ABSTRACT
Introduction
Materials and methods
Fungal strains
Mycelium preparation, DNA and RNA extraction
Amplification of A3-hox1 and A3-hox2 genes
Co-transformation method
DAPI and Fluorescent Brightener 28 staining andmicroscopic observation
Construction of two plasmid vectors for overexpressionof the A3-hox1 and A3-hox2 genes
Southern hybridization
Real-time PCR assay
Results and discussions
A single introduced hox gene is insufficient to inducetrue clamps in high frequency
Two separated, introduced hox gene increases thefrequency of clamps
Two introduced combined hox gene also increasethe frequency of fused hook cell
Greater expression of the hox genes drive the realclamp formation
Different growth condition was observed in differentkinds of transformants
Different expression amount of four hox gene indifferent kinds of transformants
REFERENCES