Genetic Encoding of Caged Cysteine and Caged Homocysteine in Bacterial and Mammalian Cells

被引:59
作者
Uprety, Rajendra [1 ]
Luo, Ji [2 ]
Liu, Jihe [2 ]
Naro, Yuta [2 ]
Samanta, Subhas [2 ]
Deiters, Alexander [1 ,2 ]
机构
[1] N Carolina State Univ, Dept Chem, Raleigh, NC 27695 USA
[2] Univ Pittsburgh, Dept Chem, Pittsburgh, PA 15260 USA
基金
美国国家科学基金会;
关键词
amino acids; caged compounds; cysteine; gene technology; homocysteine; protein modifications; TRANSFER-RNA SYNTHETASE; CONFORMATIONAL STATES; PHOTOCHEMICAL CONTROL; ACTIVE-SITE; AMINO-ACIDS; PROTEIN; LUCIFERASE; EXPRESSION; DESIGN; CODE;
D O I
10.1002/cbic.201400073
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
We report the genetic incorporation of caged cysteine and caged homocysteine into proteins in bacterial and mammalian cells. The genetic code of these cells was expanded with an engineered pyrrolysine tRNA/tRNA synthetase pair that accepts both light-activatable amino acids as substrates. Incorporation was validated by reporter assays, western blots, and mass spectrometry, and differences in incorporation efficiency were explained by molecular modeling of synthetase-amino acid interactions. As a proof-of-principle application, the genetic replacement of an active-site cysteine residue with a caged cysteine residue in Renilla luciferase led to a complete loss of enzyme activity; however, upon brief exposure to UV light, a >150-fold increase in enzymatic activity was observed, thus showcasing the applicability of the caged cysteine in live human cells. A simultaneously conducted genetic replacement with homocysteine yielded an enzyme with greatly reduced activity, thereby demonstrating the precise probing of a protein active site. These discoveries provide a new tool for the optochemical control of protein function in mammalian cells and expand the set of genetically encoded unnatural amino acids.
引用
收藏
页码:1793 / 1799
页数:7
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