SILEC:一种生成和使用同位素标记辅酶 A 质谱标准品的方案。
SILEC: a protocol for generating and using isotopically labeled coenzyme A mass spectrometry standards.
机构信息
Centers of Excellence in Environmental Toxicology and Cancer Pharmacology, Perelman School of Medicine at the University of Pennsylvania, Philadelphia, USA.
出版信息
Nat Protoc. 2011 Dec 8;7(1):1-12. doi: 10.1038/nprot.2011.421.
Abstract
Stable isotope labeling by essential nutrients in cell culture (SILEC) was recently developed to generate isotopically labeled coenzyme A (CoA) and short-chain acyl-CoA thioesters. This was accomplished by modifying the widely used technique of stable isotope labeling by amino acids in cell culture to include [(13)C(3)(15)N]-pantothenate (vitamin B(5)), a CoA precursor, instead of the isotopically labeled amino acids. The lack of a de novo pantothenate synthesis pathway allowed for efficient and near-complete labeling of the measured CoA species. This protocol provides a step-by-step approach for generating stable isotope-labeled short-chain acyl-CoA internal standards in mammalian and insect cells as well as instructions on how to use them in stable isotope dilution mass spectrometric-based analyses. Troubleshooting guidelines, as well as a list of unlabeled and labeled CoA species, are also included. This protocol represents a prototype for generating stable isotope internal standards from labeled essential nutrients such as pantothenate. The generation and use of SILEC standards takes approximately 2-3 weeks.
摘要
稳定同位素标记的必需营养物在细胞培养中的应用(SILEC)最近被开发出来,用于生成同位素标记的辅酶 A(CoA)和短链酰基辅酶 A 硫酯。这是通过修改广泛使用的稳定同位素标记的氨基酸在细胞培养中的技术来实现的,包括[(13)C(3)(15)N]-泛酸盐(维生素 B(5)),一种 CoA 前体,而不是同位素标记的氨基酸。由于缺乏从头合成泛酸盐的途径,使得所测量的 CoA 物种能够得到高效且近乎完全的标记。该方案提供了在哺乳动物和昆虫细胞中生成稳定同位素标记的短链酰基辅酶 A 内标物的分步方法,以及如何在基于稳定同位素稀释质谱的分析中使用它们的说明。还包括故障排除指南以及未标记和标记 CoA 物质的列表。该方案代表了从标记的必需营养素(如泛酸盐)生成稳定同位素内标的原型。SILEC 标准品的生成和使用大约需要 2-3 周的时间。
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