4.8 Article

Ideal Bioorthogonal Reactions Using A Site-Specifically Encoded Tetrazine Amino Acid

Journal

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY
Volume 137, Issue 32, Pages 10044-10047

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/jacs.5b03275

Keywords

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Funding

  1. Direct For Biological Sciences
  2. Div Of Molecular and Cellular Bioscience [1518265] Funding Source: National Science Foundation
  3. Division Of Chemistry
  4. Direct For Mathematical & Physical Scien [1112409] Funding Source: National Science Foundation
  5. NIEHS NIH HHS [P30 ES00210] Funding Source: Medline

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Bioorthogonal reactions for labeling biomolecules in live cells have been limited by slow reaction rates or low component selectivity and stability. Ideal bioorthogonal reactions with high reaction rates, high selectivity, and high stability would allow for stoichiometric labeling of biomolecules in minutes and eliminate the need to wash out excess labeling reagent. Currently, no general method exists for controlled stoichiometric or substoichiometric labeling of proteins in live cells. To overcome this limitation, we developed a significantly improved tetrazine-containing amino acid (Tet-v2.0) and genetically encoded Tet-v2.0 with an evolved aminoacyl-tRNA synthetase/tRNA((CUA)) pair. We demonstrated in cellulo that protein containing Tet-v2.0 reacts selectively with cyclopropane-fused trans-cyclooctene (sTCO) with a bimolecular rate constant of 72,500 +/- 1660 M-1 s(-1) without reacting with other cellular components. This bioorthogonal ligation of Tet-v2.0-protein reacts in cellulo with substoichiometric amounts of sTCO-label fast enough to remove the labeling reagent from media in minutes, thereby eliminating the need to wash out label. This ideal bioorthogonal reaction will enable the monitoring of a larger window of cellular processes in real time.

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