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小鼠金属硫蛋白-I基因的金属调控元件

Metal regulatory elements of the mouse metallothionein-I gene.

作者信息

Searle P F, Stuart G W, Palmiter R D

机构信息

Howard Hughes Medical Institute Laboratory, Department of Biochemistry, University of Washington, Seattle 98195.

出版信息

Experientia Suppl. 1987;52:407-14. doi: 10.1007/978-3-0348-6784-9_39.

Abstract

The promoter of the mouse metallothionein-I (mMT-I) gene contains multiple metal regulatory elements (MREs) which allow transcription of the gene to be induced by heavy metals. Insertion into the promoter of the TK gene of two or more synthetic MREs enables that gene to respond to heavy metals. We tested each of the MREs from the mMT-I promoter in this assay, and found four to be functional. We have commenced a systematic analysis of single nucleotide changes within an MRE, to determine the contribution of each nucleotide. The MRE core sequence in which single nucleotide changes can abolish function is TGCRCNCG; certain changes outside this sequence have lesser effects. MREs can act cooperatively with distal promoter elements of the TK gene, but in the presence of just a TATA-box they function as heavy-metal dependent promoter elements. Experiments to determine the effect of spacing suggest a range of at least 90 bp for interaction of two MREs, but the range for efficient stimulation of transcription from a TATA-box appears to be shorter. Stimulation of MT gene transcription by heavy metals is probably mediated by heavy metal-activated regulatory proteins binding cooperatively to the multiple MREs.

摘要

小鼠金属硫蛋白-I(mMT-I)基因的启动子含有多个金属调节元件(MREs),这些元件可使该基因的转录被重金属诱导。将两个或更多个合成MREs插入TK基因的启动子中,可使该基因对重金属产生反应。我们在此检测中测试了来自mMT-I启动子的每个MREs,发现其中四个具有功能。我们已开始对MRE内的单核苷酸变化进行系统分析,以确定每个核苷酸的作用。单核苷酸变化可消除功能的MRE核心序列为TGCRCNCG;该序列外的某些变化影响较小。MREs可与TK基因的远端启动子元件协同作用,但在仅存在TATA框的情况下,它们作为重金属依赖性启动子元件发挥作用。确定间距影响的实验表明,两个MREs相互作用的范围至少为90 bp,但从TATA框有效刺激转录的范围似乎更短。重金属对MT基因转录的刺激可能是由重金属激活的调节蛋白与多个MREs协同结合介导的。

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