This is particularly true for transport of cytosolic cargoes where the inherent solubility of these proteins makes optical imaging challenging. In previous studies, we transfected fluorescent-tagged soluble proteins in cultured
hippocampal neurons and imaged thin distal axons, visualizing discernible individual particles within a diffuse background of fluorescent molecules (Roy et al., 2007 and Roy et al., 2008). Based on observations LY2157299 concentration that cytosolic particles moved rapidly but more infrequently than fast component proteins, we speculated that population dynamics of cytosolic cargoes were akin to neurofilament transport, in which compelling evidence indicates that the intermittent fast movements of individual neurofilaments leads Docetaxel purchase to the overall slow rates seen in the radiolabeling studies (Roy et al., 2000, Wang et al., 2000 and Yan and Brown, 2005). However, limited to the analysis of observable particles in thin distal axons, our previous methods did not allow us to visualize and analyze the population as a whole or consider potential roles of nonparticulate or diffusible protein pools on overall transport, an issue that we overcame by using our current imaging paradigm. Moreover, these studies did not take
into account the minor pools of cytosolic proteins moving in fast transport. In hindsight, it seems probable that the vast majority of the transient, short-range movements that we see with our photoactivation paradigm were not apparent with steady-state labeling, where they were perhaps hidden within the background fluorescence. The presence of fast-moving particles also complicates the interpretation of our previous studies. Finally, some studies have reported the biased movement of soluble, cytoskeletal proteins in extruded squid axons by exogenously introducing (stabbing) these proteins within the axon shaft (Galbraith crotamiton et al., 1999 and Terada et al., 2000). The physiologic relevance of this experimental paradigm is unclear and
these studies do not provide much mechanistic insight beyond what is known from using pulse-chase radiolabeling. In summary, our experiments with live imaging, in vivo biochemical assays, and biophysical modeling suggest a working model that can explain the mechanistic logic behind the slow axonal transport of cytosolic proteins. Though the model can explain how clusters of cytosolic proteins can be transported efficiently, further insights into the rules of cytosolic protein transport will have to await identification of specific transport machineries and the detailed characterization of the complexes themselves. Hippocampal cultures were obtained from brains of postnatal (P0–P2) CD-1 mice following standard protocols. Briefly, dissociated cells were plated at a density of 50,000 cells/cm2 in poly-D-lysine-coated glass-bottom culture dishes (MatTek, Ashland, MA) and maintained in Neurobasal + B27 media (Invitrogen, Carlsbad, CA) supplemented with 0.5 mM glutamine.