Plasmodiophora brassicae-Triggered Cell Enlargement and Loss of Cellular Integrity in Root Systems Are Mediated by Pectin Demethylation

Karolina Stefanowicz; Monika Szymanska-Chargot; William Truman; Piotr Walerowski; Marcin Olszak; Adam Augustyniak; Arkadiusz Kosmala; Artur Zdunek; Robert Malinowski

doi:10.3389/fpls.2021.711838

Plasmodiophora brassicae-Triggered Cell Enlargement and Loss of Cellular Integrity in Root Systems Are Mediated by Pectin Demethylation

Front Plant Sci. 2021 Jul 29:12:711838. doi: 10.3389/fpls.2021.711838. eCollection 2021.

Authors

Karolina Stefanowicz¹, Monika Szymanska-Chargot², William Truman¹, Piotr Walerowski¹, Marcin Olszak³, Adam Augustyniak⁴, Arkadiusz Kosmala¹, Artur Zdunek², Robert Malinowski¹

Affiliations

¹ Institute of Plant Genetics, Polish Academy of Sciences, Poznan, Poland.
² Institute of Agrophysics, Polish Academy of Sciences, Lublin, Poland.
³ Institute of Biochemistry and Biophysics, Polish Academy of Sciences, Warsaw, Poland.
⁴ Centre for Advanced Technology, Adam Mickiewicz University, Poznan, Poland.

Abstract

Gall formation on the belowground parts of plants infected with Plasmodiophora brassicae is the result of extensive host cellular reprogramming. The development of these structures is a consequence of increased cell proliferation followed by massive enlargement of cells colonized with the pathogen. Drastic changes in cellular growth patterns create local deformities in the roots and hypocotyl giving rise to mechanical tensions within the tissue of these organs. Host cell wall extensibility and recomposition accompany the growth of the gall and influence pathogen spread and also pathogen life cycle progression. Demethylation of pectin within the extracellular matrix may play an important role in P. brassicae-driven hypertrophy of host underground organs. Through proteomic analysis of the cell wall, we identified proteins accumulating in the galls developing on the underground parts of Arabidopsis thaliana plants infected with P. brassicae. One of the key proteins identified was the pectin methylesterase (PME18); we further characterized its expression and conducted functional and anatomic studies in the knockout mutant and used Raman spectroscopy to study the status of pectin in P. brassicae-infected galls. We found that late stages of gall formation are accompanied with increased levels of PME18. We have also shown that the massive enlargement of cells colonized with P. brassicae coincides with decreases in pectin methylation. In pme18-2 knockout mutants, P. brassicae could still induce demethylation; however, the galls in this line were smaller and cellular expansion was less pronounced. Alteration in pectin demethylation in the host resulted in changes in pathogen distribution and slowed down disease progression. To conclude, P. brassicae-driven host organ hypertrophy observed during clubroot disease is accompanied by pectin demethylation in the extracellular matrix. The pathogen hijacks endogenous host mechanisms involved in cell wall loosening to create an optimal cellular environment for completion of its life cycle and eventual release of resting spores facilitated by degradation of demethylated pectin polymers.

Keywords: Arabidopsis thaliana; Plasmodiophora brassicae; cell enlargement; cell wall; clubroot disease.