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Pkd1 regulates immortalized proliferation of renal tubular epithelial cells through p53 induction and JNK activation
Saori Nishio, … , Takeshi Tokuhisa, Toshio Mochizuki
Saori Nishio, … , Takeshi Tokuhisa, Toshio Mochizuki
Published April 1, 2005
Citation Information: J Clin Invest. 2005;115(4):910-918. https://doi.org/10.1172/JCI22850.
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Article Nephrology

Pkd1 regulates immortalized proliferation of renal tubular epithelial cells through p53 induction and JNK activation

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Abstract

Autosomal dominant polycystic kidney disease (ADPKD) is the most common human monogenic genetic disorder and is characterized by progressive bilateral renal cysts and the development of renal insufficiency. The cystogenesis of ADPKD is believed to be a monoclonal proliferation of PKD-deficient (PKD–/–) renal tubular epithelial cells. To define the function of Pkd1, we generated chimeric mice by aggregation of Pkd1–/– ES cells and Pkd1+/+ morulae from ROSA26 mice. As occurs in humans with ADPKD, these mice developed cysts in the kidney, liver, and pancreas. Surprisingly, the cyst epithelia of the kidney were composed of both Pkd1–/– and Pkd1+/+ renal tubular epithelial cells in the early stages of cystogenesis. Pkd1–/– cyst epithelial cells changed in shape from cuboidal to flat and replaced Pkd1+/+ cyst epithelial cells lost by JNK-mediated apoptosis in intermediate stages. In late-stage cysts, Pkd1–/– cells continued immortalized proliferation with downregulation of p53. These results provide a novel understanding of the cystogenesis of ADPKD patients. Furthermore, immortalized proliferation without induction of p53 was frequently observed in 3T3-type culture of mouse embryonic fibroblasts from Pkd1–/– mice. Thus, Pkd1 plays a role in preventing immortalized proliferation of renal tubular epithelial cells through the induction of p53 and activation of JNK.

Authors

Saori Nishio, Masahiko Hatano, Michio Nagata, Shigeo Horie, Takao Koike, Takeshi Tokuhisa, Toshio Mochizuki

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Figure 8

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Outgrowing Pkd1–/– MEFs. (A) The 3T3-type culture of MEFs from Pkd1–/– a...
Outgrowing Pkd1–/– MEFs. (A) The 3T3-type culture of MEFs from Pkd1–/– and wild-type mice. (B) Signaling pathways related to proliferation or apoptosis in Pkd1–/– MEFs. Expression of signal transducers and cell cycle regulators was analyzed using Western blot. Actin was used as a loading control for protein. Data presented are 1 representative of 4 independent experiments.

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