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NO 供体对大鼠胚胎成纤维细胞 3Y1 细胞中细胞蛋白的 S-亚硝基化作用:影响 S-亚硝基化的因素。

S-nitrosation of cellular proteins by NO donors in rat embryonic fibroblast 3Y1 cells: factors affecting S-nitrosation.

机构信息

Department of Applied Biological Science, Faculty of Science and Technology, Tokyo University of Science, 2641 Yamazaki, Noda, Chiba, Japan.

出版信息

Oxid Med Cell Longev. 2011;2011:450317. doi: 10.1155/2011/450317. Epub 2011 Aug 17.

Abstract

The mechanism of protein S-nitrosation in cells is not fully understood. Using rat 3Y1 cells, we addressed this issue. Among S-nitrosothiols and NO donors tested, only S-nitrosocysteine (CysNO) induced S-nitrosation when exposed in Hanks' balanced salt solution (HBSS) and not in serum-containing general culture medium. In HBSS, NO release from CysNO was almost completely abolished by sequestering metal ions with a metal chelator without affecting cellular S-nitrosation. In contrast, L-leucine, a substrate of L-type amino acid transporters (LATs), significantly inhibited S-nitrosation. The absence of S-nitrosation with CysNO in general culture medium resulted not only from a competition with amino acids in the medium for LATs but also from transnitrosation of cysteine residues in serum albumin. Collectively, these results suggest that in simple buffered saline, CysNO-dependent S-nitrosation occurs through a cellular incorporation-dependent mechanism, but if it occurs in general culture media, it may be through an NO-dependent mechanism.

摘要

细胞中蛋白质 S-亚硝基化的机制尚未完全阐明。我们使用大鼠 3Y1 细胞对此问题进行了研究。在所测试的 S-亚硝基硫醇和 NO 供体中,只有 S-亚硝基半胱氨酸(CysNO)在 Hanks 平衡盐溶液(HBSS)中暴露时会诱导 S-亚硝基化,而在含有血清的普通培养基中则不会。在 HBSS 中,用金属螯合剂螯合金属离子几乎完全消除了 CysNO 从 NO 的释放,但不影响细胞 S-亚硝基化。相比之下,L-亮氨酸,L 型氨基酸转运体(LATs)的底物,显著抑制 S-亚硝基化。CysNO 在普通培养基中没有 S-亚硝基化不仅是由于与培养基中的氨基酸竞争 LATs,还由于血清白蛋白中半胱氨酸残基的转亚硝基化。综上所述,这些结果表明,在简单的缓冲盐溶液中,CysNO 依赖性 S-亚硝基化通过细胞依赖的摄取机制发生,但如果它发生在普通培养基中,则可能通过 NO 依赖的机制发生。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bd52/3163492/f850d4fefcef/OXIMED2011-450317.001.jpg

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