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Fig. 1. Detailed genomic structure characterization of the T-DNA inserts in
transgenic Arabidopsis thaliana line EL702C. (a) Schematic construct
map of the T-DNA region in the binary vector pEL702. The plasmid was designed
such that the DNA between the right and left borders (T-DNA) can be
transferred into plant nuclei via Agrobacterium. Thus, when stable
transgenic Arabidopsis plants are treated with the synthetic
glucocorticoid dexamethasone (Dex), the expressed fusion proteins can localize
to the integrated loci by association with the lac operator array.
The numbers on the top indicate the size of DNA construct in kbp. The arrow
indicates the orientation of T-DNA from the left border to right border.
Colored areas indicate gene expression cassette: blue, glucocorticoid receptor
expression; yellow, hygromycin phosphotransferase expression; green,
GFP-LacI/NLS induced expression. Abbreviations and symbols: blue dot
rectangle, pea rbcS-E9 terminator; blue triangle, cauliflower mosaic virus 35S
promoter; green dot rectangle, pea rbcS-3A terminator; green rectangle, 6XGal4
UAS and TATA box; yellow dot rectangle, nopaline-synthase gene terminator;
yellow triangle, nopaline-synthase gene promoter; GVG, glucocorticoid binding
domain/VP16 acidic activation domain/Gal4 DNA-binding domain; HPT, hygromycin
phosphotransferase; LacO, 256mer of lac operator arrays; LB,
left border; RB, right border. (b) Molecular characterization of the
integrated loci with T-DNAs. The number of integrated loci was first
characterized by Southern blot analyses, and the borders of the insertion
sites were subsequently defined by subcloning and sequencing of the respective
regions for the different sites using various strategies. The solid circle
indicates the location of the centromere. The entire length of the chromosome
and the distance between the two insertion loci are indicated in Mbp. Arrows
indicate the direction of T-DNAs from LB to RB. Shaded rectangles represent
neighboring reading frames around the T-DNA inserts.
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