Evaluation of eliciting activity of peptidil prolyl cys/trans isomerase from Pseudonomas fluorescens encapsulated in sodium alginate regarding plant resistance to viral and fungal pahogens

Sophya B Popletaeva; Natalia V Statsyuk; Tatiana M Voinova; Lenara R Arslanova; Anton L Zernov; Anton P Bonartsev; Garina A Bonartseva; Vitaly G Dzhavakhiya

doi:10.3934/microbiol.2018.1.192

Evaluation of eliciting activity of peptidil prolyl cys/trans isomerase from Pseudonomas fluorescens encapsulated in sodium alginate regarding plant resistance to viral and fungal pahogens

AIMS Microbiol. 2018 Mar 12;4(1):192-208. doi: 10.3934/microbiol.2018.1.192. eCollection 2018.

Authors

Sophya B Popletaeva¹, Natalia V Statsyuk², Tatiana M Voinova¹, Lenara R Arslanova¹, Anton L Zernov³, Anton P Bonartsev³, Garina A Bonartseva³, Vitaly G Dzhavakhiya¹

Affiliations

¹ Department of Molecular Biology, All-Russian Research Institute of Phytopathology, Bolshie Vyazemy, Moscow region, 143050, Russia.
² Department of Potato and Vegetable Diseases, All-Russian Research Institute of Phytopathology, Bolshie Vyazemy, Moscow region, 143050, Russia.
³ Federal Research Centre "Fundamentals of Biotechnology" of the Russian Academy of Sciences, Moscow, 119071, Russia.

Abstract

Use of chemical pesticides poses a threat for environment and human health, so green technologies of crop protection are of high demand. Some microbial proteins able to activate plant defense mechanisms and prevent the development of resistance in plant pathogens, may be good alternative to chemicals, but practical use of such elicitors is limited due to need to protect them against adverse environment prior their delivery to target receptors of plant cells. In this study we examined a possibility to encapsulate heat resistant FKBP-type peptidyl prolyl cis-trans isomerase (PPIase) from Pseudomonas fluorescens, which possesses a significant eliciting activity in relation to a range of plant pathogens, in sodium alginate microparticles and evaluated the stability of resulted complex under long-term UV irradiation and in the presence of proteinase K, as well as its eliciting activity in three different "plant-pathogen" models comparing to that of free PPIase. The obtained PPIase-containing microparticles consisted of 70% of sodium alginate, 20% of bovine serum albumin, and 10% of PPIase. In contrast to free PPIase, which lost its eliciting properties after 8-h UV treatment, encapsulated PPIase kept its eliciting ability unchanged; after being exposed to proteinase K, its eliciting ability twice exceeded that of free PPIase. Using "tobacco-TMV", "tobacco-Alternaria longipes", and "wheat-Stagonospora nodorum" model systems, we showed that encapsulation process did not influence on the eliciting activity of PPIase. In the case of the "wheat-S. nodorum" model system, we also observed a significant eliciting activity of alginate-albumin complex and almost doubled activity of encapsulated PPIase as compared to the free PPIase. As far as we know, this is the first observation of a synergistic interaction between alginate and other compound possessing any bioactive properties. The results of the study show some prospects for a PPIase use in agriculture.

Keywords: Alternaria longipes; FKBP-type peptidyl prolyl cis-trans isomerase; PPIase; Stagonospora nodorum; encapsulation; induced resistance of plants; plant pathogens; protein elicitors; sodium alginate; tobacco mosaic virus.