Protein subcellular targeting inTrichoderma aggressivum f. aggressivum
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Abstract
Trichoderma aggressivum f. aggressivum is a filamentous soil fungus. Green mold disease
of commercial mushrooms caused by this species in North America has resulted in millions of
dollars in lost revenue within the mushroom growing industry. Research on the molecular level
of T aggressivum have jus t begun with the goal of understanding the functions of each gene and
protein, and their expression control. Protein targeting has not been well studied in this species
yet. Therefore, the intent of this study was to test the protein localization and production levels in
T aggressivum with green fluorescent protein (GFP) with an intron and tagged with either
nuclear localization signal (NLS) or an endoplasmic reticulum retention signal (KDEL). Two
GFP constructs (with and without the intron) were used as controls in this study.
All four constructs were successfully transferred into T aggressivum and all modified strains
showed similar growth characteristics as the wild type non-transformed isolate. GFP expression
was detected from all modified T aggressivum with confocal microscopy and the expression was
similar in all four strains. The intron tested in this study had no or very minor effects as GFP
expression was similar with or without it. The GFP signal increased over a 5 day period for all
transformants, while the GFP to total protein ratio decreased over the same period for all
transformants. The GFP-KDEL transformant showed similar protein expression level and
localization as did the control transformant lacking the KDEL retention signal. The GFP-NLS
transformant similarly failed to localize GFP into nucleus as fluorescence with this strain was
virtually identical to the GFP transformant lacking the NLS. Thus, future research is required to
find effective localization signals for T aggressivum.