SummaryIncreasing evidence indicates that cellular uptake of several molecules can occur independently of functional dynamin, but the molecular players that regulate dynamin-independent endocytosis and the subsequent trafficking steps are still largely unknown. A survival-based short-hairpin (sh) RNA screen using a cell line expressing a diphtheria toxin receptor (DTR, officially known as HBEGF) anchored to GPI (DTR-GPI), which internalizes diphtheria toxin (DT, officially known as DTX) in a dynamin-independent manner, identified PI3KC2a, a class II phosphoinositide 3-kinase (PI3K), as a specific regulator of dynamin-independent DT internalization. We found that the internalization of several proteins that enter the cell through dynamin-independent pathways led to a relocalization of PI3KC2a to cargo-positive vesicles. Furthermore, downregulation of PI3KC2a impaired internalization of CD59 as well as fluid-phase endocytosis. Our data suggest a general role for PI3KC2a in regulating physiologically relevant dynaminindependent internalization pathways by recruiting early endosome antigen 1 (EEA1) to vesicular compartments, a step required for the intracellular trafficking of vesicles generated by dynamin-independent endocytic pathways.
Journal of Cell Sciencetrafficking of vesicles generated by dynamin-independent processes.
Results
Diphtheria toxin as a probe for dynamin-independent internalization pathwaysOn the basis of previous results that has shown that several bacterial proteins can be successfully used to study the mechanisms of internalization and trafficking (Sandvig and van Deurs, 2002), we utilized the cellular toxicity of diphtheria toxin (DT, also known as DTX) to identify molecules required for its internalization. DT enters the cell through a heparin-binding EGF-like growth factor (HB-EGF) precursor (Moya et al., 1985;Naglich et al., 1992;Simpson et al., 1998) named the diphtheria toxin receptor (DTR, officially known as HBEGF). After receptor binding, the toxin is delivered to early endosomes before it translocates to the cytosol, causing cell death (Falnes and Sandvig, 2000). It was reported previously that the tetracycline-regulated expression of a mutant form of dynamin I (K44A) in HeLa cells prevented cell intoxication, suggesting that DT enters the cell using a dynamin-dependent pathway ( Fig. 1) (Lanzrein et al., 1996;Skretting et al., 1999). However, when the transmembrane and cytoplasmic domains of the DT receptor were replaced with a GPI anchor (DTR-GPI), the induced expression of the DynK44A mutant did not prevent cell intoxication, suggesting that the modified DTR allowed DT internalization independently of dynamin (Lanzrein et al., 1996;Skretting et al., 1999). To visualize the internalization of DT in the presence or absence of mutant dynamin, we monitored the uptake of a nontoxic mutant of DT, CRM197 (Uchida et al., 1972), coupled to a Cy3 fluorophore (DT-Cy3). In HeLa DynK44A cells, which express only the wild-type DT receptor, the induction of mutant dynamin prevented DT-Cy3 entry...
