Differential Expression of Cyclin D1 in the Human Hair Follicle

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Differential Expression of Cyclin D1 in the Human Hair Follicle

Xiaowei Xu^*, Stephen Lyle, Yaping Liu, Benjamin Solky and George Cotsarelis

From the Departments of Pathology^* and Dermatology, Hospital of University of Pennsylvania, Philadelphia, Pennsylvania; and the Departments of Pathology and Dermatology, Harvard Medical School, Boston, Massachusetts

The proliferation of keratinocytes in the hair follicle variesfrom slowly cycling, intermittently proliferating stem cellsin the bulge to rapidly proliferating, transient cells in thebulb. To better understand the biological differences betweenthese two compartments, we sought to identify differentiallyexpressed genes using cDNA macroarray analysis. Cyclin D1 wasone of 13 genes increased in the bulge compared to the bulb,and its differential expression was corroborated by quantitativereal-time polymerase chain reaction (PCR) on the original samples.Using immunohistochemical staining, laser-capture microdissection(LCM) and quantitative real-time PCR, we localized cyclin D1to the suprabasal cells of the telogen bulge and anagen outerroot sheath (ORS). Surprisingly, cyclin D1, D2, and D3 werenot detectable by immunohistochemistry in the rapidly proliferatinghair-producing cells of the anagen bulb (matrix cells), whilethese cells were strongly positive for Ki-67 and retinoblastomaprotein. In contrast, pilomatricoma, a tumor thought to be derivedfrom matrix cells, was positive for cyclin D1, D2, and D3. Ourresults suggest that cyclin D1 may mediate the proliferationof stem cells in the bulge to more differentiated transientamplifying cells in the suprabasal ORS. In contrast, non-cyclinD1-proteins appear to control cell division of the highly proliferativebulb matrix cells. This non-cyclin D1-mediated proliferationmay provide a protective mechanism against tumorigenesis, whichis overridden in pilomatricomas. Our data also demonstrate thatthe combination of DNA macroarray, LCM and quantitative real-timePCR is a powerful approach for the study of gene expressionin defined cell populations with limited starting material.

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