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. 2025 Apr;23(4):1243-1256.
doi: 10.1111/pbi.14582. Epub 2025 Jan 23.

Jan and mini-Jan, a model system for potato functional genomics

Affiliations

Jan and mini-Jan, a model system for potato functional genomics

Haoyang Xin et al. Plant Biotechnol J. 2025 Apr.

Abstract

Potato (Solanum tuberosum) is the third-most important food crop in the world. Although the potato genome has been fully sequenced, functional genomics research of potato lags behind that of other major food crops, largely due to the lack of a model experimental potato line. Here, we present a diploid potato line, 'Jan,' which possesses all essential characteristics for facile functional genomics studies. Jan exhibits a high level of homozygosity after seven generations of self-pollination. Jan is vigorous, highly fertile and produces tubers with outstanding traits. Additionally, it demonstrates high regeneration rates and excellent transformation efficiencies. We generated a chromosome-scale genome assembly for Jan, annotated its genes and identified syntelogs relative to the potato reference genome assembly DMv6.1 to facilitate functional genomics. To miniaturize plant architecture, we developed two 'mini-Jan' lines with compact and dwarf plant stature through CRISPR/Cas9-mediated mutagenesis targeting the Dwarf and Erecta genes involved in growth. One mini-Jan mutant, mini-JanE, is fully fertile and will permit higher-throughput studies in limited growth chamber and greenhouse space. Thus, Jan and mini-Jan offer a robust model system that can be leveraged for gene editing and functional genomics research in potato.

Keywords: functional genomics; gene editing; genome sequencing; potato.

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Conflict of interest statement

The authors have not declared a conflict of interest.

Figures

Figure 1
Figure 1
Phenotypic characteristics of Jan. (a) Plant architecture. (b) Leaflets from a single compound leaf. (c) Flower. (d) Fruits. (e) Tubers from a single plant grown in a growth chamber.
Figure 2
Figure 2
Allelic representation of DM and M6 in the Jan genome. Blocks of genomic sequence are displayed in 100 kb resolution and are colour‐coded based on parental origin: DM (blue), M6 (gold) or ambiguous (red) due to high sequence conservation between DM and M6.
Figure 3
Figure 3
Diagrams of gRNAs and constructs for CRISPR/Cas9 experiments targeting the StD gene. (a) Illustration of the T‐DNA region of the CRISPR/Cas9 construct. (b) Sequences and positions of the two gRNAs targeting the StD gene. The green‐highlighted ‘AG’ marks the 3′ splicing site within intron 8. PAM sequences are shown in red. Bold letters indicate sequences from exon 9.
Figure 4
Figure 4
Genomic composition and phenotype of mini‐Jan mutants from mutagenesis of the StD gene. (a) A single plant of Jan and four T0 mutants at 48 days after planting in a growth chamber. (b–f) Genomic DNA sequences, cDNA sequences, and predicted protein sequences of Jan (b), mutant i8‐2 (c), mutant e9‐2 (d), mutant i8‐1 (e) and mutant e9‐1 (f). Premature stop codons are highlighted in magenta. The splicing ‘AG’ sites are marked in green. Predicted protein sequences are displayed in blue. The vertical blue line separates exon 9 from intron 8 sequence.
Figure 5
Figure 5
Phenotypes of tissue culture plants of Jan and mini‐Jan. (a) Tissue culture plants of Jan and mini‐JanD after 25 days of culture. (b) Tissue culture plants of Jan and mini‐JanE after 20 days of culture. Note: both mini‐JanD and mini‐JanE exhibit a pronounced dwarf phenotype compared to the wild‐type Jan.
Figure 6
Figure 6
Genomic composition and phenotype of mini‐Jan mutants from mutagenesis of the StER gene. (a) Diagram of the gRNA used for CRISPR/Cas9 experiments targeting the StER gene. (b) Sequences of Jan, er‐1 and er‐2 in the genomic regions associated with mutations of the StER gene. (c) A single plant of Jan, er‐1 and er‐2 at 28 days after planting in a growth chamber. (d) A single plant of Jan, er‐1 and er‐2 at 48 days after planting in a growth chamber. All vertical bars = 20 cm.

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