Fig. 8

Construction of recombinant vectors. a: Schematic map of the P_NtGDSL127::GUS recombinant vectors. The promoter fragments were inserted at the HindIII and BamHI sites of PBI121. The GUS gene was driven by the P_NtGDSL127 promoter and the 5′ deletion promoters seperately. b: Agarose gel separation of PCR product of P_NtGDSL127, P_NtGDSL127-A, P_NtGDSL127-B and P_NtGDSL127-C, c: Enzymatic digestion of the recombinant plasmid P_NtGDSL127 and P_NtGDSL127-C using HindIII and BamHI. d: Enzymatic digestion of the recombinant plasmid P_NtGDSL127-A and P_NtGDSL127-B using HindIII and BamHI. 22(P_NtGDSL127::GUS), 25(P_{NtGDSL127-A::}GUS), 27(P_{NtGDSL127-B::}GUS), and 30(P_{NtGDSL127-C::}GUS) independent transformants of each construct were obtained seperately