Microaspiration of Solanum tuberosum root cells at early stages of infection by Globodera pallida

Rinu Kooliyottil; Louise-Marie Dandurand; Joseph C. Kuhl; Allan Caplan; Fangming Xiao

doi:10.1186/s13007-017-0219-x

Plant Methods (Aug 2017)

Microaspiration of Solanum tuberosum root cells at early stages of infection by Globodera pallida

Rinu Kooliyottil,
Louise-Marie Dandurand,
Joseph C. Kuhl,
Allan Caplan,
Fangming Xiao

Affiliations

Rinu Kooliyottil: Department of Plant Soil and Entomological Sciences, University of Idaho
Louise-Marie Dandurand: Department of Plant Soil and Entomological Sciences, University of Idaho
Joseph C. Kuhl: Department of Plant Soil and Entomological Sciences, University of Idaho
Allan Caplan: Department of Plant Soil and Entomological Sciences, University of Idaho
Fangming Xiao: Department of Plant Soil and Entomological Sciences, University of Idaho

DOI: https://doi.org/10.1186/s13007-017-0219-x
Journal volume & issue: Vol. 13, no. 1
pp. 1 – 9

Abstract

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Abstract Background Sedentary endoparasitic cyst nematodes form a feeding structure in plant roots, called a syncytium. Syncytium formation involves extensive transcriptional modifications, which leads to cell modifications such as increased cytoplasmic streaming, enlarged nuclei, increased numbers of organelles, and replacement of a central vacuole by many small vacuoles. When whole root RNA is isolated and analyzed, transcript changes manifested in the infected plant cells are overshadowed by gene expression from cells of the entire root system. Use of microaspiration allows isolation of the content of nematode infected cells from a heterogeneous cell population. However, one challenge with this method is identifying the nematode infected cells under the microscope at early stages of infection. This problem was addressed by staining nematode juveniles with a fluorescent dye prior to infection so that the infected cells could be located and microaspirated. Results In the present study, we used the fluorescent vital stain PKH26 coupled with a micro-rhizosphere chamber to locate the infected nematode Globodera pallida in Solanum tuberosum root cells. This enabled microaspiration of nematode-infected root cells during the early stages of parasitism. To study the transcriptional events occurring in these cells, an RNA isolation method from microaspirated samples was optimized, and subsequently the RNA was purified using magnetic beads. With this method, we obtained an RNA quality number of 7.8. For transcriptome studies, cDNA was synthesized from the isolated RNA and assessed by successfully amplifying several pathogenesis related protein coding genes. Conclusion The use of PKH26 stained nematode juveniles enabled early detection of nematode infected cells for microaspiration. To investigate transcriptional changes in low yielding RNA samples, bead-based RNA extraction procedures minimized RNA degradation and provided high quality RNA. This protocol provides a robust procedure to analyze gene expression in nematode-infected cells.

Published in Plant Methods

ISSN: 1746-4811 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Agriculture: Plant culture; Science: Biology (General)
Website: https://plantmethods.biomedcentral.com

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