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Regulation of Biosynthetic Cargo Trafficking in Neurons

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Release : 2023
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Book Synopsis Regulation of Biosynthetic Cargo Trafficking in Neurons by : Iryna Pustova

Download or read book Regulation of Biosynthetic Cargo Trafficking in Neurons written by Iryna Pustova. This book was released on 2023. Available in PDF, EPUB and Kindle. Book excerpt: Neurons are highly polarized cells with extremely long projections: dendrites and axons (together referred to as neurites). The central secretory dogma states that all protein synthesis and early secretory events take place in the cell body of a neuron, the soma. Yet, computational studies fail to reconcile experimental evidence with this notion proposing that there must be local protein synthesis and trafficking routes in distal neurites to support the function of a neuronal cell (reviewed in Chapter 1). Indeed, multiple lines of evidence from transcriptomics and protein translation studies indicate that local protein synthesis takes place independently of the soma. Amongst locally translated proteins, there are numerous secreted and membrane proteins. Yet, it is not clear how these newly synthesized proteins can be secreted locally, mainly, because the secretory pathway is largely understudied, especially in human neurons. Thus, I used human-induced pluripotent stem cells that I differentiated into cortical neurons to study the secretory pathway in distal neurites. In Chapter 2, I show that the secretory events occur in distal neuronal projections independently of the cell body. In fact, I find that nascent proteins are trafficked using an unconventional pathway via recycling endosomes. In addition, I uncover surprising new roles for TFG, a ubiquitously expressed protein and an important player in the early secretory pathway. Missense mutations in TFG have been identified in patients with neurodegenerative disorders though it is not clear how TFG results in disease. In Chapter 2, I show that TFG is not only important in the early secretory events in the conventional ER-to-Golgi trafficking, but it also mediates the unconventional secretory route where newly synthesized proteins exit ER and enter endosomes locally in distal neurites. Curiously, I find that TFG abundantly localizes with endosomes, suggesting that it must have an additional role in the endosomal pathway. Thus, I find that TFG has three distinct roles in neuronal cells: 1) conventional ER-to-Golgi trafficking in the soma, 2) unconventional ER-to-endosome route in distal neurites, 3) regulation of endosomal pathway. Future work, discussed in Chapter 3, will shed light on how TFG regulates the latter and how mutations in TFG lead to neurodegeneration.

Local Biosynthetic Trafficking of Synaptic Proteins in Neuronal Dendrites

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Release : 2017
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Book Synopsis Local Biosynthetic Trafficking of Synaptic Proteins in Neuronal Dendrites by : Aaron Benjamin Bowen

Download or read book Local Biosynthetic Trafficking of Synaptic Proteins in Neuronal Dendrites written by Aaron Benjamin Bowen. This book was released on 2017. Available in PDF, EPUB and Kindle. Book excerpt: Neurons face the challenge of regulating the abundance, distribution and repertoire of integral membrane proteins on the surface of their immense, architecturally complex dendritic arbors. While the endoplasmic reticulum (ER) supports local translation of secretory cargo in all dendrites, most dendrites lack the Golgi apparatus (GA), an essential organelle for conventional secretory trafficking. Thus, whether secretory cargo is locally trafficked in dendrites through a non-canonical pathway remains a fundamental question. We have defined the trafficking itinerary for key synaptic molecules in dendrites. Following ER exit, the AMPA-type glutamate receptor GluA1 and neuroligin 1 undergo spatially restricted entry into the dendritic secretory pathway and accumulate in recycling endosomes (REs) located in dendrites and spines prior to reaching the plasma membrane. Surprisingly, surface delivery of GluA1 occurred even when GA function was disrupted. Thus, in addition to their canonical role in protein recycling, REs are critical mediators of forward secretory trafficking in neuronal dendrites and spines through a specialized GA-independent trafficking network. While the SNARE machinery that supports biosynthetic trafficking from the GA to the plasma membrane in neurons is not known, the SNAREs that mediate RE exocytosis have been partially defined. Surprisingly, we found that constitutive trafficking of GluA1 through REs does not depend on VAMP2, an R-SNARE with a well-defined role in RE exocytosis. Instead, the clostridial-neurotoxin insensitive SNARE VAMP7 defined a pool of GluA1-containing transport vesicles and was required for their delivery to the plasma membrane. Synaptic stimulation accelerated the delivery of GluA1 from this pool. Interestingly, while this activity-regulated delivery required VAMP2, inhibition of VAMP7 had no effect on activity-induced exocytosis. Thus, VAMP2 and VAMP7 play complementary roles in activity-induced and constitutive delivery of new synaptic proteins. Overall we have identified a novel biosynthetic pathway that involves GA-independent transfer of cargoes to the dendritic RE compartment. Subsequent exocytosis of biosynthetic REs is constitutively maintained by VAMP7, but can be promoted by synaptic activity in a VAMP2-dependent manner. These results provide crucial insight into membrane trafficking processes that could support experience-dependent learning by rapidly delivering locally synthesized proteins to synaptic locations. Ongoing efforts are focused on the development of novel optical approaches to control secretory trafficking that will ultimately expand our capability to dissect the spatial trafficking of cargoes within the dendrite.

Shaping the Postsynaptic Landscape: Understanding the Role of Neuronal Activity in Local Secretory and Endocytic Protein Trafficking Dynamics

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Release : 2018
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Book Synopsis Shaping the Postsynaptic Landscape: Understanding the Role of Neuronal Activity in Local Secretory and Endocytic Protein Trafficking Dynamics by : Ashley M. Bourke

Download or read book Shaping the Postsynaptic Landscape: Understanding the Role of Neuronal Activity in Local Secretory and Endocytic Protein Trafficking Dynamics written by Ashley M. Bourke. This book was released on 2018. Available in PDF, EPUB and Kindle. Book excerpt: Neuronal development, morphology, excitability and synapse function rely on the ability to maintain and dynamically regulate the repertoire of channel, receptor and adhesion integral membrane proteins presented on the cell surface with extraordinary spatiotemporal specificity. The requirement for the exact spatiotemporal control of surface protein abundance and spatial distribution is an especially tall order for neuronal cells given their immense size, intricate morphology and segregated domain structure. Precise regulation of biosynthetic and endocytic protein trafficking is further confounded by synaptic activity, and the polarization of the somatic Golgi apparatus (GA) presents an arduous undertaking by newly synthesized dendritic integral membrane proteins. How are these challenges reconciled with space- and time-sensitive protein movements to effectively sustain neuronal function? Where, when and how key synaptic receptor proteins are trafficked to and within remote dendritic domains to meet the exigent demands of the cell have remained fundamental yet challenging questions in neuronal cell biology. Recent findings from the Kennedy lab and others propose the existence of a compartmentalized secretory trafficking network in dendrites yet experimentally investigating the relevance of local vs. centralized trafficking pathways has been impossible because currently there is no way to selectively control forward secretory trafficking from distinct subcellular domains. Here I describe the development and implementation of an opto/chemogenetic approach that allows for local, light-triggered forward trafficking of endoplasmic reticulum (ER)-sequestered proteins from user-defined regions within the cell (e.g. the neuronal cell body vs. individual dendritic branches). We discovered that proteins originating in the cell body could be transported deep into dendrites before surface insertion, with distinct cargoes displaying strikingly different kinetics, spatial distributions and activity dependencies. Surprisingly, proteins entering the dendritic secretory pathway were rapidly dispersed before reaching the surface. Additionally, we discovered that select cargoes are rapidly inserted in the plasma membrane at the axon initial segment (AIS), demonstrating a previously unappreciated role of the AIS as a major forward trafficking hub even for somatodendritic cargoes. Finally, we demonstrate that activity may have opposite effects on subcellular targeting of cargoes processed through somatic and dendritic networks. Our results provide the first quantitative characterization of compartmentalized secretory trafficking, placing important experimental constraints on current models for long-range and local protein trafficking. Once newly delivered synaptic proteins arrive at their functional destinations on the dendritic spine PM, their abundance and spatial distribution can be maintained or drastically modified through their endocytic trafficking depending on the current activity state of the synapse. We hypothesized that local alterations to synapses are mediated in part by regulated trafficking of postsynaptic proteins through organelles called recycling endosomes (REs), which act as reservoirs for important postsynaptic molecules. REs are housed within a large fraction of dendritic spines, the major postsynaptic sites of excitatory neurotransmission, and are thus well-poised to rapidly respond to changes in local activity to modulate synaptic structure and function. Using optical techniques coupled with local synapse activation and inactivation, we discovered that the rate of constitutive cargo flux through REs bidirectionally scales with synaptic activity at individual synaptic sites. Additionally, we demonstrate that RE cargo trafficking is coupled to synaptic activity by NMDA receptors and extracellular calcium. Finally, we demonstrate the synapse-specific, activity-dependent internalization of AMPA-type glutamate receptor 1 (GluA1), a key synaptic protein and known RE cargo. Overall, we have developed a novel optical approach for controlling secretory trafficking and we have characterized how neuronal activity influences the spatiotemporal properties of secretory and endocytic protein trafficking within distinct neuronal sub-compartments. These results provide crucial insight into how membrane trafficking processes might establish, maintain and modulate the molecular composition of synapses to support diverse forms of experience-dependent plasticity. Ongoing efforts are focused on both the proteomic mapping of the RE as well as the application of our novel optical approach to control the secretory trafficking of endogenous proteins.

Trafficking Inside Cells

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Release : 2010-05-30
Genre : Science
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Book Rating : 77X/5 ( reviews)

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Book Synopsis Trafficking Inside Cells by : Nava Segev

Download or read book Trafficking Inside Cells written by Nava Segev. This book was released on 2010-05-30. Available in PDF, EPUB and Kindle. Book excerpt: This book covers the past, present and future of the intra-cellular trafficking field, which has made a quantum leap in the last few decades. It details how the field has developed and evolved as well as examines future directions.

Molecular Biology of The Cell

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Release : 2002
Genre : Cytology
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Book Rating : 183/5 ( reviews)

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Book Synopsis Molecular Biology of The Cell by : Bruce Alberts

Download or read book Molecular Biology of The Cell written by Bruce Alberts. This book was released on 2002. Available in PDF, EPUB and Kindle. Book excerpt:

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