Abstract

BackgroundThe establishment of mutant populations together with the strategies for targeted mutation detection has been applied successfully to a large number of organisms including many species in the plant kingdom. Considerable efforts have been invested into research on tomato as a model for berry-fruit plants. With the progress of the tomato sequencing project, reverse genetics becomes an obvious and achievable goal.ResultsHere we describe the treatment of Solanum lycopersicum seeds with 1% EMS and the development of a new mutated tomato population. To increase targeted mutant detection throughput an automated seed DNA extraction has been combined with novel mutation detection platforms for TILLING in plants. We have adapted two techniques used in human genetic diagnostics: Conformation Sensitive Capillary Electrophoresis (CSCE) and High Resolution DNA Melting Analysis (HRM) to mutation screening in DNA pools. Classical TILLING involves critical and time consuming steps such as endonuclease digestion reactions and gel electrophoresis runs. Using CSCE or HRM, the only step required is a simple PCR before either capillary electrophoresis or DNA melting curve analysis. Here we describe the development of a mutant tomato population, the setting up of two polymorphism detection platforms for plants and the results of the first screens as mutation density in the populations and estimation of the false-positives rate when using HRM to screen DNA pools.ConclusionThese results demonstrate that CSCE and HRM are fast, affordable and sensitive techniques for mutation detection in DNA pools and therefore allow the rapid identification of new allelic variants in a mutant population. Results from the first screens indicate that the mutagen treatment has been effective with an average mutation detection rate per diploid genome of 1.36 mutation/kb/1000 lines.

Highlights

  • The establishment of mutant populations together with the strategies for targeted mutation detection has been applied successfully to a large number of organisms including many species in the plant kingdom

  • This optimism was tempered by the complexity of using such mutants in classical breeding practice due to the difficulties in the identification of which mutation in a plant displaying an altered trait was responsible for the phenotype [2]

  • In this paper we present two high throughput technologies that have been adapted to tilling in plants together with the characterization of a large tomato ethyl methanesulfonate (EMS) mutated population

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Summary

Introduction

The establishment of mutant populations together with the strategies for targeted mutation detection has been applied successfully to a large number of organisms including many species in the plant kingdom. Generating new genetic variation by mutagenesis in plants for the unraveling of biological processes and for the alteration of agronomic traits was viewed with great optimism in the mid sixties [1] Later, this optimism was tempered by the complexity of using such mutants in classical breeding practice due to the difficulties in the identification of which mutation in a plant displaying an altered trait was responsible for the phenotype [2]. The development of plant molecular biology and biochemistry has facilitated the identification of individual genes insight into their function using reverse genetic tools such as antisense (PTGS) or RNAi [3-5]. These technologies opened up the possibilities of developing molecular tools for crop improvement. There is no methodological restriction in the technique to model plants and large complex genomes proved amenable to the TILLING process [7-19]

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