Site-selective tyrosine bioconjugation via photoredox catalysis for native-to-bioorthogonal protein transformation

被引:102
|
作者
Li, Beryl X. [1 ]
Kim, Daniel K. [1 ]
Bloom, Steven [1 ]
Huang, Richard Y. -C. [2 ]
Qiao, Jennifer X. [3 ]
Ewing, William R. [3 ]
Oblinsky, Daniel G. [4 ]
Scholes, Gregory D. [4 ]
MacMillan, David W. C. [1 ]
机构
[1] Princeton Univ, Merck Ctr Catalysis, Princeton, NJ 08544 USA
[2] Bristol Myers Squibb Co, Pharmaceut Candidate Optimizat Res & Dev, Princeton, NJ USA
[3] Bristol Myers Squibb Co, Discovery Chem Res & Dev, Princeton, NJ USA
[4] Princeton Univ, Dept Chem, Princeton, NJ 08544 USA
基金
美国国家科学基金会;
关键词
AMINO-ACID; FLUORESCENT;
D O I
10.1038/s41557-021-00733-y
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
The growing prevalence of synthetically modified proteins in pharmaceuticals and materials has exposed the need for efficient strategies to enable chemical modifications with high site-selectivity. While genetic engineering can incorporate non-natural amino acids into recombinant proteins, regioselective chemical modification of wild-type proteins remains a challenge. Herein, we use photoredox catalysis to develop a site-selective tyrosine bioconjugation pathway that incorporates bioorthogonal formyl groups, which subsequently allows for the synthesis of structurally defined fluorescent conjugates from native proteins. A water-soluble photocatalyst, lumiflavin, has been shown to induce oxidative coupling between a previously unreported phenoxazine dialdehyde tag and a single tyrosine site, even in the presence of multiple tyrosyl side chains, through the formation of a covalent C-N bond. A variety of native proteins, including those with multiple tyrosines, can successfully undergo both tyrosine-specific and single-site-selective labelling. This technology directly introduces aldehyde moieties onto native proteins, enabling rapid product diversification using an array of well-established bioorthogonal functionalization protocols including the alkyne-azide click reaction.
引用
收藏
页码:902 / +
页数:8
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