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小鼠激素敏感性脂肪酶基因的分离与鉴定

Isolation and characterization of the gene for mouse hormone-sensitive lipase.

作者信息

Li Z, Sumida M, Birchbauer A, Schotz M C, Reue K

机构信息

West Los Angeles VA Medical Center, California 90073.

出版信息

Genomics. 1994 Nov 15;24(2):259-65. doi: 10.1006/geno.1994.1614.

DOI:10.1006/geno.1994.1614
PMID:7698747
Abstract

Hormone-sensitive lipase (HSL) is the rate-limiting enzyme in hydrolysis of triglycerides in adipose tissue and of cholesteryl esters in steroidogenic tissues and macrophages. The gene encoding mouse HSL has been isolated and characterized from two overlapping lambda clones. The gene spans approximately 10.4 kb and comprises 9 exons interrupted by 8 introns. The deduced amino acid sequence specifies a protein of 759 amino acids with a Mr of 83,297 in the absence of posttranslational modifications. The known functional domains of the HSL protein are encoded by discrete exons, with the putative catalytic site (Ser423) encoded by exon 6, and the basal and regulatory phosphorylation sites (Ser557 and Ser559) encoded by exon 8. In addition, a putative lipid binding domain occurs in exon 9. The mouse protein shows 94% identity with the previously determined rat sequence and 85% identity with the recently determined human sequence. Interestingly, despite the high degree of similarity, the three species diverge significantly for a stretch of 16 amino acid residues upstream of the phosphorylation sites. In addition, an error was discovered in the carboxyl-terminal portion of the previously reported rat sequence, which produced a frame shift and premature termination of the coding sequence. The corrected rat sequence alters the identity of 12 amino acid residues and extends the protein an additional 11 residues. We have also examined the mouse HSL gene and 5' flanking region for nucleotide sequences that may modulate HSL gene transcription. Using primer extension, we identified a major transcription initiation site 593 nucleotides upstream of the protein coding sequence.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

激素敏感性脂肪酶(HSL)是脂肪组织中甘油三酯以及类固醇生成组织和巨噬细胞中胆固醇酯水解的限速酶。从小鼠中分离出编码HSL的基因,并通过两个重叠的λ克隆对其进行了表征。该基因跨度约为10.4 kb,包含9个外显子,被8个内含子打断。推导的氨基酸序列确定了一个由759个氨基酸组成的蛋白质,在没有翻译后修饰的情况下,其相对分子质量为83,297。HSL蛋白的已知功能域由离散的外显子编码,推测的催化位点(Ser423)由外显子6编码,基础和调节性磷酸化位点(Ser557和Ser559)由外显子8编码。此外,推测的脂质结合域出现在外显子9中。小鼠蛋白与先前确定的大鼠序列具有94%的同一性,与最近确定的人类序列具有85%的同一性。有趣的是,尽管相似度很高,但这三个物种在磷酸化位点上游的一段16个氨基酸残基处存在显著差异。此外,在先前报道的大鼠序列的羧基末端部分发现了一个错误,该错误导致编码序列发生移码和过早终止。校正后的大鼠序列改变了12个氨基酸残基的同一性,并使蛋白质额外延伸了11个残基。我们还检查了小鼠HSL基因和5'侧翼区域中可能调节HSL基因转录的核苷酸序列。使用引物延伸法,我们在蛋白质编码序列上游593个核苷酸处确定了一个主要转录起始位点。(摘要截短为250字)

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