Protein modification by ubiquitin can be classified as poly- or monoubiquitination (Price & Kwaik, 2010; Fujita & Yoshimori, 2011). Polyubiquitination occurs when a chain of four or more covalently linked ubiquitin moieties is added to a single lysine of a target protein. In monoubiquitination, a single ubiquitin molecule is conjugated to one or several (multi-monoubiquitination) lysines (Haglund
& Dikic, 2005; Liu & Walters, 2010). Poly- and monoubiquitination differentially dictate the localization and/or activity of the modified protein. Polyubiquitination has long been known to destine proteins for 26S proteasome-mediated destruction, but can also direct proteins to lysosomes for degradation, activate protein
kinases, and contribute to DNA repair (Thrower et al., 2000; Chen & Sun, 2009). Monoubiquitination does not www.selleckchem.com/products/XL184.html target proteins for degradation, but rather occurs after ligand binding to a variety of cell surface receptors and can act as an internalization signal, thereby directing plasma membrane-associated proteins to endosomes (Hicke & Dunn, 2003; Patel et al., 2009; Collins & Brown, 2010). Monoubiquitination of the peroxisome membrane targets the organelle for autophagosome-mediated destruction (Kim et al., 2008). Additionally, monoubiquitination is involved in transcriptional regulation and DNA repair (Hicke & Dunn, 2003; Liu, 2004). Lastly, ubiquitination of a variety of human pathogens in the host cell Temsirolimus clinical trial cytosol targets them to autophagosomes (Clague & Urbe, 2010; Collins & Brown, 2010). While this process is emerging as an infection control against intracellular selleck inhibitor pathogens, evidence also hints that intracellular bacteria can subvert it, as Salmonella enterica serovar Typhimurium, after being mono- and polyubiquitinated in the cytosol, survives to occupy a damaged membranous compartment (Birmingham
et al., 2006). Given the importance of ubiquitination in modulating numerous eukaryotic cell processes, it is not surprising that many vacuole-adapted pathogens have evolved mechanisms to exploit the ubiquitin conjugation pathway. For example, the Legionella pneumophila-containing vacuole (LCV) recruits polyubiquitinated proteins by virtue of the actions of translocated bacterial effector proteins (Dorer et al., 2006; Price et al., 2009; Kubori et al., 2010). Salmonella Typhimurium manipulates the ubiquitin pathway to ensure proper trafficking of its effector, SopB to the Salmonella-containing vacuole (SCV) (Knodler et al., 2009; Patel et al., 2009). Given that A. phagocytophilum hijacks an array of intracellular trafficking pathways, we set out to test the hypothesis that the ApV co-opts ubiquitin. In this study, we demonstrate that ubiquitinated proteins accumulate on the AVM during infection of mammalian myeloid and endothelial cells and, to a lesser extent, tick cells.