UV-LASER adjuvant-surfactant-facilitated delivery of mobile dsRNA to tomato plant vasculature and evidence of biological activity by gene knockdown in the potato psyllid

Neha Thakre; Megan Carver; Jorge R Paredes-Montero; Mosharrof Mondal; Jiahuai Hu; Esmaeil Saberi; Nathaniel Ponvert; Jawwad A Qureshi; Judith K Brown

doi:10.1002/ps.7952

UV-LASER adjuvant-surfactant-facilitated delivery of mobile dsRNA to tomato plant vasculature and evidence of biological activity by gene knockdown in the potato psyllid

Pest Manag Sci. 2024 Apr;80(4):2141-2153. doi: 10.1002/ps.7952. Epub 2024 Jan 19.

Authors

Affiliations

¹ School of Plant Sciences, The University of Arizona, Tucson, AZ, USA.
² Division of Biological Sciences, Section of Cell and Developmental Biology, University of California San Diego, La Jolla, CA, USA.
³ Biology Department, Saginaw Valley State University, University Center, USA.
⁴ Facultad de Ciencias de la Vida, Escuela Superior Politécnica del Litoral, ESPOL, Campus Gustavo Galindo, Guayaquil, Ecuador.
⁵ Department of Entomology and Nematology, IFAS, Southwest Florida Research and Education Center, University of Florida, Immokalee, FL, USA.

PMID: 38146104
DOI: 10.1002/ps.7952

Abstract

Background: Double-stranded RNA (dsRNA) biopesticides are of interest for the abatement of insect vectors of pathogenic bacteria such as 'Candidatus Liberibacter', which infects both its psyllid and plant hosts. Silencing of genes essential for psyllids, or for Liberibacter, is anticipated to lead to mortality or impeded bacterial multiplication. Foliar delivery is preferred for biopesticide application; however, the cuticle impedes dsRNA penetration into the vasculature. Here, conditions were established for wounding tomato leaves using ultraviolet light amplification by stimulated emissions of radiation (UV-LASER) to promote dsRNA penetration into leaves and vasculature.

Results: UV-LASER treatment with application of select adjuvants/surfactants resulted in vascular delivery of 100-, 300- and 600-bp dsRNAs that, in general, were correlated with size. The 100-bp dsRNA required no pretreatment, whereas 300- and 600-bp dsRNAs entered the vasculature after UV-LASER treatment only and UV-LASER adjuvant/surfactant treatment, respectively. Of six adjuvant/surfactants evaluated, plant-derived oil combined with an anionic organosilicon compound performed most optimally. Localization of dsRNAs in the tomato vasculature was documented using fluorometry and fluorescence confocal microscopy. The biological activity of in planta-delivered dsRNA (200-250 bp) was determined by feeding third-instar psyllids on tomato leaves post UV-LASER adjuvant/surfactant treatment, with or without psyllid cdc42- and gelsolin dsRNAs. Gene knockdown was quantified by quantitative, real-time polymerase chain reaction with reverse transcription (RT-qPCR) amplification. At 10 days post the ingestion-access period, knockdown of cdc42 and gelsolin expression was 61% and 56%, respectively, indicating that the dsRNAs delivered to the tomato vasculature were mobile and biologically active.

Conclusion: Results indicated that UV-LASER adjuvant/surfactant treatments facilitated the delivery of mobile, biologically active dsRNA molecules to the plant vasculature. © 2023 The Authors. Pest Management Science published by John Wiley & Sons Ltd on behalf of Society of Chemical Industry.

Keywords: UV-LASER; citrus greening disease; double-stranded RNA; foliar uptake; gene knockdown; surfactants.

MeSH terms

Animals
Gelsolin / genetics
Gelsolin / metabolism
Gene Knockdown Techniques
Hemiptera* / metabolism
Lasers
Plant Diseases / microbiology
RNA Interference
RNA, Double-Stranded / genetics
Solanum lycopersicum* / genetics
Surface-Active Agents / pharmacology
Ultraviolet Rays

Substances

RNA, Double-Stranded
Surface-Active Agents
Gelsolin

Grants and funding

2018-70016-27411/USDA-NIFA CDRE