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Peer-reviewed

Correction Notice: Single-step Precision Genome Editing in Yeast Using CRISPR-Cas9

AA Azat Akhmetov
JL Jon M Laurent
Jimmy Gollihar Jimmy Gollihar
EG Elizabeth C Gardner
RG Riddhiman K Garge
AE Andrew D Ellington
AK Aashiq H Kachroo
EM Edward M Marcotte

Published: Apr 5, 2020 DOI: 10.21769/BioProtoc.3610 Views: 1646

Reviewed by: Anonymous reviewer(s)

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After official publication of our protocol in bio-protocol (https://bio-protocol.org/e2765), we noted some errors in the protocol and wished to correct the protocol. The edits to be performed are as the following:

  1. The original Figure 1 does not appropriately indicate the generation of the Cas9 transcription unit. The process of how to create a Cas9 transcription unit with suitable promoters, terminators, and connectors has now been included in the new Figure 1. All the transcription units were made in the pYTK095 background, which has also been edited.


    Figure 1. Overview of the CRISPR/Cas9-gRNA expression vector construction process. In the first step Xs and Ys represent the gRNA sequence selected, and BsmBI recognition site is indicated in bold.

  2. Table 2 now shows an additional reaction for generating the transcription unit for the Cas9, as shown in Figure 1. The new Table 2 is attached below.

    Table 2. Golden Gate reaction for making Cas9 and gRNA transcription unit/cassette plasmids with appropriate connectors


  3. Table 3 has also been edited that includes the title and footnote edits. The edits are the following:
    a.The correct cassette plasmids with connectors are indicated in the reagents section.
    b.The volumes of ligase and enzymes have been edited from 0.5 µl to 0.5 - 1 µl.
    c.The Title shows that this plasmid now serves as an expression vector in a yeast cell.
    d.The footnote for the table now indicates the End-On-Ligation step required at the end of the Golden Gate reaction cycle to generate a CEN6-URA-GFP vector.

    Table 3. Golden Gate reaction for making Cas9 and gRNA yeast expression vector

    *Cen6-Ura is constructed by assembling YTK plasmids (008, 047, 073, 074, 081, and 084) using BsaI enzyme and End-ON-Ligation step for the Golden Gate reaction.

References

  1. Akhmetov, A., Laurent, J. M., Gollihar, J., Gardner, E. C., Garge, R. K., Ellington, A. D., Kachroo, A. H. and Marcotte, E. M. (2018). Single-step precision genome editing in yeast using CRISPR-Cas9. Bio-protocol 8(6): e2765.

Article Information

Copyright

Akhmetov et al. This article is distributed under the terms of the Creative Commons Attribution License (CC BY 4.0).

How to cite

Akhmetov, A., Laurent, J. M., Gollihar, J., Gardner, E. C., Garge, R. K., Ellington, A. D., Kachroo, A. H. and Marcotte, E. M. (2020). Correction Notice: Single-step Precision Genome Editing in Yeast Using CRISPR-Cas9. Bio-protocol 10(7): e3610. DOI: 10.21769/BioProtoc.3610.

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