A single residue change in the product of the chrysanthemum gene TPL1-2 leads to a failure in its repression of flowering

Plant Sci. 2019 Aug:285:165-174. doi: 10.1016/j.plantsci.2019.04.027. Epub 2019 May 14.

Abstract

The TPL/TPR co-repressor is involved in many plant signaling pathways, including those regulating the switch from vegetative to reproductive growth. Here, a TPL homolog (TPL 1-2) was isolated from chrysanthemum. Its product was found to be deposited in the nucleus. The abundance of TPL1-2 transcript varied across the plant, with its highest level being recorded in the stem apex, and its lowest in the root and stem. In the leaf, the abundance of TPL1-2 transcript was highest at dusk in plants exposed to long days, and at dawn in those exposed to short days. Site-directed mutagenesis was used to induce an N176H mutation in TPL1-2. The constitutive expression in Arabidopsis thaliana of the wild type and the mutated alleles of TPL1-2 had a contrasting effect on flowering time, with the mutant transgene expressors flowering later than the wild type transgene expressors. The flowering-related genes FT, TSF, FUL and AP1 were all more strongly transcribed in the mutant transgene expressors than in the wild type transgene expressors.

Keywords: Constitutive expression; Point mutation; Protein interaction; Protein structure; qRT-PCR.

MeSH terms

  • Arabidopsis
  • Chrysanthemum / genetics*
  • Chrysanthemum / growth & development
  • Chrysanthemum / physiology
  • Flowers / growth & development*
  • Gene Expression Profiling
  • Gene Expression Regulation, Plant / genetics
  • Genes, Plant / genetics*
  • Genes, Plant / physiology
  • Plant Proteins / genetics*
  • Plant Proteins / physiology
  • Plants, Genetically Modified
  • Real-Time Polymerase Chain Reaction
  • Sequence Analysis, DNA
  • Time Factors
  • Two-Hybrid System Techniques

Substances

  • Plant Proteins