Lowe syndrome patient fibroblasts display Ocrl1-specific cell migration defects that cannot be rescued by the homologous Inpp5b phosphatase

doi:10.1093/hmg/ddp407

Human Molecular Genetics Advance Access originally published online on August 21, 2009
Human Molecular Genetics 2009 18(23):4478-4491; doi:10.1093/hmg/ddp407

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Lowe syndrome patient fibroblasts display Ocrl1-specific cell migration defects that cannot be rescued by the homologous Inpp5b phosphatase

Brian G. Coon¹^,2, Debarati Mukherjee¹^,2, Claudia B. Hanna¹^,2, David J. Riese, II², Martin Lowe³ and R. Claudio Aguilar¹^,2^,*

¹ Department of Biological Sciences and ² Purdue Center for Cancer Research, Purdue University, West Lafayette, IN 47907, USA and ³ Faculty of Life Sciences, University of Manchester, Manchester M13 9PT, UK

^* To whom correspondence should be addressed. +1 7654963547; Fax: +1 7654961496; Email: claudio{at}purdue.edu

Received May 20, 2009; Revised July 24, 2009; Accepted August 20, 2009

The Lowe syndrome (LS) is a life-threatening, developmentaldisease characterized by mental retardation, cataracts and renalfailure. Although this human illness has been linked to defectivefunction of the phosphatidylinositol 5-phosphatase, Ocrl1 (Oculo-Cerebro-Renalsyndrome of Lowe protein 1), the mechanism by which this enzymedeficiency triggers the disease is not clear. Ocrl1 is knownto localize mainly to the Golgi apparatus and endosomes, howeverit translocates to plasma membrane ruffles upon cell stimulationwith growth factors. The functional implications of this inducibletranslocation to the plasma membrane are presently unknown.Here we show that Ocrl1 is required for proper cell migration,spreading and fluid-phase uptake in both established cell linesand human dermal fibroblasts. We found that primary fibroblastsfrom two patients diagnosed with LS displayed defects in thesecellular processes. Importantly, these abnormalities were suppressedby expressing wild-type Ocrl1 but not by a phosphatase-deficientmutant. Interestingly, the homologous human PI-5-phosphatase,Inpp5b, was unable to complement the Ocrl1-dependent cell migrationdefect. Further, Ocrl1 variants that cannot bind the endocyticadaptor AP2 or clathrin, like Inpp5b, were less apt to rescuethe migration phenotype. However, no defect in membrane recruitmentof AP2/clathrin or in transferrin endocytosis by patient cellswas detected. Collectively, our results suggest that Ocrl1,but not Inpp5b, is involved in ruffle-mediated membrane remodeling.Our results provide new elements for understanding how Ocrl1deficiency leads to the abnormalities associated with the LS.

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