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绵羊肉碱棕榈酰转移酶1肝脏和肌肉同工型的克隆与表达:肌肉同工型N端的残基影响该酶的动力学特性。

Cloning and expression of the liver and muscle isoforms of ovine carnitine palmitoyltransferase 1: residues within the N-terminus of the muscle isoform influence the kinetic properties of the enzyme.

作者信息

Price Nigel T, Jackson Vicky N, van der Leij Feike R, Cameron Jacqueline M, Travers Maureen T, Bartelds Beatrijs, Huijkman Nicolette C, Zammit Victor A

机构信息

Hannah Research Institute, Ayr KA6 5HL, UK.

出版信息

Biochem J. 2003 Jun 15;372(Pt 3):871-9. doi: 10.1042/BJ20030086.

Abstract

The nucleotide sequence data reported will appear in DDBJ, EMBL, GenBank(R) and GSDB Nucleotide Sequence Databases; the sequences of ovine CPT1A and CPT1B cDNAs have the accession numbers Y18387 and AJ272435 respectively and the partial adipose tissue and liver CPT1A clones have the accession numbers Y18830 and Y18829 respectively. Fatty acid and ketone body metabolism differ considerably between monogastric and ruminant species. The regulation of the key enzymes involved may differ accordingly. Carnitine palmitoyltransferase 1 (CPT 1) is the key locus for the control of long-chain fatty acid beta-oxidation and liver ketogenesis. Previously we showed that CPT 1 kinetics in sheep and rat liver mitochondria differ. We cloned cDNAs for both isoforms [liver- (L-) and muscle- (M-)] of ovine CPT 1 in order to elucidate the structural features of these proteins and their genes ( CPT1A and CPT1B ). Their deduced amino acid sequences show a high degree of conservation compared with orthologues from other mammalian species, with the notable exception of the N-terminus of ovine M-CPT 1. These differences were also present in bovine M-CPT 1, whose N-terminal sequence we determined. In addition, the 5'-end of the sheep CPT1B cDNA suggested a different promoter architecture when compared with previously characterized CPT1B genes. Northern blotting revealed differences in tissue distribution for both CPT1A and CPT1B transcripts compared with other species. In particular, ovine CPT1B mRNA was less tissue restricted, and the predominant transcript in the pancreas was CPT1B. Expression in yeast allowed kinetic characterization of the two native enzymes, and of a chimaera in which the distinctive N-terminal segment of ovine M-CPT 1 was replaced with that from rat M-CPT 1. The ovine N-terminal segment influences the kinetics of the enzyme for both its substrates, such that the K (m) for palmitoyl-CoA is decreased and that for carnitine is increased for the chimaera, relative to the parental ovine M-CPT 1.

摘要

所报道的核苷酸序列数据将出现在DDBJ、EMBL、GenBank(R)和GSDB核苷酸序列数据库中;绵羊CPT1A和CPT1B cDNA的序列登录号分别为Y18387和AJ272435,部分脂肪组织和肝脏CPT1A克隆的登录号分别为Y18830和Y18829。单胃动物和反刍动物在脂肪酸和酮体代谢方面存在很大差异。所涉及的关键酶的调节可能也相应不同。肉碱棕榈酰转移酶1(CPT 1)是控制长链脂肪酸β-氧化和肝脏生酮作用的关键位点。此前我们发现绵羊和大鼠肝脏线粒体中的CPT 1动力学存在差异。我们克隆了绵羊CPT 1两种同工型[肝脏型(L-)和肌肉型(M-)]的cDNA,以阐明这些蛋白质及其基因(CPT1A和CPT1B)的结构特征。与其他哺乳动物物种的直系同源物相比,它们推导的氨基酸序列显示出高度保守性,但绵羊M-CPT 1的N端除外。这些差异在牛M-CPT 1中也存在,我们测定了其N端序列。此外,与先前表征的CPT1B基因相比,绵羊CPT1B cDNA的5'端提示了一种不同的启动子结构。Northern印迹分析显示,与其他物种相比,CPT1A和CPT1B转录本在组织分布上存在差异。特别是,绵羊CPT1B mRNA的组织限制性较小,胰腺中的主要转录本是CPT1B。在酵母中的表达使得能够对两种天然酶以及一种嵌合体进行动力学表征,在该嵌合体中,绵羊M-CPT 1独特的N端片段被大鼠M-CPT 1的相应片段所取代。相对于亲本绵羊M-CPT 1,绵羊N端片段影响该酶对其两种底物的动力学,使得嵌合体中棕榈酰辅酶A的K(m)降低,肉碱的K(m)升高。

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