Nour-Eldin HH , Nørholm MH , Halkier BA .

	Figure 1. Screening for glucose uptake activity in Xenopus oocytes expressing pools of cRNA of Arabidopsis transporter cDNAs. cRNA of 96 genes transcribed with native plant UTRs were pooled in columns and rows and screened for glucose uptake in Xenopus oocytes. High glucose uptake was measured in column 5 and row C, which suggests that the marked well contains a glucose transporter.
	Figure 2. Confirmation of glucose uptake activity by AtSTP13. cRNA of AtSTP13 representing the single clone C5 was injected into nine oocytes. Measurement of glucose uptake by the oocytes was compared to oocytes injected with row C and column 5, respectively.
	Figure 3. Effect of different UTRs on gene expression in Xenopus oocytes. CDSs of AtSTP1, AtSTP4, AtSTP13, AtSUCI, and AtSUC2 were expressed with their native plant UTRs or with Xenopus-specific β-globin gene UTRs. Water injected oocytes functioned as negative controls for endogenous glucose or sucrose uptake by oocytes. Assays were performed with 15 μM radio labelled glucose or sucrose (~100 μCi/μmol).
	Figure 4. Screening for glucose uptake in oocytes expressingpools of cRNA of Arabidopsis transporter cDNAs optimized for Xenopus expression. cRNAs of 96 genes transcribed with Xenopus UTRs were pooled in columns and rows and screened for glucose uptake in oocytes. High glucose uptake was measured in row A, C and E and column 4, 5 and 7, which suggests that the marked wells, contain glucose transporters.

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