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Characterisation of CRISPR mutants targeting genes modulating pectin degradation in ripening tomato
Saturday, 2019/01/12 | 05:14:00

Duoduo Wang, Nurul Samsulrizal, Cheng Yan, Natalie S Allcock, Jim Craigon, Barbara Blanco-Ulate, Isabel Ortega-Salazar, Susan E Marcus, Hassan Moeiniyan Bagheri, Laura Perez-Fons, Paul David Fraser, Timothy Foster, Rupert George Fray, J. Paul Knox, Graham B. Seymour

Plant Physiology Published November 2018. DOI: https://doi.org/10.1104/pp.18.01187

ABSTRACT

Tomato (Solanum lycopersicum) is a globally important crop with an economic value in the tens of billions of dollars, and a significant supplier of essential vitamins, minerals and phytochemicals in the human diet. Shelf life is a key quality trait related to alterations in cuticle properties and remodelling of the fruit cell walls. Studies with transgenic tomato plants undertaken over the last 20 years have indicated that a range of pectin degrading enzymes are involved in cell wall remodelling. These studies usually involved silencing of only a single gene and it has proved difficult to compare the effects of silencing these genes across the different experimental systems. Here we report the generation of CRISPR-based mutants in the ripening-related genes encoding the pectin degrading enzymes pectate lyase (PL), polygalacturonase 2a (PG2a) and β-galactanase (TBG4). Comparison of the physiochemical properties of the fruits from a range of PL, PG2a and TBG4 CRISPR lines demonstrated that only mutations in PL resulted in firmer fruits, although mutations in PG2a and TBG4 influenced fruit colour and weight. Pectin localisation, distribution and solubility in the pericarp cells of the CRISPR mutant fruits were investigated using the monoclonal antibody probes LM19 to de-esterified homogalacturonan (HG), INRA-RU1 to rhamnogalacturonan I, LM5 to β1-4-galactan and LM6 to arabinan epitopes, respectively. The data indicate that PL, PG2a and TBG4 act on separate cell wall domains and the importance of cellulose microfibril-associated pectin is reflected in its increased occurrence in the different mutant lines.

 

See: http://www.plantphysiol.org/content/early/2018/11/20/pp.18.01187

Figure 1: Generation of a range of CRISPR alleles in PL, PG2a and TBG4. The mutations generated in specific regions of gene coding sequences are shown. The region for the single guide RNA sequences are in red and insertions in blue. Deletions are indicated by a dotted line. The PAM site is show in yellow.

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