Abstract

BackgroundPhaseolus vulgaris is one of the most extensively studied model legumes in the world. The P. vulgaris genome sequence is available; therefore, the need for an efficient and rapid transformation system is more imperative than ever. The functional characterization of P. vulgaris genes is impeded chiefly due to the non-amenable nature of Phaseolus sp. to stable genetic transformation. Transient transformation systems are convenient and versatile alternatives for rapid gene functional characterization studies. Hence, the present work focuses on standardizing methodologies for protoplast isolation from multiple tissues and transient transformation protocols for rapid gene expression analysis in the recalcitrant grain legume P. vulgaris.ResultsHerein, we provide methodologies for the high-throughput isolation of leaf mesophyll-, flower petal-, hypocotyl-, root- and nodule-derived protoplasts from P. vulgaris. The highly efficient polyethylene glycol-mannitol magnesium (PEG-MMG)-mediated transformation of leaf mesophyll protoplasts was optimized using a GUS reporter gene. We used the P. vulgaris SNF1-related protein kinase 1 (PvSnRK1) gene as proof of concept to demonstrate rapid gene functional analysis. An RT-qPCR analysis of protoplasts that had been transformed with PvSnRK1-RNAi and PvSnRK1-OE vectors showed the significant downregulation and ectopic constitutive expression (overexpression), respectively, of the PvSnRK1 transcript. We also demonstrated an improved transient transformation approach, sonication-assisted Agrobacterium-mediated transformation (SAAT), for the leaf disc infiltration of P. vulgaris. Interestingly, this method resulted in a 90 % transformation efficiency and transformed 60–85 % of the cells in a given area of the leaf surface. The constitutive expression of YFP further confirmed the amenability of the system to gene functional characterization studies.ConclusionsWe present simple and efficient methodologies for protoplast isolation from multiple P. vulgaris tissues. We also provide a high-efficiency and amenable method for leaf mesophyll transformation for rapid gene functional characterization studies. Furthermore, a modified SAAT leaf disc infiltration approach aids in validating genes and their functions. Together, these methods help to rapidly unravel novel gene functions and are promising tools for P. vulgaris research.Electronic supplementary materialThe online version of this article (doi:10.1186/s12896-016-0283-8) contains supplementary material, which is available to authorized users.

Highlights

  • Phaseolus vulgaris is one of the most extensively studied model legumes in the world

  • We provide a high-efficiency and amenable method for leaf mesophyll transformation for rapid gene functional characterization studies

  • Gene functional analysis To further examine the feasibility of using P. vulgaris leaf mesophyll-derived protoplasts for the functional analysis of the genes, we explored the evolutionarily conserved SnRK1 gene that is known to regulate energy and stress signaling in eukaryotes

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Summary

Introduction

Phaseolus vulgaris is one of the most extensively studied model legumes in the world. Some reports have suggested the feasibility of the stable transformation of common bean using a microprojectile bombardment method [6], this option demands vast resources and intensive work with a miniscule yield compared to the bombardment methods of other model crop plants, including cereals [7]. Such a low efficiency makes this method potentially unusable in small-scale laboratories. This method is a transformation procedure that demands time and it is not eligible for a high-throughput analysis of heterologous gene expression

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