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Construction of Bacillus thuringiensis labeled recombinant strain and horizontal transfer of its cry1AC10 gene

ZHOU Qin,SUN Ming,LI Lin,YANG Zaiqing,YU Ziniu   

  1. State Laboratory of Agricultural Microbiology,Huazhong Agricultural University, Wuhan 430070,China

  • Received:2003-11-18 Revised:2004-03-02 Online:2005-01-18

Abstract: A recombinant plasmid pBMBZGC10 was obtained by the ligation of gfpcry1Ac10 fusion gene and vector plasmid pAD4412,which was then introduced by gene pulser into acrystalliferous strain CryB,and a recombinant strain CryB(pBMBZGC10)was obtained.Different fermentative solutions of recombinant strain were used for multi-spraying on Brassica pekinesis, Ipomoea aquatica and Lycopersicon esculentum leaves.The results of fluorescent detection and PCR amplification revealed that cry1Ac10 gene did not transfer into indigenous bacteria,actinomyces and fungi in test soil,and could not be detected in roots,stems and leaves of test plants.

Key words: Grass, Life form, Germination rates, Ruderals, Disturbance