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一种与人c-myc mRNA的C末端编码区域结合的蛋白质的纯化及特性

Purification and properties of a protein that binds to the C-terminal coding region of human c-myc mRNA.

作者信息

Prokipcak R D, Herrick D J, Ross J

机构信息

McArdle Laboratory for Cancer Research, University of Wisconsin, Madison 53706.

出版信息

J Biol Chem. 1994 Mar 25;269(12):9261-9.

PMID:8132663
Abstract

The short half-life of c-myc mRNA is influenced by sequences in the 3'-untranslated region and the C-terminal part of the coding region. In cell-free extracts, a polysomal protein binds to RNA corresponding to the coding region stability determinant. This and other observations suggest that the protein is bound to polysome-associated c-myc mRNA and protects the mRNA from a ribosome-associated endoribonuclease (Bernstein, P.L., Herrick, D.J., Prokipcak, R.D., and Ross, J. (1992) Genes & Dev. 6, 642-654). Here, we describe a four-step purification of the binding protein: solubilization from ribosomes, ammonium sulfate precipitation, RNA affinity chromatography, and reverse-phase high performance liquid chromatography. The 70-kDa protein can be renatured from solutions containing sodium dodecyl sulfate or organic solvents, greatly facilitating its purification. Protein binding to c-myc coding region RNA is blocked by diamide and N-ethylmaleimide, indicating a requirement for sulfhydryl groups. The protein also binds to N-myc coding region RNA but with approximately 5-fold lower affinity than to the comparable c-myc region. Excess c-myc competitor RNA induces 8-fold destabilization of c-myc mRNA in cell-free mRNA decay extracts. In contrast, N-myc coding region competitor RNA has no effect on c-myc mRNA half-life. Therefore, the protein we have purified probably affects c-myc mRNA metabolism with high specificity.

摘要

c-myc信使核糖核酸(mRNA)的短半衰期受3'-非翻译区及编码区C末端部分序列的影响。在无细胞提取物中,一种多核糖体蛋白与对应编码区稳定性决定因素的RNA结合。这一现象及其他观察结果表明,该蛋白与多核糖体相关的c-myc mRNA结合,并保护mRNA免受核糖体相关的核糖核酸内切酶的作用(伯恩斯坦,P.L.,赫里克,D.J.,普罗基帕克,R.D.,和罗斯,J.(1992年)《基因与发育》6,642 - 654)。在此,我们描述了结合蛋白的四步纯化过程:从核糖体上溶解、硫酸铵沉淀、RNA亲和层析和反相高效液相色谱。这种70 kDa的蛋白可从含有十二烷基硫酸钠或有机溶剂的溶液中复性,极大地促进了其纯化。二酰胺和N-乙基马来酰亚胺可阻断该蛋白与c-myc编码区RNA的结合,表明需要巯基。该蛋白也能与N-myc编码区RNA结合,但亲和力比与相应的c-myc区域低约5倍。过量的c-myc竞争RNA在无细胞mRNA降解提取物中可诱导c-myc mRNA 8倍的不稳定。相比之下,N-myc编码区竞争RNA对c-myc mRNA半衰期没有影响。因此,我们纯化的蛋白可能以高度特异性影响c-myc mRNA的代谢。

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