Plasmid Construction Using USER and KLD

All plasmids for this study were created using either USER cloning or KLD cloning as described previously^{1 (link)}. DNA was amplified using PhusionU Green Multiplex PCR Master Mix (Thermo Fisher Scientific). Mach1 (Invitrogen) or Turbo (New England BioLabs) chemically competent E. coli were used for plasmid construction.

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Doman J.L., Raguram A., Newby G.A, & Liu D.R. (2020). Evaluation and Minimization of Cas9-Independent Off-Target DNA Editing by Cytosine Base Editors. Nature biotechnology, 38(5), 620-628.

Publication 2020

PhusionU Green Multiplex PCR Master Mix Mach1

E coli Multiplex pcr Plasmid

Corresponding Organization :

Other organizations : Broad Institute

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Variable analysis

independent variables

Cloning method: USER cloning or KLD cloning

dependent variables

Not explicitly mentioned

control variables

DNA amplification using PhusionU Green Multiplex PCR Master Mix (Thermo Fisher Scientific)
Bacterial strains used for plasmid construction: Mach1 (Invitrogen) or Turbo (New England BioLabs) chemically competent E. coli

controls

Positive control: Not specified
Negative control: Not specified

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