[HTML][HTML] SBDS-deficient cells undergo accelerated apoptosis through the Fas-pathway

P Rujkijyanont, K Watanabe, C Ambekar… - …, 2008 - haematologica.org
P Rujkijyanont, K Watanabe, C Ambekar, H Wang, A Schimmer, J Beyene, Y Dror
haematologica, 2008haematologica.org
Background Shwachman-Diamond syndrome is an inherited multisystem disorder
characterized by bone marrow and pancreatic dysfunction as well as metaphyseal
dysostosis. Ninety percent of the patients have mutations in the Shwachman-Bodian-
Diamond syndrome gene (SBDS). The relationship between SBDS and cell survival is
unknown. In this study we investigated whether deficiency of the SBDS protein can cause
increased apoptosis and, if so, what pathways are involved in this process. Design and …
Abstract
Background Shwachman-Diamond syndrome is an inherited multisystem disorder characterized by bone marrow and pancreatic dysfunction as well as metaphyseal dysostosis. Ninety percent of the patients have mutations in the Shwachman-Bodian-Diamond syndrome gene (SBDS). The relationship between SBDS and cell survival is unknown. In this study we investigated whether deficiency of the SBDS protein can cause increased apoptosis and, if so, what pathways are involved in this process. Design and Methods To determine whether accelerated apoptosis of Shwachman-Diamond syndrome cells is caused by a deficiency in SBDS we generated two SBDS-knockdown cell clones. We then evaluated, Fas expression and levels of the intracellular proteins, BAX, BCL-2 and BCL-X L and determined the effects of apoptosis inhibitors. Using oligonucteotide-microarrays we also analyzed apoptosis-related gene expression in Shwachman-Diamond syndrome marrow cells. Results We found that knocking down SBDS by short interfering hairpin RNA in HeLa cells resulted in a prominent increase in cell death. The mechanism for the accelerated apoptosis was related to marked hypersensitivity to Fas stimulation, and increased Fas expression. In contrast, there was no increase in the expression ratio of the pro-apoptotic factor, BAX, to the pro-survival factors, BCL2 and BCL-X L in the SBDS-knockdown cells and in the patients’ marrow cells. Furthermore, inhibition of Fas and caspase 8, but not caspase 9, significantly improved the defective cell growth phenotype. Conclusions Our work provides new data about the pro-survival properties of SBDS, whose inhibition results in accelerated apoptosis through the Fas pathway.
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