4.7 Article

A modified GFP facilitates counting membrane protein subunits by step-wise photobleaching in Arabidopsis

Journal

JOURNAL OF PLANT PHYSIOLOGY
Volume 213, Issue -, Pages 129-133

Publisher

ELSEVIER GMBH
DOI: 10.1016/j.jplph.2017.03.009

Keywords

Monomeric GFP; VA-TIRFM; Step-wise photobleaching; Subunit counting; Arabidopsis

Categories

Funding

  1. Major Science Foundation of the Ministry of Education of China (111 project) [313008]
  2. Programof Introducing Talents of Discipline to Universities (111 project) [B13007]
  3. National Nature Science Foundation of China [31270224, 31270412]

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Membrane proteins exert functions by forming oligomers or molecular complexes. Currently, step-wise photobleaching has been applied to count the fluorescently labelled subunits in plant cells, for which an accurate and reliable control is required to distinguish individual subunits and define the basal fluorescence. However, the common procedure using immobilized GFP molecules is obviously not applicable for analysis in living plant cells. Using the spatial intensity distribution analysis (SpIDA), we found that the A206K mutation reduced the dimerization of GFP molecules. Further ectopic expression of Myristoyl-GFP(A206K) driven by the endogenous AtCLC2 promoter allowed imaging of individual molecules at a low expression level. As a result, the percentage of dimers in the transgenic pCLC2::Myristoyl-mGFP(A206K) line was significantly reduced in comparison to that of the pCLC2::Myristoyl-GFP line, confirming its application in defining the basal fluorescence intensity of GFP. Taken together, our results demonstrated that pCLC2::Myristoyl-mGFP(A206K) can be used as a standard control for monomer GFP, facilitating the analysis of the step-wise photobleaching of membrane proteins in Arabidopsis thaliana.

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