Endoplasmic Reticulum Targeting and Insertion of Tail-Anchored Membrane Proteins by the GET Pathway

Hundreds of eukaryotic membrane proteins are anchored to membranes by a single transmembrane domain at their carboxyl terminus. Many of these tail-anchored (TA) proteins are posttranslationally targeted to the endoplasmic reticulum (ER) membrane for insertion by the guided-entry of TA protein insertion (GET) pathway. In recent years, most of the components of this conserved pathway have been biochemically and structurally characterized. Get3 is the pathway-targeting factor that uses nucleotide-linked conformational changes to mediate the delivery of TA proteins between the GET pretargeting machinery in the cytosol and the transmembrane pathway components in the ER. Here we focus on the mechanism of the yeast GET pathway and make a speculative analogy between its membrane insertion step and the ATPase-driven cycle of ABC transporters.The mechanism of membrane protein insertion into the endoplasmic reticulum (ER) has been extensively studied for many years (Shao and Hegde 2011). From this work, the signal recognition particle (SRP)/Sec61 pathway has emerged as a textbook example of a cotranslational membrane insertion mechanism (Grudnik et al. 2009). The SRP binds a hydrophobic segment (either a cleavable amino-terminal signal sequence or a transmembrane domain) immediately after it emerges from the ribosomal exit tunnel. This results in a translational pause that persists until SRP engages its receptor in the ER and delivers the ribosome-nascent chain complex to the Sec61 channel. Last, the Sec61 channel enables protein translocation into the ER lumen along with partitioning of hydrophobic transmembrane domains into the lipid bilayer through the Sec61 lateral gate (Rapoport 2007).Approximately 5% of all eukaryotic membrane proteins have an ER targeting signal in a single carboxy-terminal transmembrane domain that emerges from the ribosome exit tunnel following completion of protein synthesis and is not recognized by the SRP (Stefanovic and Hegde 2007). Nonetheless, because hydrophobic peptides in the cytoplasm are prone to aggregation and subject to degradation by quality control systems (Hessa et al. 2011), these tail-anchored (TA) proteins still have to be specifically recognized, shielded from the aqueous environment, and guided to the ER membrane for insertion. In the past five years, the guided-entry of TA proteins (GET) pathway has come to prominence as the major machinery for performing these tasks and the enabler of many key cellular processes mediated by TA proteins including vesicle fusion, membrane protein insertion, and apoptosis. This research has rapidly yielded biochemical and structural insights (​and2)2) into many of the GET pathway components (Hegde and Keenan 2011; Chartron et al. 2012a; Denic 2012). In particular, Get3 is an ATPase that uses metabolic energy to bridge recognition of TA proteins by upstream pathway components with TA protein recruitment to the ER for membrane insertion. However, the precise mechanisms of nucleotide-dependent TA protein binding to Get3 and how the GET pathway inserts tail anchors into the membrane are still poorly understood. Here, we provide an overview of the budding yeast GET pathway with emphasis on mechanistic insights that have come from structural studies of its membrane-associated steps and make a speculative juxtaposition with the ABC transporter mechanism.

Table 1.

A catalog of GET pathway component structures

Sequence-specific Retention and Regulated Integration of a Nascent Membrane Protein by the Endoplasmic Reticulum Sec61 Translocon

A defining feature of eukaryotic polytopic protein biogenesis involves integration, folding, and packing of hydrophobic transmembrane (TM) segments into the apolar environment of the lipid bilayer. In the endoplasmic reticulum, this process is facilitated by the Sec61 translocon. Here, we use a photocross-linking approach to examine integration intermediates derived from the ATP-binding cassette transporter cystic fibrosis transmembrane conductance regulator (CFTR) and show that the timing of translocon-mediated integration can be regulated at specific stages of synthesis. During CFTR biogenesis, the eighth TM segment exits the ribosome and enters the translocon in proximity to Sec61α. This interaction is initially weak, and TM8 spontaneously dissociates from the translocon when the nascent chain is released from the ribosome. Polypeptide extension by only a few residues, however, results in stable TM8-Sec61α photocross-links that persist after peptidyl-tRNA bond cleavage. Retention of these untethered polypeptides within the translocon requires ribosome binding and is mediated by an acidic residue, Asp924, near the center of the putative TM8 helix. Remarkably, at this stage of synthesis, nascent chain release from the translocon is also strongly inhibited by ATP depletion. These findings contrast with passive partitioning models and indicate that Sec61α can retain TMs and actively inhibit membrane integration in a sequence-specific and ATP-dependent manner.     

Titanium Dioxide Nanoparticles Induce Endoplasmic Reticulum Stress-Mediated Autophagic Cell Death via Mitochondria-Associated Endoplasmic Reticulum Membrane Disruption in Normal Lung Cells

Nanomaterials are used in diverse fields including food, cosmetic, and medical industries. Titanium dioxide nanoparticles (TiO₂-NP) are widely used, but their effects on biological systems and mechanism of toxicity have not been elucidated fully. Here, we report the toxicological mechanism of TiO₂-NP in cell organelles. Human bronchial epithelial cells (16HBE14o-) were exposed to 50 and 100 μg/mL TiO₂-NP for 24 and 48 h. Our results showed that TiO₂-NP induced endoplasmic reticulum (ER) stress in the cells and disrupted the mitochondria-associated endoplasmic reticulum membranes (MAMs) and calcium ion balance, thereby increasing autophagy. In contrast, an inhibitor of ER stress, tauroursodeoxycholic acid (TUDCA), mitigated the cellular toxic response, suggesting that TiO₂-NP promoted toxicity via ER stress. This novel mechanism of TiO₂-NP toxicity in human bronchial epithelial cells suggests that further exhaustive research on the harmful effects of these nanoparticles in relevant organisms is needed for their safe application.     

Peroxisomal Membrane Proteins Insert into the Endoplasmic Reticulum

We show that a comprehensive set of 16 peroxisomal membrane proteins (PMPs) encompassing all types of membrane topologies first target to the endoplasmic reticulum (ER) in Saccharomyces cerevisiae. These PMPs insert into the ER membrane via the protein import complexes Sec61p and Get3p (for tail-anchored proteins). This trafficking pathway is representative for multiplying wild-type cells in which the peroxisome population needs to be maintained, as well as for mutant cells lacking peroxisomes in which new peroxisomes form after complementation with the wild-type version of the mutant gene. PMPs leave the ER in a Pex3p-Pex19p–dependent manner to end up in metabolically active peroxisomes. These results further extend the new concept that peroxisomes derive their basic framework (membrane and membrane proteins) from the ER and imply a new functional role for Pex3p and Pex19p.     

Degradation of the Endoplasmic Reticulum by Autophagy during Endoplasmic Reticulum Stress in Arabidopsis

In this article, we show that the endoplasmic reticulum (ER) in Arabidopsis thaliana undergoes morphological changes in structure during ER stress that can be attributed to autophagy. ER stress agents trigger autophagy as demonstrated by increased production of autophagosomes. In response to ER stress, a soluble ER marker localizes to autophagosomes and accumulates in the vacuole upon inhibition of vacuolar proteases. Membrane lamellae decorated with ribosomes were observed inside autophagic bodies, demonstrating that portions of the ER are delivered to the vacuole by autophagy during ER stress. In addition, an ER stress sensor, INOSITOL-REQUIRING ENZYME-1b (IRE1b), was found to be required for ER stress–induced autophagy. However, the IRE1b splicing target, bZIP60, did not seem to be involved, suggesting the existence of an undiscovered signaling pathway to regulate ER stress–induced autophagy in plants. Together, these results suggest that autophagy serves as a pathway for the turnover of ER membrane and its contents in response to ER stress in plants.     

Protein Translocation Across the Membrane of the Endoplasmic Reticulum

Saccharomyces cerevisiae and mammals concerning the mechanisms of the translocation step and discuss the roles of the proteins implicated in this process. Received: 5 June 1996/Revised: 20 September 1996     

Development of Endoplasmic Reticulum and Glyoxysomal Membrane Redox Activities during Castor Bean Germination

Redox activities, NADH:ferricyanide reductase, NAD(P)H:cytochrome reductases, and NADH:ascorbate free-radical reductase, are present in endoplasmic reticulum (ER) and glyoxysomal membranes from the endosperm of germinating castor bean (Ricinus comminus L. var Hale). The development of these functions was followed in glyoxysomes and ER isolated on sucrose gradients from castor bean endosperm daily from 0 through 6 days of germination. On a per seed basis, glyoxysomal and ER protein, glyoxysomal and ER membrane redox enzyme activities, and glyoxylate cycle activities peaked at day 4 as did the ER membrane content of cytochrome P-450. NADH:ferricyanide reductase was present in glyoxysomes and ER isolated from dry seed. This activity increased only about twofold in glyoxysomes and threefold in ER during germination relative to the amount of protein in the respective fractions. The other reductases, NADH:cytochrome reductase and NADH:ascorbate free-radical reductase, increased about 10-fold in the ER relative to protein up to 4 to 5 days, then declined. NADPH:cytochrome reductase reached maximum activity relative to protein at day 2 in both organelles. The increases in redox activities during germination indicate that the membranes of the ER and glyoxysome are being enriched with redox proteins during their development. The development of redox functions in glyoxysomes was found to be coordinated with development of the glyoxylate cycle.     

Integral Membrane Proteins of the Nuclear Envelope Are Dispersed throughout the Endoplasmic Reticulum during Mitosis

We have analyzed the fate of several integral membrane proteins of the nuclear envelope during mitosis in cultured mammalian cells to determine whether nuclear membrane proteins are present in a vesicle population distinct from bulk ER membranes after mitotic nuclear envelope disassembly or are dispersed throughout the ER. Using immunofluorescence staining and confocal microscopy, we compared the localization of two inner nuclear membrane proteins (laminaassociated polypeptides 1 and 2 [LAP1 and LAP2]) and a nuclear pore membrane protein (gp210) to the distribution of bulk ER membranes, which was determined with lipid dyes (DiOC₆ and R6) and polyclonal antibodies. We found that at the resolution of this technique, the three nuclear envelope markers become completely dispersed throughout ER membranes during mitosis. In agreement with these results, we detected LAP1 in most membranes containing ER markers by immunogold electron microscopy of metaphase cells. Together, these findings indicate that nuclear membranes lose their identity as a subcompartment of the ER during mitosis. We found that nuclear lamins begin to reassemble around chromosomes at the end of mitosis at the same time as LAP1 and LAP2 and propose that reassembly of the nuclear envelope at the end of mitosis involves sorting of integral membrane proteins to chromosome surfaces by binding interactions with lamins and chromatin.     

Cisternal Organization of the Endoplasmic Reticulum during Mitosis

The endoplasmic reticulum (ER) of animal cells is a single, dynamic, and continuous membrane network of interconnected cisternae and tubules spread out throughout the cytosol in direct contact with the nuclear envelope. During mitosis, the nuclear envelope undergoes a major rearrangement, as it rapidly partitions its membrane-bound contents into the ER. It is therefore of great interest to determine whether any major transformation in the architecture of the ER also occurs during cell division. We present structural evidence, from rapid, live-cell, three-dimensional imaging with confirmation from high-resolution electron microscopy tomography of samples preserved by high-pressure freezing and freeze substitution, unambiguously showing that from prometaphase to telophase of mammalian cells, most of the ER is organized as extended cisternae, with a very small fraction remaining organized as tubules. In contrast, during interphase, the ER displays the familiar reticular network of convolved cisternae linked to tubules.     

Melatonin Inhibits Endoplasmic Reticulum Stress and Epithelial-Mesenchymal Transition during Bleomycin-Induced Pulmonary Fibrosis in Mice

Several reports indicate that melatonin alleviates bleomycin (BLM)-induced pulmonary fibrosis in rodent animals. Nevertheless, the exact mechanism remains obscure. The present study investigated the effects of melatonin on endoplasmic reticulum (ER) stress and epithelial-mesenchymal transition (EMT) during BLM-induced lung fibrosis. For the induction of pulmonary fibrosis, mice were intratracheally injected with a single dose of BLM (5.0 mg/kg). Some mice were intraperitoneally injected with melatonin (5 mg/kg) daily for a period of 3 wk. Twenty-one days after BLM injection, lung fibrosis was evaluated. As expected, melatonin significantly alleviated BLM-induced pulmonary fibrosis, as evidenced by Sirius red staining. Moreover, melatonin significantly attenuated BLM-induced EMT to myofibroblasts, as determined by its repression of α-SMA expression. Further analysis showed that melatonin markedly attenuated BLM-induced GRP78 up-regulation and elevation of the cleaved ATF6 in the lungs. Moreover, melatonin obviously attenuated BLM-induced activation of pulmonary eIF2α, a downstream target of the PERK pathway. Finally, melatonin repressed BLM-induced pulmonary IRE1α phosphorylation. Correspondingly, melatonin inhibited BLM-induced activation of XBP-1 and JNK, two downstream targets of the IRE1 pathway. Taken together, these results suggest that melatonin alleviates ER stress and ER stress-mediated EMT in the process of BLM-induced pulmonary fibrosis.     

Coupled Translocation Events Generate Topological Heterogeneity at the Endoplasmic Reticulum Membrane

Topogenic determinants that direct protein topology at the endoplasmic reticulum membrane usually function with high fidelity to establish a uniform topological orientation for any given polypeptide. Here we show, however, that through the coupling of sequential translocation events, native topogenic determinants are capable of generating two alternate transmembrane structures at the endoplasmic reticulum membrane. Using defined chimeric and epitope-tagged full-length proteins, we found that topogenic activities of two C-trans (type II) signal anchor sequences, encoded within the seventh and eighth transmembrane (TM) segments of human P-glycoprotein were directly coupled by an inefficient stop transfer (ST) sequence (TM7b) contained within the C-terminus half of TM7. Remarkably, these activities enabled TM7 to achieve both a single- and a double-spanning TM topology with nearly equal efficiency. In addition, ST and C-trans signal anchor activities encoded by TM8 were tightly linked to the weak ST activity, and hence topological fate, of TM7b. This interaction enabled TM8 to span the membrane in either a type I or a type II orientation. Pleiotropic structural features contributing to this unusual topogenic behavior included 1) a short, flexible peptide loop connecting TM7a and TM7b, 2) hydrophobic residues within TM7b, and 3) hydrophilic residues between TM7b and TM8.     

Sec62 Protein Mediates Membrane Insertion and Orientation of Moderately Hydrophobic Signal Anchor Proteins in the Endoplasmic Reticulum (ER)

Nascent chains are known to be targeted to the endoplasmic reticulum membrane either by a signal recognition particle (SRP)-dependent co-translational or by an SRP-independent post-translational translocation route depending on signal sequences. Using a set of model and cellular proteins carrying an N-terminal signal anchor sequence of controlled hydrophobicity and yeast mutant strains defective in SRP or Sec62 function, the hydrophobicity-dependent targeting efficiency and targeting pathway preference were systematically evaluated. Our results suggest that an SRP-dependent co-translational and an SRP-independent post-translational translocation are not mutually exclusive for signal anchor proteins and that moderately hydrophobic ones require both SRP and Sec62 for proper targeting and translocation to the endoplasmic reticulum. Further, defect in Sec62 selectively reduced signal sequences inserted in an N_in-C_out (type II) membrane topology, implying an undiscovered role of Sec62 in regulating the orientation of the signal sequence in an early stage of translocation.     

Positive Charges of Translocating Polypeptide Chain Retrieve an Upstream Marginal Hydrophobic Segment from the Endoplasmic Reticulum Lumen to the Translocon

Positively charged amino acid residues are well recognized topology determinants of membrane proteins. They contribute to the stop-translocation of a polypeptide translocating through the translocon and to determine the orientation of signal sequences penetrating the membrane. Here we analyzed the function of these positively charged residues during stop-translocation in vitro. Surprisingly, the positive charges facilitated membrane spanning of a marginally hydrophobic segment, even when separated from the hydrophobic segment by 70 residues. In this case, the hydrophobic segment was exposed to the lumen, and then the downstream positive charges triggered the segment to slide back into the membrane. The marginally hydrophobic segment spanned the membrane, but maintained access to the water environment. The positive charges not only fix the hydrophobic segment in the membrane at its flanking position, but also have a much more dynamic action than previously realized.     

Tracking Single Serotonin Transporter Molecules at the Endoplasmic Reticulum and Plasma Membrane

Transmembrane proteins are synthesized and folded in the endoplasmic reticulum (ER), an interconnected network of flattened sacs or tubes. Up to now, this organelle has eluded a detailed analysis of the dynamics of its constituents, mainly due to the complex three-dimensional morphology within the cellular cytosol, which precluded high-resolution, single-molecule microscopy approaches. Recent evidences, however, pointed out that there are multiple interaction sites between ER and the plasma membrane, rendering total internal reflection microscopy of plasma membrane proximal ER regions feasible. Here we used single-molecule fluorescence microscopy to study the diffusion of the human serotonin transporter at the ER and the plasma membrane. We exploited the single-molecule trajectories to map out the structure of the ER close to the plasma membrane at subdiffractive resolution. Furthermore, our study provides a comparative picture of the diffusional behavior in both environments. Under unperturbed conditions, the majority of proteins showed similar mobility in the two compartments; at the ER, however, we found an additional 15% fraction of molecules moving with 25-fold faster mobility. Upon degradation of the actin skeleton, the diffusional behavior in the plasma membrane was strongly influenced, whereas it remained unchanged in the ER.Live-cell microscopy and three-dimensional electron tomography has boosted our understanding of endoplasmic reticulum (ER) dynamics and morphology. Proteins have been identified which regulate the formation of cisternae versus tubelike membranes, and the contacts between ER and the various cellular organelles have been studied in detail (1). Little information, however, is available when it comes to protein dynamics and organization within the ER membrane. Its complex three-dimensional topology hampers standard diffraction-limited fluorescence microscopy approaches: in fluorescence recovery after photobleaching, for example, the obtained diffusion coefficients can be several-folds off, if the ER morphology is not correctly taken into account (2). A method is therefore needed which allows for resolving molecular movements on length scales below the typical dimensions of the ER structures.In principle, single-molecule tracking would provide the required spatial resolution due to the high precision in localizing the moving point emitters: localization errors of <40 nm can be easily achieved (3). This technique has given rise to multiple studies, in which the paths of the diffusing objects were used to make conclusions on the properties of the environment; particularly, the plasma membrane has become a favorite target for such investigations, yielding precise determinations of the diffusion coefficients of a variety of membrane proteins or lipids (4).Here, we report what is, to our knowledge, the first application of single-molecule tracking for a comparative study of the diffusion dynamics of a membrane protein at the ER versus the plasma membrane. As the protein of interest, we chose the human serotonin transporter (SERT): it is a polytopic membrane protein containing 12 transmembrane domains, with both C- and N-termini residing in the cytoplasm. Stable SERT oligomers of various degrees were observed to coexist in the plasma membrane (5). Functionally, SERT (6) is a pivotal element in shaping serotonergic neurotransmission: SERT-mediated high-affinity uptake of released serotonin clears the synaptic cleft and supports refilling of vesicular stores (7). Wild-type SERT (SERT-wt) is efficiently targeted to the presynaptic plasma membrane, whereas the truncation of its C-terminus (SERT-ΔC30) retains the mutant protein in the ER (8). The N-terminal mGFP- and eYFP-fusion constructs of the two versions of SERT thus allowed us to specifically address SERT located at the ER (eYFP-SERT-ΔC30) or at the plasma membrane (mGFP-SERT-wt (7)).Our experiments were performed at 37°C on proteins heterologously expressed in CHO cells. Total internal reflection (TIR) illumination afforded a reduction in background fluorescence and allowed for selective imaging of single mGFP-SERT-wt molecules at the cells’ plasma membrane or single eYFP-SERT-ΔC30 molecules at plasma membrane-proximal ER (Fig. 1 and see the Supporting Material). TIR was particularly crucial for single-molecule imaging of the ER-retained mutant, where out-of-focus background would surpass the weak single-molecule signals in epi-illumination.Open in a separate windowFigure 1Schematics of the plasma membrane (PM) and a part of the ER containing mGFP-SERT-wt or the ER-retained eYFP-SERT-ΔC30 mutant, respectively. Both can be excited by total internal reflection fluorescence (TIRF) excitation. Experiments were carried out either on cells expressing mGFP-SERT-wt or eYFP-SERT-ΔC30.For both mutants, the majority of molecules were mobile: in fluorescence-recovery-after-photobleaching experiments we observed a mobile fraction of 82 ± 8% for mGFP-SERT-wt and 91 ± 4% for eYFP-SERT-ΔC30. For single-molecule tracking, the high surface density of signals was reduced by completely photobleaching a rectangular part of the cell in epi-illumination; after a brief recovery period, a few single-molecule signals had entered the bleached area and could be monitored and tracked at high signal/noise using TIR excitation. Samples were illuminated stroboscopically for t_ill = 2 ms, and movies of 500 frames were recorded with a delay of t_del = 6 ms; the short delay times ensured that even rapidly diffusing molecules hardly reached the borders of the ER tubes between two consecutive frames. This illumination protocol was run for 20 times per cell, yielding ∼2500 trajectories per cell.The single-molecule localizations were first used to map those areas that are accessible to the diffusing proteins. eYFP-SERT-ΔC30 showed distinct hotspots, representing plasma membrane-proximal ER, excitable by the evanescent field (Fig. 2 A). These hotspots hardly moved within the timescale of an experiment (tens of minutes, see Fig. S1 in the Supporting Material); indeed, remarkable ER stability was previously observed using superresolution microscopy (9). In contrast, a rather homogeneous distribution was observed for mGFP-SERT-wt in the plasma membrane (Fig. 2 B).Open in a separate windowFigure 2Superresolution and tracking data at the ER and the plasma membrane. Superresolution images are shown for the ER-retained SERT mutant eYFP-SERT-ΔC30 (A) and for mGFP-SERT-wt in the plasma membrane (B). (C and D) Diffusion coefficients of eYFP-SERT-ΔC30 (C) and mGFP-SERT-wt (D) are shown as normalized histograms before (blue) and after (red) Cytochalasin D treatment. Data were fitted by Gaussian mobility distributions (see Table S1 in the Supporting Material for the fit results).Next, we compared the mobility of the observed proteins. Single-molecule localizations were linked to trajectories as described in Gao and Kilfoil (10), and the apparent diffusion coefficient, D, of each molecule was estimated from the first two points of the mean-square displacement membrane. The distribution of log₁₀ D showed a pronounced single peak (Fig. 2 D). It could be well fitted by a linear combination of two Gaussian functions, with the major fraction (85%) characterized by D_wt = 0.30 μm²/s; a broad shoulder to the left indicates the presence of proteins that are immobilized during the observation period. In contrast, the mobility of the ER-retained mutant showed a substantially different distribution, containing two clearly visible peaks (Fig. 2 C). We fitted the data with a three-component Gaussian model: the main fraction (82%) behaved similar to SERT at the plasma membrane, with D_ΔC30 = 0.32 μm²/s. In addition, a large fraction (15%) with high mobility of D_ΔC30 = 7.8 μm²/s and a minor fraction (3%) with low mobility was observed. The proteins responded as expected to degradation of the actin membrane skeleton (red bars in Fig. 2, C and D): at the plasma membrane, the mobility of mGFP-SERT-wt increased 4.6-fold (mean values), whereas at the ER membrane there was only a minor change for eYFP-SERT-ΔC30 mobility (1.06-fold increase; note that the ER is not connected to actin filaments (11)).The observation of a high mobility subfraction at the ER membrane is surprising. In general, the presence of obstacles—irrespective of whether randomly distributed or clustered, mobile or immobile—reduces the diffusivity of mobile tracers in a membrane (12). It is generally assumed that the high protein density in cell membranes is responsible for the rather low fluidity when compared to synthetic membranes (compare, e.g., Saxton and Jacobson (13) with Weiss et al. (14)). Interestingly, the observed diffusion constant of 7.8 μm²/s is of similar order as the mobility determined for various proteins in synthetic lipid membranes (14). It is thus tempting to hypothesize the presence of extended protein-depleted regions of higher fluidity within the ER membrane; such membrane domains were indeed observed already at the plasma membrane (15). We were also concerned, however, that protein degradation fragments could have contributed to our data: the three-dimensional mobility of an 85-kDa protein is ∼10 μm²/s (16), similar to the high mobility diffusion constant of eYFP-SERT-ΔC30.We tested the two explanations by analyzing the spatial distribution of fast (D_ΔC30 > 1 μm²/s) versus slow trajectories (D_ΔC30 < 1 μm²/s) of eYFP-SERT-ΔC30 (Fig. 3). Both types of trajectories clustered in the same regions, and no segregation into ER subdomains was observable at the resolved length scales. This finding—on the one hand—disfavors freely diffusing protein fragments as the origin of the high mobility fraction. On the other hand, it calls for further experiments to identify the origin of the fast and the slow mobility subfraction. Interestingly, when analyzing all eYFP-SERT-ΔC30 trajectories we found that 80% of the molecules showed diffusion confined to domains of 230-nm radius (see Fig. S2). This size is clearly smaller than the lateral extensions of the visible ER regions observed in Fig. 3. The finding indicates domain formation at the ER membrane; domains are averaged out in Fig. 3 due to the long recording times. Note that free diffusion was observed for mGFP-SERT-wt at the plasma membrane (5).Open in a separate windowFigure 3Ripley’s K function analysis of the different mobility fractions in the ER. For the cell presented in Fig. 2, the first position of every slow (D < 1 μm²/s; red) and fast (D > 1 μm²/s; blue) trajectory was plotted in panel A. Contour lines indicate regions of ER attachment to the plasma membrane. In panel B, the point-correlation function L(r)−r is plotted for the slow (red) and fast (blue) fraction. Furthermore, the correlation between fast versus slow is plotted (green). All three curves show a peak at ∼450 nm, which agrees with the extensions of the ER attachment zones.In conclusion, we have shown that single-molecule tracking is feasible for constituents of the ER membrane. We found a surprising diffusion behavior of SERT resulting in the following:

• 1.A slow fraction showing mobility reminiscent of protein diffusion in the plasma membrane, likely reflecting SERT diffusing in protein-crowded regions of the ER membrane; and
• 2.A fast fraction showing 25-fold faster diffusion kinetics.

This likely represents diffusion in altered ER membrane environments, possibly of different lipid or protein composition. Given the fact that synthesis of virtually all membrane proteins and most lipids proceeds at the ER membrane, ER heterogeneity at the nanoscale due to the continuous synthesis activity and selection for correct folding appears highly plausible.     

Tracking Single Serotonin Transporter Molecules at the Endoplasmic Reticulum and Plasma Membrane

Transmembrane proteins are synthesized and folded in the endoplasmic reticulum (ER), an interconnected network of flattened sacs or tubes. Up to now, this organelle has eluded a detailed analysis of the dynamics of its constituents, mainly due to the complex three-dimensional morphology within the cellular cytosol, which precluded high-resolution, single-molecule microscopy approaches. Recent evidences, however, pointed out that there are multiple interaction sites between ER and the plasma membrane, rendering total internal reflection microscopy of plasma membrane proximal ER regions feasible. Here we used single-molecule fluorescence microscopy to study the diffusion of the human serotonin transporter at the ER and the plasma membrane. We exploited the single-molecule trajectories to map out the structure of the ER close to the plasma membrane at subdiffractive resolution. Furthermore, our study provides a comparative picture of the diffusional behavior in both environments. Under unperturbed conditions, the majority of proteins showed similar mobility in the two compartments; at the ER, however, we found an additional 15% fraction of molecules moving with 25-fold faster mobility. Upon degradation of the actin skeleton, the diffusional behavior in the plasma membrane was strongly influenced, whereas it remained unchanged in the ER.     

The Endoplasmic Reticulum Provides the Membrane Platform for Biogenesis of the Flavivirus Replication Complex

The cytoplasmic replication of positive-sense RNA viruses is associated with a dramatic rearrangement of host cellular membranes. These virus-induced changes result in the induction of vesicular structures that envelop the virus replication complex (RC). In this study, we have extended our previous observations on the intracellular location of West Nile virus strain Kunjin virus (WNV_KUN) to show that the virus-induced recruitment of host proteins and membrane appears to occur at a pre-Golgi step. To visualize the WNV_KUN replication complex, we performed three-dimensional (3D) modeling on tomograms from WNV_KUN replicon-transfected cells. These analyses have provided a 3D representation of the replication complex, revealing the open access of the replication complex with the cytoplasm and the fluidity of the complex to the rough endoplasmic reticulum. In addition, we provide data that indicate that a majority of the viral RNA species housed within the RC is in a double-stranded RNA (dsRNA) form.West Nile virus (WNV) belongs to the Flaviviridae, which is a large family of enveloped, positive-strand RNA viral pathogens that are responsible for causing severe disease and mortality in humans and animals each year. The Australian WNV strain Kunjin virus (WNV_KUN) is a relatively low-pathogenic virus that is closely related to the pathogenic WNV strain New York 99 (WNV_NY99), the causative agent of the 1999 epidemic of encephalitis in New York City (11).It has become increasingly known that the replication of most, if not all, positive-sense RNA viruses, whether they infect plants, insects, or humans, is associated with dramatic membrane alterations resulting in the formation of membranous microenvironments that facilitate efficient virus replication. In most cases the induced membrane structures house the actively replicating viral RNA and comprise 70- to 100-nm membrane “vesicles” (sometimes referred to as spherules). Although this distinct morphology is shared across virus families, the cellular origins of these membranes is diverse: the endoplasmic reticulum (ER), mitochondria, peroxisomes, and trans-Golgi membranes have been implicated in different viral systems (1, 8, 13, 23, 31, 38, 41, 45). This diversity implies that the processes involved in inducing the membrane vesicles/spherules are shared, rather than the composition of the membrane itself, although the exact purpose for utilizing membranes derived from different cellular compartments is still not completely resolved or understood.The replication of the flavivirus WNV_KUN is associated with the induction of morphologically distinct membrane structures that have defined roles during the WNV_KUN replication cycle. Three well-defined structures can be seen as large convoluted membranes (CM), paracrystalline arrays (PC), or membrane sacs containing small vesicles, termed vesicle packets (VP) (18, 20, 48). Based on localization studies with viral proteins of specific functions, we observed that components of the virus protease complex (namely, nonstructural protein 3 [NS3] with cofactor NS2B) localize specifically to the CM/PC, whereas viral double-stranded RNA (dsRNA) and the viral RNA-dependent RNA polymerase (RdRp) NS5 localized primarily to VP (20-22, 47, 48). Additionally, we observed that the CM and PC originate from and are modified membranes of the intermediate compartment (IC) and rough endoplasmic reticulum (RER), whereas the VP appear to be derived from trans-Golgi network (TGN) membranes (19). Recently, we have found that the WNV_KUN NS4A protein by itself has the intrinsic capacity to induce the CM and PC structures (35), a property also subsequently shown for Dengue virus (DENV) NS4A (29). Additionally, we have shown that upon WNV infection cellular cholesterol and cholesterol-synthesizing proteins are redistributed to the virus-induced membranes and that this redistribution severely disrupted the formation of cholesterol-rich microdomains (23). Furthermore, we have shown that the membranous structures induced during WNV replication provide partial protection of the WNV replication components from the interferon (IFN)-induced antiviral MxA protein, suggesting that the distinct compartmentalization of viral replication and components of the cellular antiviral response may be an evolutionary mechanism by which flaviviruses can protect themselves from host surveillance (6).In this study we focused on three-dimensional (3D) modeling to give insight into the 3D structure of the VP and provide evidence of how these complexes are organized and formed within the RER membrane. These results add valuable information to our understanding of how the WNV replication complex (RC) functions.     

Protein N-Myristoylation Plays a Critical Role in the Endoplasmic Reticulum Morphological Change Induced by Overexpression of Protein Lunapark,an Integral Membrane Protein of the Endoplasmic Reticulum

N-myristoylation of eukaryotic cellular proteins has been recognized as a modification that occurs mainly on cytoplasmic proteins. In this study, we examined the membrane localization, membrane integration, and intracellular localization of four recently identified human N-myristoylated proteins with predicted transmembrane domains. As a result, it was found that protein Lunapark, the human ortholog of yeast protein Lnp1p that has recently been found to be involved in network formation of the endoplasmic reticulum (ER), is an N-myristoylated polytopic integral membrane protein. Analysis of tumor necrosis factor-fusion proteins with each of the two putative transmembrane domains and their flanking regions of protein Lunapark revealed that transmembrane domain 1 and 2 functioned as type II signal anchor sequence and stop transfer sequence, respectively, and together generated a double-spanning integral membrane protein with an N-/C-terminal cytoplasmic orientation. Immunofluorescence staining of HEK293T cells transfected with a cDNA encoding protein Lunapark tagged with FLAG-tag at its C-terminus revealed that overexpressed protein Lunapark localized mainly to the peripheral ER and induced the formation of large polygonal tubular structures. Morphological changes in the ER induced by overexpressed protein Lunapark were significantly inhibited by the inhibition of protein N-myristoylation by means of replacing Gly2 with Ala. These results indicated that protein N-myristoylation plays a critical role in the ER morphological change induced by overexpression of protein Lunapark.