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编码P物质、神经激肽A、神经肽K和神经肽γ的大鼠前速激肽原基因的结构、表达及一些调控机制。

Structure, expression, and some regulatory mechanisms of the rat preprotachykinin gene encoding substance P, neurokinin A, neuropeptide K, and neuropeptide gamma.

作者信息

Carter M S, Krause J E

机构信息

Department of Anatomy and Neurobiology, Washington University School of Medicine, St. Louis, Missouri 63110.

出版信息

J Neurosci. 1990 Jul;10(7):2203-14. doi: 10.1523/JNEUROSCI.10-07-02203.1990.

DOI:10.1523/JNEUROSCI.10-07-02203.1990
PMID:1695945
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6570392/
Abstract

The rat preprotachykinin (PPT) gene encoding the neuropeptides substance P (SP), neurokinin A (NKA), neuropeptide K (NPK), and neuropeptide gamma was isolated from a lambda Charon 4A genomic library. Two overlapping clones contained all of the exons present in beta-PPT, including some 7 and 9 kb 5' and 3' flanking sequence, respectively. The presence of 1 major and 2 minor transcription initiation sites was determined from primer extension and nuclease protection experiments. Analysis of the nucleotide sequence homology between the rat and bovine revealed the presence of highly conserved regions throughout the entire coding region and within the 5' flanking sequences. Primer extension and nuclease protection experiments demonstrated that the primary transcript is differentially spliced primarily into gamma- and beta-PPT mRNA in all tissues examined in the adult rat where the gene is expressed. beta-PPT mRNA contains all of the exons, whereas gamma-PPT mRNA lacks exon 4, which encodes part of the N-terminus of NPK. The alpha-PPT mRNA, which lacks exon 6 (the sequence encoding NKA and processing sites), comprises about 1% of the total PPT mRNA. An RNA secondary structure model is proposed to account for these specific exon exclusion events in the RNA splicing process. These results are discussed with regard to the mechanisms regulating SP gene expression and the functional significance of differential RNA splicing in the rat.

摘要

从λ噬菌体Charon 4A基因组文库中分离出编码神经肽P物质(SP)、神经激肽A(NKA)、神经肽K(NPK)和神经肽γ的大鼠前速激肽原(PPT)基因。两个重叠克隆包含了β-PPT中存在的所有外显子,分别包括约7 kb和9 kb的5'和3'侧翼序列。通过引物延伸和核酸酶保护实验确定了1个主要和2个次要转录起始位点。大鼠和牛之间核苷酸序列同源性分析表明,在整个编码区和5'侧翼序列中存在高度保守区域。引物延伸和核酸酶保护实验表明,在成年大鼠中该基因表达的所有组织中,初级转录本主要差异剪接为γ-和β-PPT mRNA。β-PPT mRNA包含所有外显子,而γ-PPT mRNA缺少编码NPK N端部分的外显子4。缺少外显子6(编码NKA和加工位点的序列)的α-PPT mRNA约占总PPT mRNA的1%。提出了一个RNA二级结构模型来解释RNA剪接过程中的这些特定外显子排除事件。就调节SP基因表达的机制以及大鼠中差异RNA剪接的功能意义对这些结果进行了讨论。