Synthetic yeast chromosome XI design enables extrachromosomal circular DNA formation on demand

Author:

Blount Benjamin AORCID,Lu Xinyu,Driessen Maureen R M,Jovicevic Dejana,Sanchez Mateo IORCID,Ciurkot Klaudia,Zhao YuORCID,Lauer StephanieORCID,McKiernan Robert M,Gowers Glen-Oliver FORCID,Sweeney Fiachra,Fanfani ViolaORCID,Lobzaev EvgeniiORCID,Palacios-Flores KimORCID,Walker RoyORCID,Hesketh AndyORCID,Oliver Stephen GORCID,Cai YizhiORCID,Stracquadanio GiovanniORCID,Mitchell Leslie AORCID,Bader Joel SORCID,Boeke Jef DORCID,Ellis TomORCID

Abstract

SummaryWe describe construction of the 660 kilobase synthetic yeast chromosome XI (synXI) and reveal how synthetic redesign of non-coding DNA elements impact the cell. To aid construction from synthesized 5 to 10 kilobase DNA fragments, we implemented CRISPR-based methods for synthetic crossovers in vivo and used these methods in an extensive process of bug discovery, redesign and chromosome repair, including for the precise removal of 200 kilobases of unexpected repeated sequence. In synXI, the underlying causes of several fitness defects were identified as modifications to non-coding DNA, including defects related to centromere function and mitochondrial activity that were subsequently corrected. As part of synthetic yeast chromosome design, loxPsym sequences for Cre-mediated recombination are inserted between most genes. Using the GAP1 locus from chromosome XI, we show here that targeted insertion of these sites can be used to create extrachromosomal circular DNA on demand, allowing direct study of the effects and propagation of these important molecules. Construction and characterization of synXI has uncovered effects of non-coding and extrachromosomal circular DNA, contributing to better understanding of these elements and informing future synthetic genome design.

Publisher

Cold Spring Harbor Laboratory

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