4.6 Article

A versatile Tn7 transposon-based bioluminescence tagging tool for quantitative and spatial detection of bacteria in plants

Journal

PLANT COMMUNICATIONS
Volume 3, Issue 1, Pages -

Publisher

ELSEVIER
DOI: 10.1016/j.xplc.2021.100227

Keywords

plant immunity; bacterial virulence; bioluminescence imaging; Pseudomonas syringae; Arabidopsis thaliana; Marchantia polymorpha

Funding

  1. JST PRESTO [JPMJPR17Q6]
  2. Ritsumeikan Global Innovation Research Organization [19H02960]
  3. Max Planck Society
  4. Deutsche Forschungsgemeinschaft [NA 946/1-1]

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This study developed a bioluminescence-based tool for quantitative and spatial detection of bacteria in plants. By introducing the luxCDABE luciferase operon, bacterial titers in plants can be accurately reported, and it can be applied to various plant pathogenic bacteria. Additionally, these tools can be used to study the effects of plant immunity and bacterial effectors on bacterial growth, and the spatial distribution of bacteria in plant tissues can be observed using bioluminescence imaging.
Investigation of plant-bacteria interactions requires quantification of in planta bacterial titers by means of cumbersome and time-consuming colony-counting assays. Here, we devised a broadly applicable tool for bioluminescence-based quantitative and spatial detection of bacteria in plants. We developed vectors that enable Tn7 transposon-mediated integration of the luxCDABE luciferase operon into a specific genomic location found ubiquitously across bacterial phyla. These vectors allowed for the generation of bioluminescent transformants of various plant pathogenic bacteria from the genera Pseudomonas, Rhizobium (Agrobacte-rium), and Ralstonia. Direct luminescence measurements of plant tissues inoculated with bioluminescent Pseudomonas syringae pv. tomato DC3000 (Pto-lux) reported bacterial titers as accurately as conventional colony-counting assays in Arabidopsis thaliana, Solanum lycopersicum, Nicotiana benthamiana, and Marchantia polymorpha. We further showed the usefulness of our vectors in converting previously generated Pto derivatives to isogenic bioluminescent strains. Importantly, quantitative bioluminescence assays using these Pto-lux strains accurately reported the effects of plant immunity and bacterial effectors on bacterial growth, with a dynamic range of four orders of magnitude. Moreover, macroscopic bioluminescence imaging illuminated the spatial patterns of Pto-lux growth in/on inoculated plant tissues. In conclusion, our vectors offer untapped opportunities to develop bioluminescence-based assays for a variety of plant-bacteria interactions.

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