The first 238 amino acids of the human lamin B receptor are targeted to the nuclear envelope in plants

doi:10.1093/jxb/erg102

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Journal of Experimental Botany, Vol. 54, No. 384, pp. 943-950, March 1, 2003
© 2003 Oxford University Press

The first 238 amino acids of the human lamin B receptor are targeted to the nuclear envelope in plants

Received 15 August 2002; Accepted 4 November 2002

Sarah L. Irons, David E. Evans¹^, and Federica Brandizzi

Research School of Biological and Molecular Sciences, Oxford Brookes University, Gipsy Lane, Headington, Oxford OX3 0BP, UK

¹ To whom correspondence should be addressed: Fax: +44 (0)1865 483242. E-mail: deevans{at}brookes.ac.uk
Abbreviations: NE, nuclear envelope; ONE, outer nuclear envelope; INE, inner nuclear envelope; GFP, green fluorescent protein; LBR, lamin B receptor, PLT, progressive lowering of temperature.

In plants, the nuclear envelope (NE) is one of the least characterizedcellular structures. In particular, little is known about itsdynamics during the cell cycle. This is due to the absence ofspecific markers for in vivo studies. To generate such an invivo marker, the suitability of the human lamin B receptor (LBR)was tested. When the first 238 amino acids of the LBR, fusedto the green fluorescent protein (GFP), were expressed in tobaccoplants, fluorescence accumulated only at the NE of leaf epidermalcells. This was confirmed by electron microscopy. The proteinwas shown to be membrane-integral by phase separation. Distributionof fluorescence was compared with two ER markers, GFP-calnexinand GFP-HDEL. While co-localization of all three markers wasnoted at the NE, only LBR-GFP was specific to the NE, whilethe other two also showed fluorescence of the cortical ER. Theseresults suggest that common targeting mechanisms to those inanimals and fungi exist in plants to direct and locate proteinsto the NE. This chimaeric construct is the first available fluorescentintegral membrane protein marker to be targeted exclusivelyto the plant NE and it provides a novel opportunity to investigatethe dynamics of this membrane system in vivo. With it, the cellcycle was followed in tobacco BY-2 cells stably expressing thefusion protein. The interphase labelling of the NE altered inmetaphase into an ER-like meshwork, suggesting the dispersalof the NE to ER as in animal cells. Finally, the meshwork offluorescent membranes was lost and new fluorescent NE formedaround the daughter nuclei.

Key words: GFP, lamin B receptor, membrane targeting, Nicotiana tabacum, nuclear envelope.

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