, 2008), and Cd was also shown to cause cell death in a large num

, 2008), and Cd was also shown to cause cell death in a large number of different cell types (Templeton and Liu, 2010). Cell death induction by Cd was ascribed to the causation of ER-stress

(Wang et al., 2009), mitochondrial depolarization (Messner et al., 2009), increase in ceramides and calpain-activation (Lee and Thevenod, 2008), ROS-production (Yang et al., 2007), and DNA-damage (Liu and Jan, 2000). Intriguingly, the reported final outcome of Cd-induced cell death is highly diverse, ranging from classical apoptosis (Jung et al., Torin 1 supplier 2008) and necrosis (Kaji et al., 1992 and Kishimoto et al., 1991) to programmed necrosis (Messner et al., 2009) and autophagy (Dong et al., 2009). This study was conducted to precisely define the final outcome of Cd-induced cell death in endothelial cells, and to study the cellular processes involved therein with a “bottom up” research strategy. Many previous studies on cadmium-induced cell death focussed primarily on upstream signalling analyses, lacking a hard fact characterization of the ultimate outcome. As the endpoint of cell death defines whether an agent (Cd) causes inflammation (necrosis) or not (apoptosis), the clear definition of the mode of cell death is crucial Carfilzomib for the pathophysiological understanding of Cd-caused diseases. All reagents used were of purissimum or analytical grade quality and were purchased from

Sigma–Aldrich (Sigma–Aldrich, Vienna, Austria) unless specified otherwise. The isolation and culture of human umbilical vein endothelial cells (HUVECs) has been described previously (Bernhard et al., 2003). The isolation and analysis of HUVECs were approved by the Ethics Committee of the Medical University of Innsbruck (No.: UN2979) and the Ethics Committee of the Medical University of Vienna (EK Nr. 1183/2012). Cells were routinely passaged in 0.2% gelatine-coated (Sigma, Steinheim, Germany) polysterene culture flasks (TPP, Switzerland) in endothelial growth medium (EGM, Lonza) in a humidified see more atmosphere containing 5% CO2. For cell death analyses, 3 × 105 HUVECs per well were

seeded onto gelatine-coated 6-well plates (TPP, Switzerland). Prior to each experiment, medium was replaced by fresh medium. BCL-XL viruses: For constitutive over-expression of human BCL-XL in HUVECs, BCL-XL encoding cDNA was PCR amplified and recombined into pDONR-207 (Invitrogen) using Invitrogen’s B/P recombination kit. A sequence verified clone was used for L/R recombination with pHR-SFFV-dest-IRES-Puro thereby generating the lentiviral expression plasmid pHR-SFFV-BCLXL-IRES-Puro (Sigl et al., 2009). For lentiviral transduction, human HEK 293T cells were transiently transfected with lentiviral plasmids containing cDNAs coding for human BCL-XL or eGFP, along with the packaging plasmids pCMV 8.91 and pVSV-G (kindly provided by Didier Trono). Forty eight and 72 h after transfection lentiviral supernatant was sterile filtered (0.

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