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丹吉尔病载脂蛋白A-I基因的序列与表达

Sequence and expression of Tangier apoA-I gene.

作者信息

Makrides S C, Ruiz-Opazo N, Hayden M, Nussbaum A L, Breslow J L, Zannis V I

机构信息

Department of Medicine, Boston University Medical Center, Massachusetts 02118.

出版信息

Eur J Biochem. 1988 Apr 15;173(2):465-71. doi: 10.1111/j.1432-1033.1988.tb14022.x.

Abstract

We have isolated and characterized the apoA-I gene from a lambda L47.1 genomic library constructed with DNA obtained from the lymphocytes of a Tangier disease patient. The DNA-derived protein sequence of Tangier apoA-I was found to be identical to normal apoA-I. Transfection of mouse C127 cells with a recombinant vector containing the Tangier apoA-I gene (pSV2-gpt apoA-I) allowed selection of stable clones resistant to aminopterin and mycophenolic acid. Analysis of these clones for apoA-I synthesis showed that the protein secreted by cells expressing the Tangier apoA-I gene was indistinguishable from the apoA-I secreted by HepG2 cells. These experiments establish that the Tangier apoA-I gene is structurally normal. It appears that the molecular basis of Tangier disease is not related to apoA-I structure or regulation of expression, but rather to other factors pertinent to apoA-I and high-density lipoprotein metabolism.

摘要

我们从用一名Tangier病患者淋巴细胞的DNA构建的λL47.1基因组文库中分离并鉴定了载脂蛋白A-I(apoA-I)基因。发现Tangier apoA-I的DNA衍生蛋白序列与正常apoA-I相同。用含有Tangier apoA-I基因的重组载体(pSV2-gpt apoA-I)转染小鼠C127细胞,可筛选出对氨基蝶呤和霉酚酸有抗性的稳定克隆。对这些克隆进行apoA-I合成分析表明,表达Tangier apoA-I基因的细胞分泌的蛋白与HepG2细胞分泌的apoA-I无法区分。这些实验证明Tangier apoA-I基因在结构上是正常的。看来,Tangier病的分子基础与apoA-I的结构或表达调控无关,而是与apoA-I和高密度脂蛋白代谢相关的其他因素有关。

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