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First published online February 18, 2009
doi: 10.1242/10.1242/jcs.015289
Commentary |
Department of Biological Chemistry, Weizmann Institute of Science, 76100 Rehovot, Israel
* Author for correspondence (e-mail: mike.fainzilber{at}weizmann.ac.il)
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Summary |
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 Top Summary IntroductionCytoplasmic roles for Ran...Localized regulation of axonal...Regulation of Ran state...Conclusions and perspectivesReferences |
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Key words: Ran, Axonal transport, Nucleocytoplasmic transport
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Introduction |
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TopSummaryIntroductionCytoplasmic roles for Ran...Localized regulation of axonal...Regulation of Ran state...Conclusions and perspectivesReferences |
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. By contrast, the GDP-bound form of Ran, which is prevalent in the cytoplasm, does not bind to importins, which are exported from the nucleus in association with RanGTP. In the cytosol, competitive binding of RanBP1 releases RanGTP from importins, and rebinding is prevented by RanGAP-mediated hydrolysis of Ran to the GDP-bound state. Thus, the asymmetric distribution of Ran effectors and consequently of GTP- and GDP-bound Ran provides directionality to nuclear transport (Fig. 1) (reviewed by Kalab and Heald, 2008
; Poon and Jans, 2005; Rensen et al., 2008).
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; Kalab et al., 2006). The affinity of RCC1 for chromatin is thought to enable the formation of RanGTP-RanGDP gradients even in mitotic cells, which lack the geographical subdivision of nucleus and cytoplasm. Current models for mitotic-spindle assembly postulate that the Ran gradient has a global role in spatial organization of the mitotic apparatus, and that RanGTP also acts locally to regulate the activity of spindle-assembly factors and other proteins (Clarke and Zhang, 2008). Although the RanGTP gradient can potentially be modulated throughout the cell in mitosis, sequestration of RCC1 within the nuclear envelope in interphase and postmitotic cells would seem to require that processes that are dependent on active regulation of Ran be restricted to regions in close proximity to the nucleus. However, a number of recent papers have now shaken this view. In this Commentary, we review new findings on cytoplasmic roles for Ran and on new mechanisms for Ran regulation in cytoplasmic locations that are distant from the nucleus, including neuronal axons and cytoplasmic protrusions in megakaryocytes.
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Cytoplasmic roles for Ran in interphase and postmitotic cells |
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TopSummaryIntroductionCytoplasmic roles for Ran...Localized regulation of axonal...Regulation of Ran state...Conclusions and perspectivesReferences |
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). Neurons from Drosophila embryos were incubated for 1 week in culture with dsRNAs and then inspected for different morphological phenotypes, including excessive branching, defasciculation (separation of axons from a bundle of axons known as a fascicle), axon blebbing, cell loss and reduced outgrowth. Cultures in which RAN was knocked down by RNAi revealed both excessive branching and defasciculation. This observation was recapitulated in mouse embryonic cortical neurons (Sepp et al., 2008), in which RNAi of RAN caused defects in neurite outgrowth that were indicated by the presence of processes with abnormal blebbing (Sepp et al., 2008). In addition to the blebbing phenotype, Ran-deficient neurons showed an increase in branch arborization. The branching and blebbing phenotypes were also shown to occur in vivo (in explant slices). Notably, immunostaining for Ran in dissociated cortical cultures found high levels in cell nuclei, as expected, but also in processes. These results suggest an evolutionarily conserved role for Ran in the regulation of neurite extension during embryonic development (Sepp et al., 2008).
Other studies have implicated the Ran-binding protein RanBP9 (also known as RanBPM) and, by extension, Ran in cytoplasmic signaling systems in neuronal processes, and in the regulation of neuronal outgrowth. Yeast two-hybrid screens identified RanBP9 as an interactor of the cytoplasmic domains of the neural cell-adhesion molecule L1 (Cheng et al., 2005) and the axon guidance receptor plexin A1 (Togashi et al., 2006). Overexpression of RanBP9 in mouse primary cerebellar neurons reduced neurite outgrowth that was regulated by either the L1 or plexin signaling pathways (Cheng et al., 2005; Togashi et al., 2006). Truncation or suppression of RanBP9 reduced responses to the plexin-A1 ligand semaphorin 3A (Togashi et al., 2006).
Additional examples of Ran's involvement in cytoplasmic signaling pathways were recently reported in the nematode Caenorhabditis elegans and in the protozoan parasite Toxoplasma gondii. In C. elegans, major sperm protein (MSP) acts as a signaling protein for oocyte meiotic maturation, and the MSP signal is, in part, transduced by the ephrin receptor homolog VAB1, which functions as a negative regulator of meiotic maturation unless activated by MSP. Endocytic transport of VAB1 is modulated by direct binding of Ran to the VAB1 intracellular domain (Cheng et al., 2008). In T. gondii, Ran is distributed throughout the parasite cytoplasm, rather than concentrating in and around the nucleus (Frankel and Knoll, 2008). Thus, Ran and Ran-binding proteins are directly implicated in diverse cytoplasmic signaling or trafficking events in a range of cell types, from protozoans to mammals.
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Localized regulation of axonal Ran in injured neurons |
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TopSummaryIntroductionCytoplasmic roles for Ran...Localized regulation of axonal...Regulation of Ran state...Conclusions and perspectivesReferences |
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), in acute signaling from synapses to cell bodies in Aplysia californica neurons and in rodent hippocampi (Brilli et al., 2009; Lai et al., 2008; Thompson et al., 2004), and in the injury response in lesioned peripheral sensory neurons (Hanz and Fainzilber, 2006; Hanz et al., 2003; Perlson et al., 2005). Work from our laboratory demonstrated that importins are found throughout axons and dendrites at significant distances from the cell body, and that levels of importin-β1 are increased through local translation of axonal importin-β1-encoding mRNA after lesion (Hanz et al., 2003). This leads to the formation of a complex between importin- and importin-β1 that binds to nuclear-localization signal (NLS)-containing cargo proteins with high affinity; the increased level of importin-β1 also provides additional binding sites for proteins that interact directly with importin-β1 (Perlson et al., 2005). The complex is transported retrogradely from axons to cell bodies via an interaction of importin- with the microtubule-associated motor protein dynein. The dual role of importins in retrograde transport in neuronal processes and nuclear import in cell bodies establishes this protein family as fundamental integrators and regulators of intracellular communication in neurons.
The essential roles of importins in the axonal transport of signaling cargos led us to examine the possibility that Ran regulates this process. We found Ran in both its GTP- and GDP-bound forms in axons of rat sciatic nerve at distances of 4-6 cm from neuronal cell bodies (Yudin et al., 2008). In non-injured axons, RanGTP was observed in a complex with CAS, importin- and dynein. RanBP1 and RanGAP, which facilitate the hydrolysis of RanGTP to RanGDP (see Introduction) (Fig. 1), were expressed at low levels in uninjured axons, and their concentration in axonal cytoplasm was markedly increased upon nerve injury. This upregulation occurred through local translation of axonal Ranbp1 mRNA, and through an as-yet-uncharacterized mechanism for RanGAP. The newly synthesized RanBP1, together with RanGAP, facilitated dissociation of Ran from the importin-–dynein complex in axons and the hydrolysis of RanGTP to GDP (Yudin et al., 2008), allowing binding of newly translated importin-β1 to importin- on dynein and thus creating a retrograde injury-signaling complex that is ready to bind to cargo. In contrast to the classical nuclear transport model, this mechanism might require local production of RanGTP in axonal cytoplasm, perhaps by an as-yet-unidentified axonal RanGEF (Fig. 2) (see also below). In vivo perturbation of the system by introducing a dominant-negative Ran mutant or by adding blocking antibodies against Ran or RanBP1 inhibited injury responses in the targeted neuronal population. These findings establish a new role for Ran in the regulation of retrograde injury signaling in peripheral sensory neurons, and unveil a new function for Ran in the regulation of transport in the cytoplasm. Moreover, although we originally envisaged that Ran might have a role as a `safety catch' to regulate the binding of cargo to importins on dynein (Yudin et al., 2008), it is tempting to speculate that, in other circumstances, Ran might itself act as a cargo adaptor. For example, the Ran-mediated endocytic trafficking described by Cheng et al. (Cheng et al., 2008) in nematodes might occur through interactions of Ran both with dynein complexes and endosomes.
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). Strict control of axonal RanBP1 levels might therefore allow localized changes in RanGTP hydrolysis. Maintaining latent stores of RanBP1 in the form of locally concentrated mRNA, and the activation of such stores by localized translation when required, provides an efficient mechanism for enabling spatially restricted changes in the nucleotide-bound state of Ran. Localization of mRNA might be more `cost-efficient' than protein transport, as a single mRNA can be translated into protein multiple times to initiate or maintain protein activities at spatially restricted sites within a cell. Transport and localization of specific mRNAs have been described in a variety of cells and organisms, from yeast to mammalian neurons (Gerst, 2008; Wang et al., 2007).
Only a fraction of the mRNA transcripts that are expressed in neurons are targeted into dendrites or axons (Willis et al., 2005; Willis and Twiss, 2006). Such targeting is usually dependent on localization motifs in the 3' untranslated region (UTR) of specific transcripts, which are recognized by RNA-binding proteins that mediate mRNA transport. mRNA-associated complexes are shuttled as granules on microtubules or actin filaments by motor proteins of the kinesin, dynein or myosin families (Bullock, 2007). Upon arrival at the target site, the RNA granules may dissociate to allow translation or be maintained as a localized storage point of transcript. A few examples of primary sequence motifs for RNA localization have been described in the literature (e.g. Zhang et al., 2001), but localization signals are more likely to function through secondary and tertiary structural elements. For instance, cis-acting RNA elements might encode stable secondary structures that allow recognition and docking of trans-acting RNA-binding proteins. Such structural localization motifs are very heterogeneous in their nature and complexity, and, hence, are difficult to predict. Indeed, the 3' UTR region that contains axonal localization information in RanBP1 does not contain any previously characterized localization motifs at the level of the primary sequence (Yudin et al., 2008). Intriguingly, local axonal translation of both RanBP1 and importin-β1 is Ca2+-sensitive (Yudin et al., 2008), which might indicate co-regulation of these and other transcripts that are required for the injury response.
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Regulation of Ran state and cytoskeleton dynamics by a novel cytoplasmic RanGEF |
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TopSummaryIntroductionCytoplasmic roles for Ran...Localized regulation of axonal...Regulation of Ran state...Conclusions and perspectivesReferences |
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), and there is some evidence that splice variants of RCC1 can be found at low levels in the cytoplasm under certain conditions (Hood and Clarke, 2007). So far, RanGEF activity has not been established for any of these cytoplasmic RCC1-related molecules. Strikingly, however, a cytoplasmic RanGEF candidate, RanBP10, was recently identified on the basis of its homology to RhoGEFs, rather than to RCC1 (Schulze et al., 2008).
Schulze et al. (Schulze et al., 2008) set out to study the dynamics of microtubules in megakaryocytes, which are large polyploid blood cells that – upon maturation – generate nascent blood platelets within microtubule-based cytoplasmic extensions. This process requires significant mobilization of microtubules that are enriched in β1-tubulin, the form that is required for efficient thrombopoiesis in the cell periphery. RanBP10 was implicated as a β1-tubulin interactor in a yeast two-hybrid screen, and this was confirmed biochemically using both megakaryocyte lysates and purified proteins in vitro. Furthermore, RanBP10 was demonstrated to be capable of binding to both endogenous Ran and β-tubulin simultaneously in HEK 293 cells. Finally, immunocytochemistry showed that RanBP10 associated with microtubules in megakaryocytes (Fig. 3).
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) suggest that spatiotemporally restricted generation of RanGTP by RanBP10 on the cytoplasmic microtubule cytoskeleton might influence microtubule organization and cytoskeletal dynamics. Notably, we observed concentrates of RanGAP at the growing axon tip in sensory neurons in culture (Yudin et al., 2008). It is tempting to compare these different observations from the megakaryocyte and axonal models (Fig. 3), and to speculate that the RanGEF activity of microtubule-bound RanBP10 or related molecules might antagonize RanGAP activity in other cytoplasmic microdomains, creating localized variation in RanGTP levels and thereby modulating cytoskeleton growth.
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RanBP10 is closely related to RanBP9, which – as discussed above – has been implicated in cytoplasmic signaling through a neural cell-adhesion molecule and an axon-guidance receptor in neurites (Cheng et al., 2005; Togashi et al., 2006). The candidate GEF domains of RanBP9 and RanBP10 are highly conserved (Fig. 4), which suggests that RanBP9 might also harbor RanGEF activity. Moreover, the fact that RanBP9 is linked to axon-guidance receptors on the one hand (Togashi et al., 2006) and to microtubules on the other (Nakamura et al., 1998) suggests that both of these Ran-binding molecules might directly transduce guidance signaling to cause cytoskeletal responses.
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Conclusions and perspectives |
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TopSummaryIntroductionCytoplasmic roles for Ran...Localized regulation of axonal...Regulation of Ran state...Conclusions and perspectivesReferences |
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; Rensen et al., 2008). The identification of neuronal-process-localized mRNA transcripts encoding importin-β1 and RanBP1 (Hanz et al., 2003; Yudin et al., 2008) indicates a potential new mechanism for regulating the GTP state of Ran in a temporal or transient manner. Local translation of axonal and dendritic mRNAs is proving to be of increasing importance for rapid and specific modulation of many aspects of neuronal physiology (Wang et al., 2007). Indeed, subcellular targeting and localized translation of mRNA is emerging as a widespread phenomenon in eukaryotic cells in general (Lecuyer et al., 2007). It will therefore be crucial to identify and characterize the localization motifs in mRNA transcripts encoding RanBP1 and importin-β1, and to characterize the motor and adaptor proteins that are involved in their transport. The identification of localization motifs will open the door to specific knockdown or perturbation of the localized transcripts, and will potentially allow the examination of cytoplasmic roles of the Ran system without perturbing nuclear or mitotic mechanisms.
Some of the most intriguing questions arising from the new data are whether additional RanGEFs apart from RanBP10 remain to be discovered, and how significant (quantitatively and physiologically) these putative RanGEFs are likely to be. Before addressing these issues, however, it will first be important to confirm the GEF activity of RanBP10 in additional assays and biological systems. Schulze et al. (Schulze et al., 2008) used an in vitro FRET assay to monitor nucleotide-exchange activity of recombinant RanBP10, and it would be useful to see this activity quantified in the direct GEF assays that are commonly used for RCC1 (Bischoff and Ponstingl, 1995). Moreover, the level of Ran nucleotide-exchange activity observed for RanBP10 was an order of magnitude less than that reported for RCC1 (Schulze et al., 2008); it will be interesting to determine whether this is because RanBP10 activity is dependent on specific conditions or cofactors. Does RanBP9 also harbor exchange activity for Ran, as is implied by its sequence similarity to RanBP10 (Fig. 4)? Are additional RhoGEF-related molecules likely to do `double duty' as RanGEFs? Given the diversity and promiscuity of RhoGEF-mediated signaling (Bos et al., 2007; Schiller, 2006), a positive answer to the latter question might shift the Ran field to an entirely new level of complexity. Clearly, it will be important to characterize in detail the expression of RanBP10 and other candidate RanGEFs in different cell types and tissues, and to follow up on such studies with transgenic and knockdown approaches to determine the physiological significance of the putative new RanGEFs relative to RCC1.
Finally, we should note that the findings highlighted above have emerged from highly specialized cell types – neurons and megakaryocytes. Neurons are among the largest and most morphologically complex cells known, and megakaryocytes have a unique life cycle that culminates in an elaborate wave of proplatelet formation concomitant with compression and eventual degradation of the nucleus (Patel et al., 2005). Cytoplasmic Ran regulation in these cell types might reflect an increased need for specialized regulatory or transport systems in large or specialized cells, as reported by Kaltschmidt and colleagues for NF
B transport in neurons versus non-neuronal cells (Mikenberg et al., 2006; Mikenberg et al., 2007). Alternatively, the findings of our group (Yudin et al., 2008) and of Schulze et al. (Schulze et al., 2008) might simply reflect the fact that it is easier to make such observations in cells that extend cytoplasmic protrusions a large distance from the nucleus. Nonetheless, the original observations on the cytoplasmic roles of importins in neuronal axons were quickly followed by reports that similar mechanisms are at work in HeLa cells and Xenopus oocytes (Mesika et al., 2005; Salman et al., 2005). We therefore expect that regulation of the guanine-nucleotide state of Ran in the cytoplasm will prove to be important in many eukaryotic cell types and tissues, and look forward to future work that will address these issues.
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Footnotes |
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References |
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TopSummaryIntroductionCytoplasmic roles for Ran...Localized regulation of axonal...Regulation of Ran state...Conclusions and perspectivesReferences |
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