Towards reassigning the rare AGG codon in Escherichia coli. Academic Article

abstract

• The rare AGG codon in Escherichia coli has been reassigned to code non-canonical amino acids (ncAAs) by using the PylRS-tRNA(Pyl)(CCU) pair. When N() -alloc-lysine was used as a PylRS substrate, almost quantitative occupancy of N() -alloc-lysine at an AGG codon site was achieved in minimal medium. ncAAs can be potentially incorporated at the AGG codon with varying efficiencies, depending on their activities towards corresponding enzymes. As AGG is a sense codon, the approach reported here resolves the typical low ncAA incorporation issue that has been associated with ncAA mutagenesis and therefore allows bulk preparation of proteins with site-selectively incorporated ncAAs for applications such as therapeutic protein production.

authors

• Liu, Wenshe

published proceedings

• Chembiochem

altmetric score

• 3.5

author list (cited authors)

• Zeng, Y. u., Wang, W., & Liu, W. R.

citation count

• 39

complete list of authors

• Zeng, Yu||Wang, Wei||Liu, Wenshe R

publication date

• August 2014

publisher

• Wiley  Publisher

published in

• ChemBioChem  Journal

keywords

• Agg Codon
• Agga Codon
• Amino Acids
• Amino Acyl-trna Synthetases
• Codon
• Escherichia Coli
• Genetic Code Expansion
• Molecular Conformation
• Non-canonical Amino Acids
• Sense Codon Reassignment

PubMed Central ID

• 25044341

Digital Object Identifier (DOI)

• 10.1002/cbic.201400075

start page

• 1750

end page

• 1754

volume

• 15

issue

• 12

URL

• http%3A%2F%2Fdx.doi.org%2F10.1002%2Fcbic.201400075