The optional long 5′-untranslated region of human ACAT1 mRNAs impairs the production of ACAT1 protein by promoting its mRNA decay

被引:8
作者
Zhao, Xiaonan [1 ]
Chen, Jia [1 ]
Lei, Lei [1 ]
Hu, Guangjing [1 ]
Xiong, Ying [1 ]
Xu, Jiajia [1 ]
Li, Qin [1 ]
Yang, Xinying [1 ]
Chang, Catherine C. Y. [2 ]
Song, Baoliang [1 ]
Chang, Tayuan [2 ]
Li, Boliang [1 ]
机构
[1] Chinese Acad Sci, State Key Lab Mol Biol, Inst Biochem & Cell Biol, Shanghai Inst Biol Sci, Shanghai 200031, Peoples R China
[2] Dartmouth Med Sch, Dept Biochem, Hanover, NH 03756 USA
基金
美国国家卫生研究院; 中国国家自然科学基金;
关键词
human ACAT1 mRNA; long 5 '-UTR; mRNA stability; mRNA decay; ACAT1 protein production; A-CHOLESTEROL ACYLTRANSFERASE; 2 DIFFERENT CHROMOSOMES; ACYL-COENZYME; MAMMALIAN-CELLS; IN-VITRO; TRANSLATION INITIATION; SECONDARY STRUCTURES; GENE-EXPRESSION; RICH ELEMENTS; COA;
D O I
10.1093/abbs/gmn004
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
We have previously reported that human ACAT1 mRNAs produce the 50 kDa protein using the AUG(1397-1399) initiation codon, and also a minor 56 kDa isoform using the upstream in-frame GGC(1274-1276) initiation codon. The GGC(1274-1276) codon is located at the optional long 5'-untranslated region (5'-UTR, nt 1-1396) of the mRNAs. The DNA sequences corresponding to this 5'-UTR are located in two different chromosomes, 7 and 1. In the current work, we report that the optional long 5'-UTR significantly impairs the production of human ACAT1 protein initiated from the AUG(1397-1399) codon, mainly by promoting its mRNA decay. The western blot analyses indicated that the optional long 5'-UTR potently impaired the production of different proteins initiated from the AUG(1397-1399) codon, meaning that this impairing effect was not influenced by the 3'-UTR or the coding sequence of ACAT1 mRNA. The results of reverse transcription-quantitative polymerase chain reaction demonstrated that this 5'-UTR dramatically reduced the contents of its linked mRNAs. Analyses of the protein to mRNA ratios showed that this 5'-UTR mainly decreased its mRNA stability rather than altering its translational efficiency. We next performed the plasmid transfection experiments and used actinomycin D to inhibit transcription. The results showed that this 5'-UTR promoted its mRNA decay. Additional transfection and nucleofection experiments using RNAs prepared in vitro illustrated that, in both the cytoplasm and the nucleus of cells, the optional long 5'-UTR-linked mRNAs decayed faster than those without the link. Overall, our study brings new insight to the regulation of the human ACAT1 gene expression at the post-transcription level.
引用
收藏
页码:30 / 41
页数:12
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