Pursuit of chlorovirus genetic transformation and CRISPR/Cas9-mediated gene editing

Eric A Noel; Donald P Weeks; James L Van Etten

doi:10.1371/journal.pone.0252696

Pursuit of chlorovirus genetic transformation and CRISPR/Cas9-mediated gene editing

PLoS One. 2021 Oct 21;16(10):e0252696. doi: 10.1371/journal.pone.0252696. eCollection 2021.

Authors

Eric A Noel^{1

2}, Donald P Weeks³, James L Van Etten^{1

4}

Affiliations

¹ Nebraska Center for Virology, University of Nebraska, Lincoln, Nebraska, United States of America.
² School of Biological Sciences, University of Nebraska, Lincoln, Nebraska, United States of America.
³ Department of Biochemistry, University of Nebraska, Lincoln, Nebraska, United States of America.
⁴ Department of Plant Pathology, University of Nebraska, Lincoln, Nebraska, United States of America.

Abstract

Genetic and molecular modifications of the large dsDNA chloroviruses, with genomes of 290 to 370 kb, would expedite studies to elucidate the functions of both identified and unidentified virus-encoded proteins. These plaque-forming viruses replicate in certain unicellular, eukaryotic chlorella-like green algae. However, to date, only a few of these algal species and virtually none of their viruses have been genetically manipulated due to lack of practical methods for genetic transformation and genome editing. Attempts at using Agrobacterium-mediated transfection of chlorovirus host Chlorella variabilis NC64A with a specially-designed binary vector resulted in successful transgenic cell selection based on expression of a hygromycin-resistance gene, initial expression of a green fluorescence gene and demonstration of integration of Agrobacterium T-DNA. However, expression of the integrated genes was soon lost. To develop gene editing tools for modifying specific chlorovirus CA-4B genes using preassembled Cas9 protein-sgRNA ribonucleoproteins (RNPs), we tested multiple methods for delivery of Cas9/sgRNA RNP complexes into infected cells including cell wall-degrading enzymes, electroporation, silicon carbide (SiC) whiskers, and cell-penetrating peptides (CPPs). In one experiment two independent virus mutants were isolated from macerozyme-treated NC64A cells incubated with Cas9/sgRNA RNPs targeting virus CA-4B-encoded gene 034r, which encodes a glycosyltransferase. Analysis of DNA sequences from the two mutant viruses showed highly targeted nucleotide sequence modifications in the 034r gene of each virus that were fully consistent with Cas9/RNP-directed gene editing. However, in ten subsequent experiments, we were unable to duplicate these results and therefore unable to achieve a reliable system to genetically edit chloroviruses. Nonetheless, these observations provide strong initial suggestions that Cas9/RNPs may function to promote editing of the chlorovirus genome, and that further experimentation is warranted and worthwhile.

Publication types

Research Support, U.S. Gov't, Non-P.H.S.

MeSH terms

Agrobacterium / virology
CRISPR-Associated Protein 9 / genetics*
CRISPR-Cas Systems / genetics*
Chlorella / virology
DNA Viruses / genetics
Electroporation / methods
Gene Editing / methods
Phycodnaviridae / genetics*
Ribonucleoproteins / genetics
Transformation, Genetic / genetics*
Viral Proteins / genetics

Substances

Ribonucleoproteins
Viral Proteins
CRISPR-Associated Protein 9

Grants and funding

This work was funded in part by National Science Foundation Grant 1736030 (JVE) and the National Science Foundation Graduate Research Fellowship Program Grant 250506019500 (EN) (www.nsf.gov). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.