Enhanced Directed Evolution in Mammalian Cells Yields a Hyperefficient Pyrrolysyl tRNA for Noncanonical Amino Acid Mutagenesis

Author:

Jewel Delilah1,Kelemen Rachel E.1,Huang Rachel L.1ORCID,Zhu Zeyu2,Sundaresh Bharathi2ORCID,Malley Kaitlin1,Pham Quan1,Loynd Conor1,Huang Zeyi1ORCID,van Opijnen Tim23ORCID,Chatterjee Abhishek1ORCID

Affiliation:

1. Department of Chemistry Boston College 2609 Beacon Street Chestnut Hill MA 02467 USA

2. Department of Biology Boston College Chestnut Hill MA 02467 USA

3. Broad Institute of MIT and Harvard Cambridge MA 02142 USA

Abstract

AbstractHeterologous tRNAs used for noncanonical amino acid (ncAA) mutagenesis in mammalian cells typically show poor activity. We recently introduced a virus‐assisted directed evolution strategy (VADER) that can enrich improved tRNA mutants from naïve libraries in mammalian cells. However, VADER was limited to processing only a few thousand mutants; the inability to screen a larger sequence space precluded the identification of highly active variants with distal synergistic mutations. Here, we report VADER2.0, which can process significantly larger mutant libraries. It also employs a novel library design, which maintains base‐pairing between distant residues in the stem regions, allowing us to pack a higher density of functional mutants within a fixed sequence space. VADER2.0 enabled simultaneous engineering of the entire acceptor stem of M. mazei pyrrolysyl tRNA (tRNAPyl), leading to a remarkably improved variant, which facilitates more efficient incorporation of a wider range of ncAAs, and enables facile development of viral vectors and stable cell‐lines for ncAA mutagenesis.

Funder

Division of Molecular and Cellular Biosciences

National Institute of General Medical Sciences

Division of Microbiology and Infectious Diseases, National Institute of Allergy and Infectious Diseases

Publisher

Wiley

Subject

General Chemistry,Catalysis

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