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小鼠脂蛋白脂肪酶基因的结构:一个B1重复元件插入到mRNA的3'非翻译区。

The structure of the mouse lipoprotein lipase gene: a B1 repetitive element is inserted into the 3' untranslated region of the mRNA.

作者信息

Zechner R, Newman T C, Steiner E, Breslow J L

机构信息

Institute of Medical Biochemistry, University of Graz, Austria.

出版信息

Genomics. 1991 Sep;11(1):62-76. doi: 10.1016/0888-7543(91)90102-k.

Abstract

The catabolism of triglycerides-rich lipoproteins and the subsequent uptake of free fatty acids by muscle and adipose tissue is dependent on the enzyme lipoprotein lipase (LPL). To better understand the regulation of this enzyme, we have isolated and characterized the mouse LPL gene. The gene is 28 kb in length and comprises 10 exons which encode a 4.0-kb mRNA. In this report, almost 6 kb of DNA sequence is presented, including 1251 bp 5' to the gene, over 4 kb of exon and exon-intron junctions, and 583 bp 3' to the gene. RNA from differentiated 3T3-L1 adipocytes was used in primer extension and RNase protection assays to show that the 5' untranslated region is not interrupted by an intron and the start site of transcription is 199 bp 5' to the ATG codon that begins translation. The first exon codes for the 5' untranslated region and the signal peptide of 27 amino acids and 2 amino acids of the mature protein, exons 2-9 code for 445 amino acids of the mature protein. These exons are short and vary in length from 102 to 287 bp. The 10th exon codes for the 3' untranslated region and is 2346 bp long. This exon contains a single copy of a B1 repetitive element of 152 bp followed by a 169-bp homopurine stretch. These elements are flanked by a pair of 16-bp direct repeats. The mouse gene is similar in size to the human, which also contains 10 exons in similar locations. There is a high degree of sequence homology between the two genes, 5' region (700 bp), 75%; 5' untranslated region, 74%; coding region, 88%; 3' untranslated region, 75%. The most striking difference is the absence of the B1 repetitive element and homopurine region in the human 3' untranslated region. This information about the mouse LPL gene may lead to a better understanding of its regulation and role in plasma lipoprotein metabolism.

摘要

富含甘油三酯的脂蛋白的分解代谢以及随后肌肉和脂肪组织对游离脂肪酸的摄取依赖于脂蛋白脂肪酶(LPL)。为了更好地理解这种酶的调控机制,我们分离并鉴定了小鼠LPL基因。该基因长度为28 kb,由10个外显子组成,编码一个4.0 kb的mRNA。在本报告中,呈现了近6 kb的DNA序列,包括基因5'端的1251 bp、超过4 kb的外显子和外显子 - 内含子连接区以及基因3'端的583 bp。来自分化的3T3 - L1脂肪细胞的RNA用于引物延伸和RNA酶保护试验,以表明5'非翻译区未被内含子打断,转录起始位点在开始翻译的ATG密码子的5'端199 bp处。第一个外显子编码5'非翻译区以及27个氨基酸的信号肽和成熟蛋白的2个氨基酸,外显子2 - 9编码成熟蛋白的445个氨基酸。这些外显子较短,长度从102到287 bp不等。第10个外显子编码3'非翻译区,长度为2346 bp。该外显子包含一个152 bp的B1重复元件的单拷贝,其后是一个169 bp的同嘌呤序列。这些元件两侧是一对16 bp的直接重复序列。小鼠基因的大小与人类相似,在相似位置也包含10个外显子。两个基因之间存在高度的序列同源性,5'区域(700 bp)为75%;5'非翻译区为74%;编码区为88%;3'非翻译区为75%。最显著的差异是人类3'非翻译区不存在B1重复元件和同嘌呤区域。关于小鼠LPL基因的这些信息可能有助于更好地理解其在血浆脂蛋白代谢中的调控和作用。

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