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蛋白激酶A刺激多种蛋白质与乳酸脱氢酶A mRNA 3'非翻译区中富含U的结构域结合,该结构域是调节mRNA稳定性所必需的。

Protein kinase A stimulates binding of multiple proteins to a U-rich domain in the 3'-untranslated region of lactate dehydrogenase A mRNA that is required for the regulation of mRNA stability.

作者信息

Tian D, Huang D, Brown R C, Jungmann R A

机构信息

Department of Cellular and Molecular Biology and Cancer Center, Northwestern University Medical School, Chicago, Illinois 60611, USA.

出版信息

J Biol Chem. 1998 Oct 23;273(43):28454-60. doi: 10.1074/jbc.273.43.28454.

Abstract

We have explored the molecular basis of the cAMP-induced stabilization of lactate dehydrogenase A (LDH-A) mRNA and identified four cytoplasmic proteins of 96, 67, 52, and 50 kDa that specifically bind to a 30-nucleotide uridine-rich sequence in the LDH 3'-untranslated region with a predicted stem-loop structure. Mutational analysis revealed that specific protein binding is dependent upon an intact primary nucleotide sequence in the loop as well as integrity of the adjoining double-stranded stem structure, thus indicating a high degree of primary and secondary structure specificity. The critical stem-loop region is located between nucleotides 1473 and 1502 relative to the mRNA cap site and contains a previously identified cAMP-stabilizing region (CSR) required for LDH-A mRNA stability regulation by the protein kinase A pathway. The 3'-untranslated region binding activity of the proteins is up-regulated after protein kinase A activation, whereas protein dephosphorylation is associated with a loss of binding activity. These results imply a cause and effect relationship between LDH-A mRNA stabilization and CSR-phosphoprotein binding activity. We propose that the U-rich CSR is a recognition signal for CSR-binding proteins and for an mRNA processing pathway that specifically stabilizes LDH mRNA in response to activation of the protein kinase A signal transduction pathway.

摘要

我们探究了环磷酸腺苷(cAMP)诱导乳酸脱氢酶A(LDH-A)信使核糖核酸(mRNA)稳定性的分子基础,并鉴定出四种细胞质蛋白,分子量分别为96、67、52和50千道尔顿,它们能特异性结合LDH 3'非翻译区一段富含尿苷的30个核苷酸序列,该序列具有预测的茎环结构。突变分析表明,特异性蛋白结合依赖于环内完整的一级核苷酸序列以及相邻双链茎结构的完整性,这表明其具有高度的一级和二级结构特异性。关键的茎环区域相对于mRNA帽位点位于核苷酸1473至1502之间,并且包含先前鉴定的cAMP稳定区域(CSR),该区域是蛋白激酶A途径调节LDH-A mRNA稳定性所必需的。蛋白激酶A激活后,这些蛋白的3'非翻译区结合活性上调,而蛋白去磷酸化与结合活性丧失相关。这些结果暗示了LDH-A mRNA稳定性与CSR-磷蛋白结合活性之间存在因果关系。我们提出,富含尿苷的CSR是CSR结合蛋白以及一种mRNA加工途径的识别信号,该途径可响应蛋白激酶A信号转导途径的激活而特异性地稳定LDH mRNA。

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