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在Cat1基因敲除细胞系中,Cat3介导的阳离子氨基酸转运增加在功能上起到了补偿作用。

Increased Cat3-mediated cationic amino acid transport functionally compensates in Cat1 knockout cell lines.

作者信息

Nicholson B, Sawamura T, Masaki T, MacLeod C L

机构信息

San Diego Cancer Center and Department of Medicine, University of California, La Jolla, California 92093-0684, USA.

出版信息

J Biol Chem. 1998 Jun 12;273(24):14663-6. doi: 10.1074/jbc.273.24.14663.

Abstract

Arginine transport is important for a number of biological processes in vertebrates, and its transport may be rate-limiting for the production of nitric oxide. The majority of L-Arg transport is mediated by System y+, although several other carriers have been kinetically defined. System y+ cationic amino acid transport is mediated by proteins encoded by a family of genes, Cat1, Cat2, and Cat3. High affinity L-arginine transport was investigated in embryonic fibroblast cells derived from Cat1 knockout mice that lack functional Cat1. Both wild type and knockout cells transport arginine with comparable Km and Vmax. However, the apparent affinity for lysine transport was 2.4 times lower in Cat1(-/-) cells when compared with wild type cells, a property characteristic of Cat3-mediated transport. Northern analysis-documented Cat2 mRNA increased 2-fold, whereas Cat3 mRNA levels increased 11-fold in Cat1(-/-) relative to Cat1(+/+) cells. The low affinity Cat2a mRNA was not detectably expressed in these cells. Even though Cat3 expression is normally limited to adult brain, there was a large increase in the amount of Cat3 protein present at the plasma membrane of Cat1(-/-) embryonic fibroblast cells. These results suggest that Cat3 compensates for the loss of functional Cat1 in cells derived from Cat1 knockout mice and mediates the majority of high affinity arginine transport.

摘要

精氨酸转运对脊椎动物的许多生物学过程都很重要,其转运可能是一氧化氮生成的限速环节。大多数L-精氨酸的转运由y+系统介导,尽管还通过动力学方法定义了其他几种载体。y+系统阳离子氨基酸转运由一组基因(Cat1、Cat2和Cat3)编码的蛋白质介导。在缺乏功能性Cat1的Cat1基因敲除小鼠来源的胚胎成纤维细胞中研究了高亲和力L-精氨酸转运。野生型和基因敲除细胞转运精氨酸时的Km和Vmax相当。然而,与野生型细胞相比,Cat1(-/-)细胞中赖氨酸转运的表观亲和力低2.4倍,这是Cat3介导转运的特性。Northern分析表明,与Cat1(+/+)细胞相比,Cat1(-/-)细胞中Cat2 mRNA增加了2倍,而Cat3 mRNA水平增加了11倍。在这些细胞中未检测到低亲和力的Cat2a mRNA表达。尽管Cat3的表达通常局限于成年大脑,但在Cat1(-/-)胚胎成纤维细胞的质膜上,Cat3蛋白的量大幅增加。这些结果表明,Cat3补偿了Cat1基因敲除小鼠来源细胞中功能性Cat1的缺失,并介导了大部分高亲和力精氨酸转运。

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