CREEPY: CRISPR-mediated editing of synthetic episomes in yeast

Author:

Zhao Yu1ORCID,Coelho Camila1ORCID,Lauer Stephanie1ORCID,Majewski Miłosz12ORCID,Laurent Jon M1ORCID,Brosh Ran1ORCID,Boeke Jef D134ORCID

Affiliation:

1. Institute for Systems Genetics, NYU Langone Health , New York , NY 10016 , USA

2. Maastricht Science Programme, Maastricht University , Maastricht 6200 MD , The Netherlands

3. Department of Biochemistry and Molecular Pharmacology, NYU Langone Health , New York , NY 10016 , USA

4. Department of Biomedical Engineering, NYU Tandon School of Engineering , Brooklyn , NY 11201, USA

Abstract

Abstract Use of synthetic genomics to design and build ‘big’ DNA has revolutionized our ability to answer fundamental biological questions by employing a bottom-up approach. Saccharomyces cerevisiae, or budding yeast, has become the major platform to assemble large synthetic constructs thanks to its powerful homologous recombination machinery and the availability of well-established molecular biology techniques. However, introducing designer variations to episomal assemblies with high efficiency and fidelity remains challenging. Here we describe CRISPR Engineering of EPisomes in Yeast, or CREEPY, a method for rapid engineering of large synthetic episomal DNA constructs. We demonstrate that CRISPR editing of circular episomes presents unique challenges compared to modifying native yeast chromosomes. We optimize CREEPY for efficient and precise multiplex editing of >100 kb yeast episomes, providing an expanded toolkit for synthetic genomics.

Funder

NIH

NHGRI

Publisher

Oxford University Press (OUP)

Subject

Genetics

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