Abstract
BackgroundForest trees have important economic and ecological value. As a model tree, poplar has played a significant role in elucidating the molecular mechanisms underlying tree biology. However, a lack of mutant libraries and time-consuming stable genetic transformation processes severely limit progress into the functional characterization of poplar genes. A convenient and fast transient transformation method is therefore needed to enhance progress on functional genomics in poplar.MethodsA total of 11 poplar clones were screened for amenability to syringe infiltration. Syringe infiltration was performed on the lower side of the leaves of young soil-grown plants. Transient expression was evaluated by visualizing the reporters β-glucuronidase (GUS) and green fluorescent protein (GFP). The experimental parameters of the syringe agroinfiltration were optimized based on the expression levels of the reporter luciferase (LUC). Stably transformed plants were regenerated from transiently transformed leaf explants through callus-induced organogenesis. The functions of Populus genes in secondary cell wall-thickening were characterized by visualizing lignin deposition therein after staining with basic fuchsin.ResultsWe greatly improved the transient transformation efficiency of syringe Agrobacterium infiltration in poplar through screening for a suitable poplar clone from a variety of clones and optimizing the syringe infiltration procedure. The selected poplar clone, Populus davidiana × P. bolleana, is amenable to Agrobacterium syringe infiltration, as indicated by the easy diffusion of the bacterial suspension inside the leaf tissues. Using this technique, we localized a variety of poplar proteins in specific intracellular organelles and illustrated the protein–protein and protein–DNA interactions. The transiently transformed leaves could be used to generate stably transformed plants with high efficiency through callus induction and differentiation processes. Furthermore, transdifferentiation of the protoxylem-like vessel element and ectopic secondary wall thickening were induced in the agroinfiltrated leaves via the transient overexpression of genes associated with secondary wall formation.ConclusionsThe application of P. davidiana × P. bolleana in Agrobacterium syringe infiltration provides a foundation for the rapid and high-throughput functional characterization of Populus genes in intact poplar plants, including those involved in wood formation, and provides an effective alternative to Populus stable genetic transformation.
Highlights
Forest trees have important economic and ecological value
The application of P. davidiana × P. bolleana in Agrobacterium syringe infiltration provides a foundation for the rapid and high-throughput functional characterization of Populus genes in intact poplar plants, including those involved in wood formation, and provides an effective alternative to Populus stable genetic transformation
Screening of poplar clones for Agrobacterium syringe infiltration To enhance the syringe infiltration method for transient assay in poplar, a total of 11 poplar clones, including four white poplar clones (P. alba var. pyramidalis, i.e., P. bolleana, P. tomentosa ‘BJHR01’, P. tomentosa ‘741’, and P. tomentosa ‘B331’), three aspen or hybrid aspen (P. davidiana, P. alba × glandulosa ‘84 K’, and P. tremula × alba ‘INRA 717-1B4’), one aspen hybrid (P. davidiana × bolleana), two cottonwood (P. euramericana ‘74/76’ and P. trichocarpa), and one P. popularis ‘35–44’, were screened for amenability to syringe infiltration
Summary
Forest trees have important economic and ecological value. As a model tree, poplar has played a significant role in elucidating the molecular mechanisms underlying tree biology. The lack of mutant libraries and the timeconsuming stable genetic transformation process severely limit progress on functional genomics in poplar. A convenient and rapid transient transformation method in poplar is required and will enhance high-throughput functional analyses of Populus genes. The removal of cell walls during protoplast preparation causes an alteration in the subcellular organization of the cytoskeleton and endoplasmic reticulum (ER), which will compromise the experimental results for the proteins localized in these compartments [9]. These limitations in biolistic bombardment and protoplast transformation make Agrobacterium infiltration a preferred method for transient transformation. Agrobacterium infiltration has become the favorable gene delivery method for transient expression in plants [11, 12]
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