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Cancer Research 67, 8580, September 15, 2007. doi: 10.1158/0008-5472.CAN-07-2023
© 2007 American Association for Cancer Research

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Molecular Biology, Pathobiology, and Genetics

In Non-neoplastic Barrett's Epithelial Cells, Acid Exerts Early Antiproliferative Effects through Activation of the Chk2 Pathway

Hui-Ying Zhang1, Xi Zhang1, Kathy Hormi-Carver1, Linda A. Feagins1, Stuart J. Spechler1 and Rhonda F. Souza1,2

1 Department of Medicine, Dallas Veterans Affairs Medical Center and the University of Texas Southwestern Medical School, and 2 Harold C. Simmons Comprehensive Cancer Center, University of Texas Southwestern Medical Center at Dallas, Dallas, Texas

Requests for reprints: Rhonda F. Souza, Department of Gastroenterology, MC 111B1, Dallas Veterans Affairs Medical Center, 4500 South Lancaster Road, Dallas, TX 75216. Phone: 214-857-0301; Fax: 214-857-0328; E-mail: rhonda.souza{at}UTSouthwestern.edu.

Acid exerts pro-proliferative effects in Barrett's-associated esophageal adenocarcinoma cells. In non-neoplastic Barrett's epithelial (BAR-T) cells, in contrast, we have shown that acid exposure has antiproliferative effects. To explore our hypothesis that the acid-induced, antiproliferative effects are mediated by alterations in the proteins that regulate the G1-S cell cycle checkpoint, we exposed non-neoplastic Barrett's cells to acidic media (pH 4.0) and analyzed G1-S checkpoint proteins' expression, phosphorylation, and activity levels by Western blot. We studied acid effects on growth (by cell counts), proliferation (by flow cytometry and bromodeoxyuridine incorporation), cell viability (by trypan blue staining), and apoptosis (by annexin V staining), and we used caffeine and small interfering RNA to assess the effects of checkpoint kinase 2 (Chk2) inhibition on G1-S progression. Acid exposure significantly decreased cell numbers without affecting cell viability and with only a slight increase in apoptosis. Within 2 h of acid exposure, there was a delay in progression through the G1-S checkpoint that was associated with increased phosphorylation of Chk2, decreased levels of Cdc25A, and decreased activity of cyclin E–cyclin-dependent kinase 2; by 4 h, a continued delay at G1-S was associated with increased expression of p53 and p21. Caffeine and Chk2 siRNA abolished the acid-induced G1-S delay at 2 but not at 4 h. We conclude that acid exposure in non-neoplastic BAR-T cells causes early antiproliferative effects that are mediated by the activation of Chk2. Thus, we have elucidated a mechanism whereby acid can exert disparate effects on proliferation in neoplastic and non-neoplastic BAR-T cells. [Cancer Res 2007;67(18):8580–7]




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Copyright © 2007 by the American Association for Cancer Research.