Issue 9, 2005

Use of GFP tags to monitor localization of different luciferases in E. coli

Abstract

The utility of the green fluorescent protein (GFP) as a probe to monitor protein localization in living cells is gaining a great deal of attention. In this study, to understand the localization of luciferases in E. coli, we have attached GFP tags at both the N- and the C-terminus of firefly luciferase (FF-Luc) (from Pyrocoelia miyako) and of red (RE-Luc) and green (GR-Luc) bioluminescence-emitting luciferases (from Phrixothrix railroad-worms), respectively. There was no significant change in the bioluminescence emission spectrum for any of the three luciferases following the tagging with GFP at either the N- or C-terminus, confirming the absence of energy transfer between one another. Using confocal imaging microscopy, we observed that all three luciferases expressed in the E.coli cultured at 37 °C tend to aggregate and are seen to localize in the poles, thus confirming their poor folding properties. In contrast, in the E.coli cultured at 18 °C FF-Luc was found to be highly expressed in the soluble form when compared to RE-Luc and GR-Luc. These results support our previous finding that the folding properties of FF-Luc and RE/GR-Luc are totally different.

Graphical abstract: Use of GFP tags to monitor localization of different luciferases in E. coli

Article information

Article type
Paper
Submitted
03 Nov 2004
Accepted
22 Apr 2005
First published
09 Jun 2005

Photochem. Photobiol. Sci., 2005,4, 740-743

Use of GFP tags to monitor localization of different luciferases in E. coli

B. Venkatesh, M. Arifuzzaman, H. Mori, S. Suzuki, T. Taguchi and Y. Ohmiya, Photochem. Photobiol. Sci., 2005, 4, 740 DOI: 10.1039/B416747C

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