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Sandra Rodrigo Blomqvist, Hilmar Vidarsson, Sharyn Fitzgerald, Bengt R. Johansson, Anna Ollerstam, Russell Brown, A. Erik G. Persson, Göran Bergström, Sven Enerbäck
Published in Volume 113, Issue 11
J Clin Invest. 2004; 113(11):1560–1570 doi:10.1172/JCI20665
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Figure 5

Transcript levels and transcriptional regulation in WT and Foxi1–/–. Northern blot analysis of whole-kidney RNA preparations derived from either WT or Foxi1–/– kidneys (A). While Foxi1, Pds, and AE1 signals are absent in kidney RNA prepared from Foxi1–/– mice, the same levels of ATP6B1 and Kcc4 signals are present in WT and Foxi1–/– RNA preparations. At least three independent animals (for each genotype) were examined for each probe in three independent experiments, with representative results shown. Results shown in A represent RNA from different mice. Transfection assays (B), promoter reporter gene constructs for AE1, and Pds, were transfected to COS-7 cells, together with an FOXI1 expression vector (20 and 40 ng) with or without insert. Reporter gene activity is shown as fold induction relative to an expression vector void of FOXI1 insert.