Your search keyword '"Jörn, Kötteritzsch"' showing total 2 results

1. alpha5-integrin is crucial for L1CAM-mediated chemoresistance in pancreatic adenocarcinoma

Author

Susanne, Sebens Müerköster, Jörn, Kötteritzsch, Claudia, Geismann, Daniela, Gast, Marie-Luise, Kruse, Peter, Altevogt, Ulrich R, Fölsch, and Heiner, Schäfer

Subjects

Reverse Transcriptase Polymerase Chain Reaction, Blotting, Western, Nitric Oxide Synthase Type II, Apoptosis, Neural Cell Adhesion Molecule L1, Integrin alpha5, Adenocarcinoma, Flow Cytometry, Transfection, Antineoplastic Agents, Phytogenic, Pancreatic Neoplasms, Drug Resistance, Neoplasm, Caspases, Mutagenesis, Site-Directed, Tumor Cells, Cultured, Humans, RNA, Messenger, RNA, Small Interfering, Carcinoma, Pancreatic Ductal, Etoposide

Abstract

We recently showed that the adhesion molecule L1CAM (CD171) is overexpressed in pancreatic adenocarcinoma (PDAC) essentially contributing to chemoresistance of PDAC cells. In search of the mechanisms of this effect we now identified alpha5-integrin as the L1CAM ligand being essential for L1CAM-mediated chemoresistance of these highly malignant tumor cells. Thus, blockade or knock-down of alpha5-integrin in the L1CAM expressing PDAC cell lines PT45-P1res, Colo357 and Panc1 increased anti-cancer drug sensitivity. In line with the previously reported NO-dependent caspase inhibition resulting from L1CAM induced iNOS expression, the loss of chemoresistance upon alpha5-integrin inhibition was preceded by decreased iNOS expression and enhanced caspase-3/-7 activation. Accordingly, the loss of anti-cancer drug protection by alpha5-integrin inhibition could be overcome by administration of the NO-donor SNAP. Moreover, the gain of chemoresistance of parental PT45-P1 cells when transfected with L1CAM was abrogated by alpha5-integrin inhibition, whereas transfection of PT45-P1 cells with an integrin binding-deficient L1CAM mutant (L1mutRGE) did neither induce chemoresistance or iNOS expression nor conferred sensitivity to alpha5-integrin inhibition as seen upon transfection with wild-type L1CAM. Thus, mutational loss of the integrin binding site in the L1CAM molecule or the blockade of alpha5-integrin abolished the induction of iNOS expression and chemoresistance by L1CAM, indicating that both a functional L1CAM and alpha5-integrin are indispensable of L1CAM-induced drug resistance in PDAC cells.

Published

2008

2. α5-integrin is crucial for L1CAM-mediated chemoresistance in pancreatic adenocarcinoma

Author

Claudia Geismann, Jörn Kötteritzsch, Heiner Schäfer, Peter Altevogt, Susanne Sebens Müerköster, Daniela Gast, Ulrich R. Fölsch, and Marie-Luise Kruse

Subjects

Cancer Research, biology, Oncogene, urogenital system, Cell, Integrin, Transfection, Cell cycle, medicine.anatomical_structure, Oncology, Cell culture, embryonic structures, medicine, biology.protein, Cancer research, Caspase, Integrin binding

Abstract

We recently showed that the adhesion molecule L1CAM (CD171) is overexpressed in pancreatic adenocarcinoma (PDAC) essentially contributing to chemoresistance of PDAC cells. In search of the mechanisms of this effect we now identified alpha5-integrin as the L1CAM ligand being essential for L1CAM-mediated chemoresistance of these highly malignant tumor cells. Thus, blockade or knock-down of alpha5-integrin in the L1CAM expressing PDAC cell lines PT45-P1res, Colo357 and Panc1 increased anti-cancer drug sensitivity. In line with the previously reported NO-dependent caspase inhibition resulting from L1CAM induced iNOS expression, the loss of chemoresistance upon alpha5-integrin inhibition was preceded by decreased iNOS expression and enhanced caspase-3/-7 activation. Accordingly, the loss of anti-cancer drug protection by alpha5-integrin inhibition could be overcome by administration of the NO-donor SNAP. Moreover, the gain of chemoresistance of parental PT45-P1 cells when transfected with L1CAM was abrogated by alpha5-integrin inhibition, whereas transfection of PT45-P1 cells with an integrin binding-deficient L1CAM mutant (L1mutRGE) did neither induce chemoresistance or iNOS expression nor conferred sensitivity to alpha5-integrin inhibition as seen upon transfection with wild-type L1CAM. Thus, mutational loss of the integrin binding site in the L1CAM molecule or the blockade of alpha5-integrin abolished the induction of iNOS expression and chemoresistance by L1CAM, indicating that both a functional L1CAM and alpha5-integrin are indispensable of L1CAM-induced drug resistance in PDAC cells.

Published

1992