant lower transcriptional activity of the insulin gene. These findings indicate that SUMO-1 modification is associated with both the localization and stability of Pdx1 as well as its effect on insulin gene activation.

摘要

胰腺十二指肠同源盒蛋白-1(Pdx1)是一种转录因子,其磷酸化被认为是胰岛素基因表达激活所必需的。这种磷酸化与分子量从31 kDa伴随性地转变为46 kDa有关。然而,我们发现,在转染了Pdx1 cDNA的β-TC-6和COS-7细胞中,Pdx1被小泛素相关修饰物1(SUMO-1)修饰。这种修饰导致Pdx1的分子量从31 kDa增加到46 kDa。此外,经SUMO修饰的Pdx1定位于细胞核。通过RNA干扰(SUMO-iRNAs)降低SUMO-1蛋白水平,导致细胞核中Pdx1蛋白显著减少。在蛋白酶体抑制剂乳胞素存在的情况下,暴露于SUMO-iRNAs的细胞检测到一种34 kDa形式的Pdx1。此外,细胞核中经SUMO修饰的Pdx1含量降低与胰岛素基因的转录活性显著降低有关。这些发现表明,SUMO-1修饰与Pdx1的定位、稳定性及其对胰岛素基因激活的作用均相关。

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