FEASIBILITY ANALYSIS OF LEAF DISC SAMPLES PRODUCED VIA AGROINFILTRATION FOR PROMOTER TRAPPING STUDIES

D. Natorajan; H.Y. Yong; I. Ismail; Z. Zainal

doi:10.9755/ejfa.v22i6.4662

Authors

D. Natorajan 1School of Biosciences and Biotechnology, Faculty of Science and Technology, Universiti Kebangsaan Malaysia, Bangi, 43600 Selangor, Malaysia; 2Centre for Plant Biotechnology, Institute of System Biology, Universiti Kebangsaan Malaysia, Bangi, 43600 Selangor, Malaysia; 3Current address: ACGT Sdn Bhd, Technology Park Malaysia, Bukit Jalil, 5700, Kuala Lumpur, Malaysia
H.Y. Yong 1School of Biosciences and Biotechnology, Faculty of Science and Technology, Universiti Kebangsaan Malaysia, Bangi, 43600 Selangor, Malaysia; 2Centre for Plant Biotechnology, Institute of System Biology, Universiti Kebangsaan Malaysia, Bangi, 43600 Selangor, Malaysia; 3Current address: ACGT Sdn Bhd, Technology Park Malaysia, Bukit Jalil, 5700, Kuala Lumpur, Malaysia
I. Ismail 2 Centre for Plant Biotechnology, Institute of System Biology, Universiti Kebangsaan Malaysia, Bangi, 43600 Selangor, Malaysia.
Z. Zainal 2 Centre for Plant Biotechnology, Institute of System Biology, Universiti Kebangsaan Malaysia, Bangi, 43600 Selangor, Malaysia

DOI:

https://doi.org/10.9755/ejfa.v22i6.4662

Keywords:

Agrobacterium tumefaciens, T-DNA insertion, agroinfiltration, non-destructive GUS detection

Abstract

Promoter trapping is a method used to isolate and characterize regulatory regions from genomes by elucidating the expression of a promoterless reporter gene flanked by two transposable elements. The conventional method of promoter trapping requires the generation of stable transformed tissue culture derived plant lines. Nevertheless,this method can be laborious, time consuming and expensive. As an alternative method, leaf disc samples produced via leaf agroinfiltration was employed in this work. A promoter trapping construct named pCAMDIN was created which contains a promoterless GUS (?-glucuronidase) gene flanked by the left and right T-DNA border using pCAMBIA 1301 and pBI 121. Following that,the protocol for agroinfiltration of tomato plants using both direct agroinfiltration and vacuum agroinfiltration was optimized. Non-destructive protocols for detection of GUS genes were tested and optimised. Following that, GUS gene expression was studied and areas which showed expression were isolated by making leaf punches. Analysis was carried out by Southern blotting and T-DNA fingerprinting to determine the gene copy number.