A Traceable DNA-Replicon Derived Vector to Speed Up Gene Editing in Potato: Interrupting Genes Related to Undesirable Postharvest Tuber Traits as an Example

Giovana Acha; Ricardo Vergara; Marisol Muñoz; Roxana Mora; Carlos Aguirre; Manuel Muñoz; Julio Kalazich; Humberto Prieto

doi:10.3390/plants10091882

A Traceable DNA-Replicon Derived Vector to Speed Up Gene Editing in Potato: Interrupting Genes Related to Undesirable Postharvest Tuber Traits as an Example

Plants (Basel). 2021 Sep 10;10(9):1882. doi: 10.3390/plants10091882.

Authors

Giovana Acha¹, Ricardo Vergara², Marisol Muñoz², Roxana Mora², Carlos Aguirre², Manuel Muñoz³, Julio Kalazich⁴, Humberto Prieto²

Affiliations

¹ Programa de Doctorado en Biotecnología, Universidad de Santiago, Santiago 9170020, Chile.
² Laboratorio de Biotecnología, Instituto de Investigaciones Agropecuarias-La Platina, Santiago 8831314, Chile.
³ Instituto de Investigaciones Agropecuarias-Remehue, Osorno 5290000, Chile.
⁴ Carrera de Agronomía, Campus Osorno, Universidad de Los Lagos, Osorno 5290000, Chile.

Abstract

In potato (Solanum tuberosum L.), protoplast techniques are limited to a few genotypes; thus, the use of regular regeneration procedures of multicellular explants causes us to face complexities associated to CRISPR/Cas9 gene editing efficiency and final identification of individuals. Geminivirus-based replicons contained in T-DNAs could provide an improvement to these procedures considering their cargo capability. We built a Bean yellow dwarf virus-derived replicon vector, pGEF-U, that expresses all the editing reagents under a multi-guide RNA condition, and the Green Fluorescent Protein (GFP) marker gene. Agrobacterium-mediated gene transfer experiments were carried out on 'Yagana-INIA', a relevant local variety with no previous regeneration protocol. Assays showed that pGEF-U had GFP transient expression for up to 10 days post-infiltration when leaf explants were used. A dedicated potato genome analysis tool allowed for the design of guide RNA pairs to induce double cuts of genes associated to enzymatic browning (StPPO1 and 2) and to cold-induced sweetening (StvacINV1 and StBAM1). Monitoring GFP at 7 days post-infiltration, explants led to vector validation as well as to selection for regeneration (34.3% of starting explants). Plant sets were evaluated for the targeted deletion, showing individuals edited for StPPO1 and StBAM1 genes (1 and 4 lines, respectively), although with a transgenic condition. While no targeted deletion was seen in StvacINV1 and StPPO2 plant sets, stable GFP-expressing calli were chosen for analysis; we observed different repair alternatives, ranging from the expected loss of large gene fragments to those showing punctual insertions/deletions at both cut sites or incomplete repairs along the target region. Results validate pGEF-U for gene editing coupled to regular regeneration protocols, and both targeted deletion and single site editings encourage further characterization of the set of plants already generated.

Keywords: CRISPR/Cas9; agrobacterium-mediated transformation; geminivirus replicons; genome editing; green fluorescent protein; potato.

Abstract

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