Your search keyword '"Erik L. Snapp"' showing total 84 results

1. Interleukin 2 modulates thymic-derived regulatory T cell epigenetic landscape

Author

Laurent Chorro, Masako Suzuki, Shu Shien Chin, Tere M. Williams, Erik L. Snapp, Livia Odagiu, Nathalie Labrecque, and Grégoire Lauvau

Subjects

Science

Abstract

Regulatory T (Treg) cells are developed in the thymus, and are essential for suppressing detrimental autoimmunity. Here the authors show, using mice with dampened interleukin 2 (IL-2) signaling, that IL-2 helps position the pioneer factor SATB1 to control genome-wide chromatin accessibility to facilitate Treg cell lineage commitment in the thymus.

Published

2018

2. Unfolded Protein Responses With or Without Unfolded Proteins?

Author

Erik L. Snapp

Subjects

unfolded protein response, endoplasmic reticulum, misfolded protein, BIP, stress, Ire1, inositol, Cytology, QH573-671

Abstract

The endoplasmic reticulum (ER) is the site of secretory protein biogenesis. The ER quality control (QC) machinery, including chaperones, ensures the correct folding of secretory proteins. Mutant proteins and environmental stresses can overwhelm the available QC machinery. To prevent and resolve accumulation of misfolded secretory proteins in the ER, cells have evolved integral membrane sensors that orchestrate the Unfolded Protein Response (UPR). The sensors, Ire1p in yeast and IRE1, ATF6, and PERK in metazoans, bind the luminal ER chaperone BiP during homeostasis. As unfolded secretory proteins accumulate in the ER lumen, BiP releases, and the sensors activate. The mechanisms of activation and attenuation of the UPR sensors have exhibited unexpected complexity. A growing body of data supports a model in which Ire1p, and potentially IRE1, directly bind unfolded proteins as part of the activation process. However, evidence for an unfolded protein-independent mechanism has recently emerged, suggesting that UPR can be activated by multiple modes. Importantly, dysregulation of the UPR has been linked to human diseases including Type II diabetes, heart disease, and cancer. The existence of alternative regulatory pathways for UPR sensors raises the exciting possibility for the development of new classes of therapeutics for these medically important proteins.

Published

2012

3. A New Transferrin Receptor Aptamer Inhibits New World Hemorrhagic Fever Mammarenavirus Entry

Author

Keith E Maier, Rohit K Jangra, Kevin R Shieh, David K Cureton, Hui Xiao, Erik L Snapp, Sean P Whelan, Kartik Chandran, and Matthew Levy

Subjects

aptamer, C2.min, Junin, Machupo, mammarenavirus, receptor-mediated endocytosis, SELEX, transferrin receptor, Waz, Therapeutics. Pharmacology, RM1-950

Abstract

Pathogenic New World hemorrhagic fever mammarenaviruses (NWM) utilize Glycoprotein 1 (GP1) to target the apical domain of the human transferrin receptor (hTfR) for facilitating cell entry. However, the conservation between their GP1s is low. Considering this and the slow evolutionary progression of mammals compared to viruses, therapeutic targeting of hTfR provides an attractive avenue for cross-strain inhibition and diminishing the likelihood of escape mutants. Aptamers present unique advantages for the development of inhibitors to vial entry, including ease of synthesis, lack of immunogenicity, and potentially cold-chain breaking solutions to diseases endemic to South America. Here, recognizing that in vivo competition with the natural ligand, transferrin (Tf), likely drove the evolution of GP1 to recognize the apical domain, we performed competitive in vitro selections against hTfR-expressing cells with supplemented Tf. The resultant minimized aptamer, Waz, binds the apical domain of the receptor and inhibits infection of human cells by recombinant NWM in culture (EC50 ≃400 nmol/l). Aptamer multimerization further enhanced inhibition >10-fold (EC50 ≃30 nmol/l). Together, our results highlight the ability to use a competitor to bias the outcome of a selection and demonstrate how avidity effects can be leveraged to enhance both aptamer binding and the potency of viral inhibition.

Published

2016

4. Imaging Cellular Proteins and Structures

Author

Aubrey V. Weigel and Erik L. Snapp

Subjects

Signal-to-noise ratio, Super-resolution microscopy, Chemistry, Biophysics, Cellular proteins

Published

2020

5. Trans -endocytosis of intact IL-15Rα–IL-15 complex from presenting cells into NK cells favors signaling for proliferation

Author

Michael J. Hollander, Eric O. Long, Sumati Rajagopalan, Erik L. Snapp, Olga M. Anton, Thomas A. Waldmann, K. Christopher Garcia, David W. Dorward, Mary E. Peterson, Javier Traba, and Gunjan Arora

Subjects

Multidisciplinary, biology, Chemistry, medicine.medical_treatment, Cell, Biological Sciences, Cell biology, medicine.anatomical_structure, Cytokine, Interleukin 15, Ribosomal protein s6, medicine, biology.protein, Phosphorylation, Gene silencing, Receptor, STAT5

Abstract

Interleukin 15 (IL-15) is an essential cytokine for the survival and proliferation of natural killer (NK) cells. IL-15 activates signaling by the β and common γ (γ(c)) chain heterodimer of the IL-2 receptor through trans-presentation by cells expressing IL-15 bound to the α chain of the IL-15 receptor (IL-15Rα). We show here that membrane-associated IL-15Rα–IL-15 complexes are transferred from presenting cells to NK cells through trans-endocytosis and contribute to the phosphorylation of ribosomal protein S6 and NK cell proliferation. NK cell interaction with soluble or surface-bound IL-15Rα–IL-15 complex resulted in Stat5 phosphorylation and NK cell survival at a concentration or density of the complex much lower than required to stimulate S6 phosphorylation. Despite this efficient response, Stat5 phosphorylation was reduced after inhibition of metalloprotease-induced IL-15Rα–IL-15 shedding from trans-presenting cells, whereas S6 phosphorylation was unaffected. Conversely, inhibition of trans-endocytosis by silencing of the small GTPase TC21 or expression of a dominant-negative TC21 reduced S6 phosphorylation but not Stat5 phosphorylation. Thus, trans-endocytosis of membrane-associated IL-15Rα–IL-15 provides a mode of regulating NK cells that is not afforded to IL-2 and is distinct from activation by soluble IL-15. These results may explain the strict IL-15 dependence of NK cells and illustrate how the cellular compartment in which receptor–ligand interaction occurs can influence functional outcome.

Published

2019

6. Human liver cell trafficking mutants: characterization and whole exome sequencing.

Author

Fei Yuan, Erik L Snapp, Phyllis M Novikoff, Sylvia O Suadicani, David C Spray, Barry Potvin, Allan W Wolkoff, and Pamela Stanley

Subjects

Medicine, Science

Abstract

The HuH7 liver cell mutant Trf1 is defective in membrane trafficking and is complemented by the casein kinase 2α subunit CK2α''. Here we identify characteristic morphologies, trafficking and mutational changes in six additional HuH7 mutants Trf2-Trf7. Trf1 cells were previously shown to be severely defective in gap junction functions. Using a Lucifer yellow transfer assay, remarkable attenuation of gap junction communication was revealed in each of the mutants Trf2-Trf7. Electron microscopy and light microscopy of thiamine pyrophosphatase showed that several mutants exhibited fragmented Golgi apparatus cisternae compared to parental HuH7 cells. Intracellular trafficking was investigated using assays of transferrin endocytosis and recycling and VSV G secretion. Surface binding of transferrin was reduced in all six Trf2-Trf7 mutants, which generally correlated with the degree of reduced expression of the transferrin receptor at the cell surface. The mutants displayed the same transferrin influx rates as HuH7, and for efflux rate, only Trf6 differed, having a slower transferrin efflux rate than HuH7. The kinetics of VSV G transport along the exocytic pathway were altered in Trf2 and Trf5 mutants. Genetic changes unique to particular Trf mutants were identified by exome sequencing, and one was investigated in depth. The novel mutation Ile34Phe in the GTPase RAB22A was identified in Trf4. RNA interference knockdown of RAB22A or overexpression of RAB22AI34F in HuH7 cells caused phenotypic changes characteristic of the Trf4 mutant. In addition, the Ile34Phe mutation reduced both guanine nucleotide binding and hydrolysis activities of RAB22A. Thus, the RAB22A Ile34Phe mutation appears to contribute to the Trf4 mutant phenotype.

Published

2014

7. moxMaple3: a Photoswitchable Fluorescent Protein for PALM and Protein Highlighting in Oxidizing Cellular Environments

Author

Kaberniuk Aa, Manuel A. Mohr, Vladislav V. Verkhusha, and Erik L. Snapp

Subjects

0301 basic medicine, Protein Folding, education, Green Fluorescent Proteins, lcsh:Medicine, 010402 general chemistry, 01 natural sciences, Article, 03 medical and health sciences, Humans, Cysteine, Amino Acids, lcsh:Science, Secretory pathway, chemistry.chemical_classification, Multidisciplinary, Point mutation, lcsh:R, Chromophore, Fusion protein, Fluorescence, Protein tertiary structure, 0104 chemical sciences, Amino acid, Protein Structure, Tertiary, Luminescent Proteins, 030104 developmental biology, Eukaryotic Cells, chemistry, Microscopy, Fluorescence, Biophysics, lcsh:Q, Oxidation-Reduction

Abstract

The ability of fluorescent proteins (FPs) to fold robustly is fundamental to the autocatalytic formation of the chromophore. While the importance of the tertiary protein structure is well appreciated, the impact of individual amino acid mutations for FPs is often not intuitive and requires direct testing. In this study, we describe the engineering of a monomeric photoswitchable FP, moxMaple3, for use in oxidizing cellular environments, especially the eukaryotic secretory pathway. Surprisingly, a point mutation to replace a cysteine substantially improved the yield of correctly folded FP capable of chromophore formation, regardless of cellular environment. The improved folding of moxMaple3 increases the fraction of visibly tagged fusion proteins, as well as FP performance in PALM super-resolution microscopy, and thus makes moxMaple3 a robust monomeric FP choice for PALM and optical highlighting applications.

Published

2018

8. How to design a chalk talk—the million dollar sales pitch

Author

Erik L. Snapp

Subjects

0303 health sciences, Communication, Teaching, Advertising, Cell Biology, Biology, 03 medical and health sciences, 0302 clinical medicine, Research Design, Perspective, ComputingMilieux_COMPUTERSANDEDUCATION, Liberian dollar, Humans, Students, Molecular Biology, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Each faculty recruiting season, many postdocs ask, “What is a chalk talk?” The chalk talk is many things—a sales pitch, a teaching demonstration, a barrage of questions, and a description of a future research program. The chalk talk is arguably the most important component of a faculty search interview. Yet few postdocs or grad students receive training or practice in giving a chalk talk. In the following essay, I’ll cover the basics of chalk talk design and preparation.

Published

2019

9. Structural insights into triglyceride storage mediated by fat storage-inducing transmembrane (FIT) protein 2.

Author

David A Gross, Erik L Snapp, and David L Silver

Subjects

Medicine, Science

Abstract

Fat storage-Inducing Transmembrane proteins 1 & 2 (FIT1/FITM1 and FIT2/FITM2) belong to a unique family of evolutionarily conserved proteins localized to the endoplasmic reticulum that are involved in triglyceride lipid droplet formation. FIT proteins have been shown to mediate the partitioning of cellular triglyceride into lipid droplets, but not triglyceride biosynthesis. FIT proteins do not share primary sequence homology with known proteins and no structural information is available to inform on the mechanism by which FIT proteins function. Here, we present the experimentally-solved topological models for FIT1 and FIT2 using N-glycosylation site mapping and indirect immunofluorescence techniques. These methods indicate that both proteins have six-transmembrane-domains with both N- and C-termini localized to the cytosol. Utilizing this model for structure-function analysis, we identified and characterized a gain-of-function mutant of FIT2 (FLL(157-9)AAA) in transmembrane domain 4 that markedly augmented the total number and mean size of lipid droplets. Using limited-trypsin proteolysis we determined that the FLL(157-9)AAA mutant has enhanced trypsin cleavage at K86 relative to wild-type FIT2, indicating a conformational change. Taken together, these studies indicate that FIT2 is a 6 transmembrane domain-containing protein whose conformation likely regulates its activity in mediating lipid droplet formation.

Published

2010

10. An in vitro compartmentalization-based method for the selection of bond-forming enzymes from large libraries

Author

Paul Gianella, Matthew Levy, and Erik L. Snapp

Subjects

0301 basic medicine, chemistry.chemical_classification, 030102 biochemistry & molecular biology, Chemistry, Mutant, Bioengineering, Directed evolution, Applied Microbiology and Biotechnology, 03 medical and health sciences, In vitro compartmentalization, 030104 developmental biology, Enzyme, Biochemistry, Cytoplasm, Sortase A, Nucleic acid, Enzyme kinetics, Biotechnology

Abstract

We have developed a generalized in vitro compartmentalization-based bead display selection strategy that allows for the identification of enzymes that can perform ligation reactions. Although a number of methods have been developed to evolve such enzymes, many of them are limited in library size (10(6) -10(7) ), do not select for enzymes using a scheme that allows for multiple turnover, or only work on enzymes specific to nucleic acids. This approach is amenable to screening libraries of up to 10(12) protein variants by allowing beads to be overloaded with up to 10(4) unique mutants. Using this approach we isolated a variant of sortase A from Staphylococcus aureus that shows a 114-fold enhancement in kcat /KM in the absence of calcium compared to the wild-type and improved resistance to the inhibitory effects of cell lysates. Unlike the wild-type protein, the newly selected variant shows intracellular activity in the cytoplasm of eukaryotic cells where it may prove useful for intracellular labeling or synthetic biological applications. Biotechnol. Bioeng. 2016;113: 1647-1657. © 2016 Wiley Periodicals, Inc.

Published

2016

11. Interleukin 2 modulates thymic-derived regulatory T cell epigenetic landscape

Author

Nathalie Labrecque, Grégoire Lauvau, Laurent Chorro, Shu Shien Chin, Tere Williams, Livia Odagiu, Masako Suzuki, and Erik L. Snapp

Subjects

0301 basic medicine, Male, General Physics and Astronomy, Autoimmunity, T-Lymphocytes, Regulatory, Epigenesis, Genetic, Mice, 0302 clinical medicine, Listeriosis, lcsh:Science, Multidisciplinary, Thymocytes, FOXP3, hemic and immune systems, Cell Differentiation, Forkhead Transcription Factors, Cellular Reprogramming, humanities, Chromatin, Cell biology, medicine.anatomical_structure, Female, medicine.drug, Signal Transduction, Interleukin 2, Regulatory T cell, Science, T cell, chemical and pharmacologic phenomena, Mice, Transgenic, Thymus Gland, Biology, General Biochemistry, Genetics and Molecular Biology, Article, 03 medical and health sciences, medicine, Animals, Humans, Transcription factor, HEK 293 cells, T-cell receptor, Interleukin-2 Receptor alpha Subunit, General Chemistry, Matrix Attachment Region Binding Proteins, Mice, Inbred C57BL, Disease Models, Animal, 030104 developmental biology, HEK293 Cells, Interleukin-2, lcsh:Q, 030215 immunology

Abstract

Foxp3+CD4+ regulatory T (Treg) cells are essential for preventing fatal autoimmunity and safeguard immune homeostasis in vivo. While expression of the transcription factor Foxp3 and IL-2 signals are both required for the development and function of Treg cells, the commitment to the Treg cell lineage occurs during thymic selection upon T cell receptor (TCR) triggering, and precedes the expression of Foxp3. Whether signals beside TCR contribute to establish Treg cell epigenetic and functional identity is still unknown. Here, using a mouse model with reduced IL-2 signaling, we show that IL-2 regulates the positioning of the pioneer factor SATB1 in CD4+ thymocytes and controls genome wide chromatin accessibility of thymic-derived Treg cells. We also show that Treg cells receiving only low IL-2 signals can suppress endogenous but not WT autoreactive T cell responses in vitro and in vivo. Our findings have broad implications for potential therapeutic strategies to reprogram Treg cells in vivo., Regulatory T (Treg) cells are developed in the thymus, and are essential for suppressing detrimental autoimmunity. Here the authors show, using mice with dampened interleukin 2 (IL-2) signaling, that IL-2 helps position the pioneer factor SATB1 to control genome-wide chromatin accessibility to facilitate Treg cell lineage commitment in the thymus.

Published

2018

12. The Development and Enhancement of FRAP as a Key Tool for Investigating Protein Dynamics

Author

Erik L. Snapp, Robert D. Phair, and Jennifer Lippincott-Schwartz

Subjects

0301 basic medicine, Organelles, education.field_of_study, Chemistry, Protein dynamics, Movement, BJ Classics, Population, Cell Membrane, Biophysics, Fluorescence recovery after photobleaching, Proteins, Fluorescence Photobleaching Recovery, Photobleaching, Cell activity, 03 medical and health sciences, Protein Transport, 030104 developmental biology, 0302 clinical medicine, Proteins metabolism, Membrane dynamics, education, 030217 neurology & neurosurgery, Fluorescence Recovery After Photobleaching

Abstract

The saga of fluorescence recovery after photobleaching (FRAP) illustrates how disparate technical developments impact science. Starting with the classic 1976 Axelrod et al. work in Biophysical Journal, FRAP (originally fluorescence photobleaching recovery) opened the door to extraction of quantitative information from photobleaching experiments, laying the experimental and theoretical groundwork for quantifying both the mobility and the mobile fraction of a labeled population of proteins. Over the ensuing years, FRAP's reach dramatically expanded, with new developments in GFP technology and turn-key confocal microscopy, which enabled measurement of protein diffusion and binding/dissociation rates in virtually every compartment within the cell. The FRAP technique and data catalyzed an exchange of ideas between biophysicists studying membrane dynamics, cell biologists focused on intracellular dynamics, and systems biologists modeling the dynamics of cell activity. The outcome transformed the field of cellular biology, leading to a fundamental rethinking of long-held theories of cellular dynamism. Here, we review the pivotal FRAP studies that made these developments and conceptual changes possible, which gave rise to current models of complex cell dynamics.

Published

2018

13. Engineering and exploitation of a fluorescent HIV-1 gp120 for live cell CD4 binding assays

Author

Harris Goldstein, Betsy C. Herold, Feng Guo, Steven C. Kennedy, Susan C. Irvin, Lindsey M. Costantini, and Erik L. Snapp

Subjects

CD4-Positive T-Lymphocytes, Recombinant Fusion Proteins, viruses, Green Fluorescent Proteins, HIV Infections, HIV Envelope Protein gp120, Article, Green fluorescent protein, Diffusion, Envelope, Viral entry, Virology, Inhibitory antibody, Humans, Neutralizing antibody, chemistry.chemical_classification, biology, Ligand binding assay, virus diseases, Fluorescent protein, Molecular biology, Fusion protein, CD4, Superfolder GFP, 3. Good health, Cell biology, gp120, chemistry, Cell Tracking, HIV-1, FRAP, biology.protein, Receptors, Virus, Laser scanning cytometry, Antibody, Genetic Engineering, Glycoprotein, Intracellular

Abstract

The HIV-1 envelope glycoprotein, gp120, binds the host cell receptor, CD4, in the initial step of HIV viral entry and infection. This process is an appealing target for the development of inhibitory drugs and neutralizing antibodies. To study gp120 binding and intracellular trafficking, we engineered a fluorescent fusion of the humanized gp120 JRFL HIV-1 variant and GFP. Gp120-sfGFP is glycosylated with human sugars, robustly expressed, and secreted from cultured human cells. Protein dynamics, quality control, and trafficking can be visualized in live cells. The fusion protein can be readily modified with different gp120 variants or fluorescent proteins. Finally, secreted gp120-sfGFP enables a sensitive and easy binding assay that can quantitatively screen potential inhibitors of gp120-CD4 binding on live cells via fluorescence imaging or laser scanning cytometry. This adaptable research tool should aid in studies of gp120 cell biology and the development of novel anti-HIV drugs.

Published

2015

14. Structure and topology around the cleavage site regulate post-translational cleavage of the HIV-1 gp160 signal peptide

Author

Ilja Bontjer, Ineke Braakman, IngMarie Nilsson, Matthias Quandte, Carolina Källgren, Aafke Land, Rogier W. Sanders, Erik L. Snapp, Nicholas McCaul, Zuzana Cabartova, Gunnar von Heijne, AII - Infectious diseases, Medical Microbiology and Infection Prevention, Amsterdam institute for Infection and Immunity, Sub Cellular Protein Chemistry, and Cellular Protein Chemistry

Subjects

0301 basic medicine, Signal peptide, Cleavage factor, Protein Conformation, QH301-705.5, Science, viruses, translocation, Target peptide, Protein Sorting Signals, Cleavage (embryo), General Biochemistry, Genetics and Molecular Biology, Cell Line, HIV Envelope Protein gp160, 03 medical and health sciences, Protein structure, Biochemistry and Chemical Biology, protein folding, Humans, signal peptide, Biology (General), General Immunology and Microbiology, Chemistry, General Neuroscience, Endoplasmic reticulum, HIV, virus diseases, Cell Biology, General Medicine, 3. Good health, Protein Transport, endoplasmic reticulum, 030104 developmental biology, gp160, Proteolysis, HIV-1, Biophysics, Medicine, Protein folding, Alpha helix, Research Article, Human

Abstract

Like all other secretory proteins, the HIV-1 envelope glycoprotein gp160 is targeted to the endoplasmic reticulum (ER) by its signal peptide during synthesis. Proper gp160 folding in the ER requires core glycosylation, disulfide-bond formation and proline isomerization. Signal-peptide cleavage occurs only late after gp160 chain termination and is dependent on folding of the soluble subunit gp120 to a near-native conformation. We here detail the mechanism by which co-translational signal-peptide cleavage is prevented. Conserved residues from the signal peptide and residues downstream of the canonical cleavage site form an extended alpha-helix in the ER membrane, which covers the cleavage site, thus preventing cleavage. A point mutation in the signal peptide breaks the alpha helix allowing co-translational cleavage. We demonstrate that postponed cleavage of gp160 enhances functional folding of the molecule. The change to early cleavage results in decreased viral fitness compared to wild-type HIV.

Published

2017

15. Author response: Structure and topology around the cleavage site regulate post-translational cleavage of the HIV-1 gp160 signal peptide

Author

Rogier W. Sanders, Aafke Land, IngMarie Nilsson, Ineke Braakman, Matthias Quandte, Carolina Källgren, Nicholas McCaul, Ilja Bontjer, Gunnar von Heijne, Zuzana Cabartova, and Erik L. Snapp

Subjects

Signal peptide, Post translational, Chemistry, Stereochemistry, Human immunodeficiency virus (HIV), medicine, medicine.disease_cause, Cleavage (embryo), Topology (chemistry)

Published

2017

16. moxDendra2: an inert photoswitchable protein for oxidizing environments

Author

Nicholas C. Morano, Kaberniuk Aa, Vladislav V. Verkhusha, and Erik L. Snapp

Subjects

0301 basic medicine, animal structures, education, Golgi Apparatus, Nanotechnology, complex mixtures, Catalysis, Article, 03 medical and health sciences, Organelle, Oxidizing agent, Materials Chemistry, Animals, Humans, Amino Acid Sequence, Fluorescent Dyes, biology, Chemistry, fungi, Metals and Alloys, food and beverages, General Chemistry, biology.organism_classification, Anthozoa, Photochemical Processes, Fluorescence, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Luminescent Proteins, 030104 developmental biology, Microscopy, Fluorescence, Cytoplasm, Ceramics and Composites, Biophysics, Oxidation-Reduction, Sequence Alignment, Bacteria, HeLa Cells

Abstract

Fluorescent proteins (FPs) that can be optically highlighted enable PALM super-resolution microscopy and pulse-chase experiments of cellular molecules. Most FPs evolved in cytoplasmic environments either in the original source organism or in the cytoplasm of bacteria during the course of optimization for research applications. Consequently, many FPs may fold incorrectly in the chemically distinct environments in subcellular organelles. Here, we describe the first monomeric photoswitchable (from green to bright red) FP adapted for oxidizing environments.

Published

2017

17. Imaging the Alphavirus Exit Pathway

Author

Geoffrey S. Perumal, Maria Guadalupe Martinez, Erik L. Snapp, Frank P. Macaluso, and Margaret Kielian

Subjects

Sindbis virus, viruses, Immunology, Alphavirus, Microbiology, Virus, Cell Line, VP40, Viral envelope, Virology, Animals, Humans, Viral shedding, Instrumentation, Virus Release, Budding, biology, Alphavirus Infections, Chemistry, Virus Assembly, Cell Membrane, Viral membrane, biology.organism_classification, Transmembrane protein, Virus-Cell Interactions, Cell biology, Capsid, Insect Science, Sindbis Virus, Fluorescence Recovery After Photobleaching

Abstract

Alphaviruses are small enveloped RNA viruses with highly organized structures that exclude host cell proteins. They contain an internal nucleocapsid and an external lattice of the viral E2 and E1 transmembrane proteins. Alphaviruses bud from the plasma membrane (PM), but the process and dynamics of alphavirus assembly and budding are poorly understood. Here we generated Sindbis viruses (SINVs) with fluorescent protein labels on the E2 envelope protein and exploited them to characterize virus assembly and budding in living cells. During virus infection, E2 became enriched in localized patches on the PM and in filopodium-like extensions. These E2-labeled patches and extensions contained all of the viral structural proteins. Correlative light and electron microscopy studies established that the patches and extensions colocalized with virus budding structures, while light microscopy showed that they excluded a freely diffusing PM marker protein. Exclusion required the interaction of the E2 protein with the capsid protein, a critical step in virus budding, and was associated with the immobilization of the envelope proteins on the cell surface. Virus infection induced two distinct types of extensions: tubulin-negative extensions that were ∼2 to 4 μm in length and excluded the PM marker, and tubulin-positive extensions that were >10 μm long, contained the PM marker, and could transfer virus particles to noninfected cells. Tubulin-positive extensions were selectively reduced in cells infected with a nonbudding SINV mutant. Together, our data support a model in which alphavirus infection induces reorganization of the PM and cytoskeleton, leading to virus budding from specialized sites. IMPORTANCE Alphaviruses are important and widely distributed human pathogens for which vaccines and antiviral therapies are urgently needed. These small highly organized viruses bud from the host cell PM. Virus assembly and budding are critical but little understood steps in the alphavirus life cycle. We developed alphaviruses with fluorescent protein tags on one of the viral membrane (envelope) proteins and used a variety of microscopy techniques to follow the envelope protein and a host cell PM protein during budding. We showed that alphavirus infection induced the formation of patches and extensions on the PM where the envelope proteins accumulate. These sites excluded other PM proteins and correlated with virus budding structures. Exclusion of PM proteins required specific interactions of the viral envelope proteins with the internal capsid protein. Together, our data indicate that alphaviruses extensively reorganize the cell surface and cytoskeleton to promote their assembly and budding.

Published

2014

18. Biochemical and Cellular Analysis of Human Variants of the DYT1 Dystonia Protein, TorsinA/TOR1A

Author

Xandra O. Breakefield, Rashmi Kothary, Shelun Tsai, Kathrin Grundmann, Flávia C. Nery, Cintia Carla da Hora, Luis Fernando Saraiva Macedo Timmers, Xuan Zhang, Jasmin Hettich, Osmar Norberto de Souza, Nadia A. Atai, Erik L. Snapp, Maria Ericsson, Scott D. Ryan, Amsterdam Gastroenterology Endocrinology Metabolism, Cancer Center Amsterdam, and Cell Biology and Histology

Subjects

Models, Molecular, Protein family, Protein Conformation, Dystonia Musculorum Deformans, Biology, Molecular Dynamics Simulation, Bioinformatics, Endoplasmic Reticulum, Article, Viral Envelope Proteins, Genetics, medicine, Missense mutation, Humans, Genetics (clinical), Genetic Association Studies, Dystonia, Genetic Variation, Focal dystonia, Fibroblasts, medicine.disease, Phenotype, Protein Transport, Gene Knockdown Techniques, Mutation, Unfolded protein response, medicine.symptom, Protein Multimerization, Myoclonus, Molecular Chaperones

Abstract

Early-onset dystonia is associated with the deletion of one of a pair of glutamic acid residues (c.904_906delGAG/c.907_909delGAG; p.Glu302del/Glu303del; ΔE 302/303) near the carboxyl-terminus of torsinA, a member of the AAA+ protein family that localizes to the endoplasmic reticulum (ER) lumen and nuclear envelope (NE). This deletion commonly underlies early-onset DYT1 dystonia. While the role of the disease-causing mutation, torsinAΔE, has been established through genetic association studies, it is much less clear whether other rare human variants of torsinA are pathogenic. Two missense variations have been described in single patients; R288Q (c.863G>A; p.Arg288Gln; R288Q) identified in a patient with onset of severe generalized dystonia and myoclonus since infancy, and F205I (c.613T>A, p.Phe205Ile; F205I) in a psychiatric patient with late-onset focal dystonia. In this study, we have undertaken a series of analyses comparing the biochemical and cellular effects of these rare variants to torsinAΔE and wild-type (wt) torsinA in order to reveal whether there are common dysfunctional features. The results revealed that the variants, R288Q and F205I, are more similar in their properties to torsinAΔE protein than to torsinAwt. These findings provide functional evidence for the potential pathogenic nature of these rare sequence variants in the TOR1A gene, thus implicating these pathologies in the development of dystonia.

Published

2014

19. Cysteineless non-glycosylated monomeric blue fluorescent protein, secBFP2, for studies in the eukaryotic secretory pathway

Author

Lindsey M. Costantini, Vladislav V. Verkhusha, Erik L. Snapp, Matías Jaureguiberry-Bravo, and Oksana M. Subach

Subjects

Protein Folding, Glycosylation, Molecular Sequence Data, Biophysics, Biology, Endoplasmic Reticulum, Protein Engineering, Biochemistry, Article, chemistry.chemical_compound, N-linked glycosylation, Cell Line, Tumor, Humans, Amino Acid Sequence, Cysteine, Molecular Biology, Secretory pathway, Secretory Pathway, Endoplasmic reticulum, Cell Biology, Protein engineering, Luminescent Proteins, Eukaryotic Cells, Secretory protein, Amino Acid Substitution, chemistry, Mutagenesis, Cytoplasm, Protein folding, Protein Processing, Post-Translational

Abstract

Fluorescent protein (FP) technologies suitable for use within the eukaryotic secretory pathway are essential for live cell and protein dynamic studies. Localization of FPs within the endoplasmic reticulum (ER) lumen has potentially significant consequences for FP function. All FPs are resident cytoplasmic proteins and have rarely been evolved for the chemically distinct environment of the ER lumen. In contrast to the cytoplasm, the ER lumen is oxidizing and the site where secretory proteins are post-translationally modified by disulfide bond formation and N-glycosylation on select asparagine residues. Cysteine residues and N-linked glycosylation consensus sequences were identified within many commonly utilized FPs. Here, we report mTagBFP is post-translationally modified when localized to the ER lumen. Our findings suggest these modifications can grossly affect the sensitivity and reliability of FP tools within the secretory pathway. To optimize tools for studying events in this important intracellular environment, we modified mTagBFP by mutating its cysteines and consensus N-glycosylation sites. We report successful creation of a secretory pathway-optimized blue FP, secBFP2.

Published

2013

20. Proinsulin Intermolecular Interactions during Secretory Trafficking in Pancreatic β Cells

Author

Michael B. Wheeler, Jordan J. Wright, Alexandre B. Hardy, Michele L. Markwardt, Erik L. Snapp, Megan A. Rizzo, Ming Liu, Peter Arvan, and Leena Haataja

Subjects

Protein Folding, endocrine system, endocrine system diseases, Green Fluorescent Proteins, Gene Expression, Golgi Apparatus, Biology, Endoplasmic Reticulum, Transfection, digestive system, Biochemistry, Mice, chemistry.chemical_compound, symbols.namesake, Cell Line, Tumor, Insulin-Secreting Cells, Chlorocebus aethiops, Animals, Humans, Insulin, Protein precursor, Molecular Biology, Proinsulin, Microscopy, Confocal, C-Peptide, C-peptide, Endoplasmic reticulum, nutritional and metabolic diseases, Cell Biology, Golgi apparatus, Rats, Transport protein, Kinetics, Protein Transport, Secretory protein, chemistry, COS Cells, symbols, Protein folding, Dimerization, hormones, hormone substitutes, and hormone antagonists, Plasmids, Protein Binding

Abstract

Classically, exit from the endoplasmic reticulum (ER) is rate-limiting for secretory protein trafficking because protein folding/assembly occurs there. In this study, we have exploited "hPro-CpepSfGFP," a human proinsulin bearing "superfolder" green fluorescent C-peptide expressed in pancreatic β cells where it is processed to human insulin and CpepSfGFP. Remarkably, steady-state accumulation of hPro-CpepSfGFP and endogenous proinsulin is in the Golgi region, as if final stages of protein folding/assembly were occurring there. The Golgi regional distribution of proinsulin is dynamic, influenced by fasting/refeeding, and increased with β cell zinc deficiency. However, coexpression of ER-entrapped mutant proinsulin-C(A7)Y shifts the steady-state distribution of wild-type proinsulin to the ER. Endogenous proinsulin coprecipitates with hPro-CpepSfGFP and even more so with hProC(A7)Y-CpepSfGFP. Using Cerulean and Venus-tagged proinsulins, we find that both WT-WT and WT-mutant proinsulin pairs exhibit FRET. The data demonstrate that wild-type proinsulin dimerizes within the ER but accumulates at a poorly recognized slow step within the Golgi region, reflecting either slow kinetics of proinsulin hexamerization, steps in formation of nascent secretory granules, or other unknown molecular events. However, in the presence of ongoing misfolding of a subpopulation of proinsulin in β cells, the rate-limiting step in transport of the remaining proinsulin shifts to the ER.

Published

2013

21. A New Transferrin Receptor Aptamer Inhibits New World Hemorrhagic Fever Mammarenavirus Entry

Author

Rohit K. Jangra, David K. Cureton, Kevin Shieh, Matthew Levy, Erik L. Snapp, Sean P. J. Whelan, Hui Xiao, Kartik Chandran, and Keith E. Maier

Subjects

0301 basic medicine, receptor-mediated endocytosis, Waz, Aptamer, Transferrin receptor, Biology, 03 medical and health sciences, Drug Discovery, Avidity, chemistry.chemical_classification, mammarenavirus, SELEX, Immunogenicity, lcsh:RM1-950, aptamer, Junin, Receptor-mediated endocytosis, transferrin receptor, Ligand (biochemistry), Virology, Machupo, lcsh:Therapeutics. Pharmacology, 030104 developmental biology, chemistry, Transferrin, Molecular Medicine, Systematic evolution of ligands by exponential enrichment, C2.min

Abstract

Pathogenic New World hemorrhagic fever mammarenaviruses (NWM) utilize Glycoprotein 1 (GP1) to target the apical domain of the human transferrin receptor (hTfR) for facilitating cell entry. However, the conservation between their GP1s is low. Considering this and the slow evolutionary progression of mammals compared to viruses, therapeutic targeting of hTfR provides an attractive avenue for cross-strain inhibition and diminishing the likelihood of escape mutants. Aptamers present unique advantages for the development of inhibitors to vial entry, including ease of synthesis, lack of immunogenicity, and potentially cold-chain breaking solutions to diseases endemic to South America. Here, recognizing that in vivo competition with the natural ligand, transferrin (Tf), likely drove the evolution of GP1 to recognize the apical domain, we performed competitive in vitro selections against hTfR-expressing cells with supplemented Tf. The resultant minimized aptamer, Waz, binds the apical domain of the receptor and inhibits infection of human cells by recombinant NWM in culture (EC50 ≃400 nmol/l). Aptamer multimerization further enhanced inhibition >10-fold (EC50 ≃30 nmol/l). Together, our results highlight the ability to use a competitor to bias the outcome of a selection and demonstrate how avidity effects can be leveraged to enhance both aptamer binding and the potency of viral inhibition.

Published

2016

22. ERdj4 Protein Is a Soluble Endoplasmic Reticulum (ER) DnaJ Family Protein That Interacts with ER-associated Degradation Machinery

Author

Chunwei Walter Lai, Joel H. Otero, Linda M. Hendershot, and Erik L. Snapp

Subjects

Vesicle-associated membrane protein 8, Membrane Glycoproteins, Endoplasmic reticulum, Peripheral membrane protein, Membrane Proteins, Endoplasmic Reticulum-Associated Degradation, Intracellular Membranes, Cell Biology, Protein Sorting Signals, Biology, Endoplasmic-reticulum-associated protein degradation, Endoplasmic Reticulum, Models, Biological, Biochemistry, Cell Line, Cell biology, Transport protein, Mice, Protein Transport, Dogs, Membrane protein, Unfolded protein response, Animals, Molecular Biology, Integral membrane protein

Abstract

Protein localization within cells regulates accessibility for interactions with co-factors and substrates. The endoplasmic reticulum (ER) BiP co-factor ERdj4 is up-regulated by ER stress and has been implicated in ER-associated degradation (ERAD) of multiple unfolded secretory proteins. Several other ERdj family members tend to interact selectively with nascent proteins, presumably because those ERdj proteins associate with the Sec61 translocon that facilitates entry of nascent proteins into the ER. How ERdj4 selects and targets terminally misfolded proteins for destruction remains poorly understood. In this study, we determined properties of ERdj4 that might aid in this function. ERdj4 was reported to retain its signal sequence and to be resistant to mild detergent extraction, suggesting that it was an integral membrane protein. However, live cell photobleaching analyses of GFP-tagged ERdj4 revealed that the protein exhibits diffusion coefficients uncommonly high for an ER integral membrane protein and more similar to the mobility of a soluble luminal protein. Biochemical characterization established that the ERdj4 signal sequence is cleaved to yield a soluble protein. Importantly, we found that both endogenous and overexpressed ERdj4 associate with the integral membrane protein, Derlin-1. Our findings now directly link ERdj4 to the ERAD machinery and suggest a model in which ERjd4 could help recruit clients from throughout the ER to ERAD sites.

Published

2012

23. Assessing the Tendency of Fluorescent Proteins to Oligomerize Under Physiologic Conditions

Author

Matteo Fossati, Lindsey M. Costantini, Erik L. Snapp, and Maura Francolini

Subjects

animal structures, Endoplasmic reticulum, Cell Biology, Biology, Biochemistry, Fluorescence, Green fluorescent protein, Cell biology, Cytosol, Membrane, Membrane protein, Structural Biology, Cytoplasm, Genetics, Signal transduction, Molecular Biology

Abstract

Several fluorescent proteins (FPs) are prone to forming low-affinity oligomers. This undesirable tendency is exacerbated when FPs are confined to membranes or when fused to naturally oligomeric proteins. Oligomerization of FPs limits their suitability for creating fusions with proteins of interest. Unfortunately, no standardized method evaluates the biologically relevant oligomeric state of FPs. Here, we describe a quantitative visual assay for assessing whether FPs are sufficiently monomeric under physiologic conditions. Membrane-associated FP-fusion proteins, by virtue of their constrained planar geometry, achieve high effective concentrations. We exploited this propensity to develop an assay to measure FP tendencies to oligomerize in cells. FPs were fused on the cytoplasmic end of an endoplasmic reticulum (ER) signal-anchor membrane protein (CytERM) and expressed in cells. Cells were scored based on the ability of CytERM to homo-oligomerize with proteins on apposing membranes and restructure the ER from a tubular network into organized smooth ER (OSER) whorl structures. The ratio of nuclear envelope and OSER structures mean fluorescent intensities for cells expressing enhanced green fluorescent protein (EGFP) or monomeric green fluorescent protein (mGFP) CytERM established standards for comparison of uncharacterized FPs. We tested three FPs and identified two as sufficiently monomeric, while a third previously reported as monomeric was found to strongly oligomerize.

Published

2012

24. Sec24p and Sec16p cooperate to regulate the GTP cycle of the COPII coat

Author

Eugene Futai, Erik L. Snapp, Randy Schekman, Robert J.D. Reid, Rodney Rothstein, Susan Hamamoto, Jennifer G. D’Arcangelo, Silvere Pagant, John C. Dittmar, Leslie Kung, Roy Buchanan, and Elizabeth A. Miller

Subjects

General Immunology and Microbiology, GTP', General Neuroscience, Vesicle, Endoplasmic reticulum, COPI, COP-Coated Vesicles, Biology, General Biochemistry, Genetics and Molecular Biology, Cell biology, Molecular Biology, COPII, Secretory pathway, Vesicle scission

Abstract

Vesicle budding from the endoplasmic reticulum (ER) employs a cycle of GTP binding and hydrolysis to regulate assembly of the COPII coat. We have identified a novel mutation (sec24-m11) in the cargo-binding subunit, Sec24p, that specifically impacts the GTP-dependent generation of vesicles in vitro. Using a high-throughput approach, we defined genetic interactions between sec24-m11 and a variety of trafficking components of the early secretory pathway, including the candidate COPII regulators, Sed4p and Sec16p. We defined a fragment of Sec16p that markedly inhibits the Sec23p- and Sec31p-stimulated GTPase activity of Sar1p, and demonstrated that the Sec24p-m11 mutation diminished this inhibitory activity, likely by perturbing the interaction of Sec24p with Sec16p. The consequence of the heightened GTPase activity when Sec24p-m11 is present is the generation of smaller vesicles, leading to accumulation of ER membranes and more stable ER exit sites. We propose that association of Sec24p with Sec16p creates a novel regulatory complex that retards the GTPase activity of the COPII coat to prevent premature vesicle scission, pointing to a fundamental role for GTP hydrolysis in vesicle release rather than in coat assembly/disassembly.

Published

2011

25. Mechanism of Collapse of Endoplasmic Reticulum Cisternae During African Swine Fever Virus Infection

Author

Javier M. Rodríguez, Thomas Wileman, Philippa C. Hawes, María L. Salas, Paul Monaghan, Miriam Windsor, Erik L. Snapp, Ministerio de Ciencia e Innovación (España), Fundación Ramón Areces, and National Institutes of Health (US)

Subjects

Cell Culture Techniques, Fluorescent Antibody Technique, Cisternal collapse, Biology, Transfection, Biochemistry, African swine fever virus, Article, Viral Proteins, Protein structure, Microscopy, Electron, Transmission, Viral Envelope Proteins, Viral envelope, Structural Biology, Chlorocebus aethiops, Genetics, Animals, Vero Cells, Molecular Biology, Virus Assembly, Endoplasmic reticulum, Intracellular Membranes, Cell Biology, Viral envelope protein, biology.organism_classification, Protein Structure, Tertiary, Cell biology, Cell culture, Cytoplasm, Biogenesis, Plasmids

Abstract

Infection of cells with African swine fever virus (ASFV) can lead to the formation of zipper-like stacks of structural proteins attached to collapsed endoplasmic reticulum (ER) cisternae. We show that the collapse of ER cisternae observed during ASFV infection is dependent on the viral envelope protein, J13Lp. Expression of J13Lp alone in cells is sufficient to induce collapsed ER cisternae. Collapse was dependent on a cysteine residue in the N-terminal domain of J13Lp exposed to the ER lumen. Luminal collapse was also dependent on the expression of J13Lp within stacks of ER where antiparallel interactions between the cytoplasmic domains of J13Lp orientated N-terminal domains across ER cisternae. Cisternal collapse was then driven by disulphide bonds between N-terminal domains arranged in antiparallel arrays across the ER lumen. This provides a novel mechanism for biogenesis of modified stacks of ER present in cells infected with ASFV, and may also be relevant to cellular processes. © 2011 John Wiley & Sons A/S., Spanish Ministerio de Ciencia e Innovación (AGL2010-22229-C03-02); Fundación Ramón Areces; NIA 1R21AG032544-01; NIGMS 1RO1GM086530-01; NIDDK 2PO1DK041918-16

Published

2011

26. Alcohol Disrupts Endoplasmic Reticulum Function and Protein Secretion in Hepatocytes

Author

Ana M. Vacaru, Lindsey M. Costantini, Orkhontuya Tsedensodnom, Natalia Nieto, Kirsten C. Sadler, Erik L. Snapp, Deanna L. Howarth, and Elisabetta Mormone

Subjects

Endoplasmic reticulum, Medicine (miscellaneous), Biology, Toxicology, biology.organism_classification, Molecular biology, Cell biology, Psychiatry and Mental health, Secretory protein, medicine.anatomical_structure, Apoptosis, Hepatocyte, medicine, biology.protein, Unfolded protein response, Ethanol metabolism, Zebrafish, Alcohol dehydrogenase

Abstract

Background: Many alcoholic patients have serum protein deficiency that contributes to their systemic problems. The unfolded protein response (UPR) is induced in response to disequilibrium in the protein folding capability of the endoplasmic reticulum (ER) and is implicated in hepatocyte lipid accumulation and apoptosis, which are associated with alcoholic liver disease (ALD). We investigated whether alcohol affects ER structure, function, and UPR activation in hepatocytes in vitro and in vivo. Methods: HepG2 cells expressing human cytochrome P450 2E1 and mouse alcohol dehydrogenase (VL-17A) were treated for up to 48 hours with 50 and 100 mM ethanol. Zebrafish larvae at 4 days postfertilization were exposed to 350 mM ethanol for 32 hours. ER morphology was visualized by fluorescence in cells and transmission electron microscopy in zebrafish. UPR target gene activation was assessed using quantitative PCR, in situ hybridization, and Western blotting. Mobility of the major ER chaperone, BIP, was monitored in cells by fluorescence recovery after photobleaching (FRAP). Results: VL-17A cells metabolized alcohol yet only had slight activation of some UPR target genes following ethanol treatment. However, ER fragmentation, crowding, and accumulation of unfolded proteins as detected by immunofluorescence and FRAP demonstrate that alcohol induced some ER dysfunction despite the lack of UPR activation. Zebrafish treated with alcohol, however, showed modest ER dilation, and several UPR targets were significantly induced. Conclusions: Ethanol metabolism directly impairs ER structure and function in hepatocytes. Zebrafish are a novel in vivo system for studying ALD.

Published

2011

27. Static retention of the lumenal monotopic membrane protein torsinA in the endoplasmic reticulum

Author

Erik L. Snapp, Abigail B. Vander Heyden, Phyllis I. Hanson, and Teresa V. Naismith

Subjects

General Immunology and Microbiology, General Neuroscience, Endoplasmic reticulum, ER retention, Biology, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, Cell biology, Transport protein, Cell membrane, Transmembrane domain, medicine.anatomical_structure, Biochemistry, Membrane protein, Protein targeting, medicine, Molecular Biology, Peptide sequence

Abstract

TorsinA is a membrane-associated enzyme in the endoplasmic reticulum (ER) lumen that is mutated in DYT1 dystonia. How it remains in the ER has been unclear. We report that a hydrophobic N-terminal domain (NTD) directs static retention of torsinA within the ER by excluding it from ER exit sites, as has been previously reported for short transmembrane domains (TMDs). We show that despite the NTD's physicochemical similarity to TMDs, it does not traverse the membrane, defining torsinA as a lumenal monotopic membrane protein and requiring a new paradigm to explain retention. ER retention and membrane association are perturbed by a subset of nonconservative mutations to the NTD, suggesting that a helical structure with defined orientation in the membrane is required. TorsinA preferentially enriches in ER sheets, as might be expected for a lumenal monotopic membrane protein. We propose that the principle of membrane-based protein sorting extends to monotopic membrane proteins, and identify other proteins including the monotopic lumenal enzyme cyclooxygenase 1 (prostaglandin H synthase 1) that share this mechanism of retention with torsinA.

Published

2011

28. BiP Availability Distinguishes States of Homeostasis and Stress in the Endoplasmic Reticulum of Living Cells

Author

Chun Wei Lai, Erik L. Snapp, and Deborah E. Aronson

Subjects

Cell type, Protein Folding, genetic structures, Cell Survival, Recombinant Fusion Proteins, Biosynthesis and Biodegradation, Green Fluorescent Proteins, Biology, Endoplasmic Reticulum, Transfection, Cell Line, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, JUNQ and IPOD, Genes, Reporter, Stress, Physiological, Cricetinae, Animals, Homeostasis, Humans, Molecular Biology, Endoplasmic Reticulum Chaperone BiP, Heat-Shock Proteins, 030304 developmental biology, 0303 health sciences, Viscosity, Endoplasmic reticulum, Cell Biology, Tunicamycin, Articles, Cell biology, Secretory protein, chemistry, Unfolded protein response, Protein folding, 030217 neurology & neurosurgery

Abstract

BiP availability represents a powerful tool for reporting global secretory protein misfolding levels and investigating the molecular events of ER stress in single cells, independent of traditional UPR markers., Accumulation of misfolded secretory proteins causes cellular stress and induces the endoplasmic reticulum (ER) stress pathway, the unfolded protein response (UPR). Although the UPR has been extensively studied, little is known about the molecular changes that distinguish the homeostatic and stressed ER. The increase in levels of misfolded proteins and formation of complexes with chaperones during ER stress are predicted to further crowd the already crowded ER lumen. Surprisingly, using live cell fluorescence microscopy and an inert ER reporter, we find the crowdedness of stressed ER, treated acutely with tunicamycin or DTT, either is comparable to homeostasis or significantly decreases in multiple cell types. In contrast, photobleaching experiments revealed a GFP-tagged variant of the ER chaperone BiP rapidly undergoes a reversible quantitative decrease in diffusion as misfolded proteins accumulate. BiP mobility is sensitive to exceptionally low levels of misfolded protein stressors and can detect intermediate states of BiP availability. Decreased BiP availability temporally correlates with UPR markers, but restoration of BiP availability correlates less well. Thus, BiP availability represents a novel and powerful tool for reporting global secretory protein misfolding levels and investigating the molecular events of ER stress in single cells, independent of traditional UPR markers.

Published

2010

29. An in vitro compartmentalization-based method for the selection of bond-forming enzymes from large libraries

Author

Paul, Gianella, Erik L, Snapp, and Matthew, Levy

Subjects

Models, Molecular, Staphylococcus aureus, Escherichia coli Proteins, Aminoacyltransferases, Protein Engineering, Article, Repressor Proteins, Cysteine Endopeptidases, Kinetics, Bacterial Proteins, Peptide Library, Escherichia coli, Carbon-Nitrogen Ligases, Cloning, Molecular, Protein Binding

Abstract

We have developed a generalized in vitro compartmentalization-based bead display selection strategy that allows for the identification of enzymes that can perform ligation reactions. Although a number of methods have been developed to evolve such enzymes, many of them are limited in library size (10(6) -10(7) ), do not select for enzymes using a scheme that allows for multiple turnover, or only work on enzymes specific to nucleic acids. This approach is amenable to screening libraries of up to 10(12) protein variants by allowing beads to be overloaded with up to 10(4) unique mutants. Using this approach we isolated a variant of sortase A from Staphylococcus aureus that shows a 114-fold enhancement in kcat /KM in the absence of calcium compared to the wild-type and improved resistance to the inhibitory effects of cell lysates. Unlike the wild-type protein, the newly selected variant shows intracellular activity in the cytoplasm of eukaryotic cells where it may prove useful for intracellular labeling or synthetic biological applications. Biotechnol. Bioeng. 2016;113: 1647-1657. © 2016 Wiley Periodicals, Inc.

Published

2015

30. Connexin Type and Fluorescent Protein Fusion Tag Determine Structural Stability of Gap Junction Plaques*

Author

Randy F. Stout, David C. Spray, and Erik L. Snapp

Subjects

Protein Conformation, C-terminus, Gap junction, Fluorescence recovery after photobleaching, Connexin, Gap Junctions, Cell Biology, Biology, Biochemistry, Connexins, Connexin binding, Connexin 26, Luminescent Proteins, Protein structure, Cytoplasm, Biophysics, otorhinolaryngologic diseases, Connexin 30, Humans, sense organs, Molecular Biology, Intracellular, HeLa Cells

Abstract

Gap junctions (GJs) are made up of plaques of laterally clustered intercellular channels and the membranes in which the channels are embedded. Arrangement of channels within a plaque determines subcellular distribution of connexin binding partners and sites of intercellular signaling. Here, we report the discovery that some connexin types form plaque structures with strikingly different degrees of fluidity in the arrangement of the GJ channel subcomponents of the GJ plaque. We uncovered this property of GJs by applying fluorescence recovery after photobleaching to GJs formed from connexins fused with fluorescent protein tags. We found that connexin 26 (Cx26) and Cx30 GJs readily diffuse within the plaque structures, whereas Cx43 GJs remain persistently immobile for more than 2 min after bleaching. The cytoplasmic C terminus of Cx43 was required for stability of Cx43 plaque arrangement. We provide evidence that these qualitative differences in GJ arrangement stability reflect endogenous characteristics, with the caveat that the sizes of the GJs examined were necessarily large for these measurements. We also uncovered an unrecognized effect of non-monomerized fluorescent protein on the dynamically arranged GJs and the organization of plaques composed of multiple connexin types. Together, these findings redefine our understanding of the GJ plaque structure and should be considered in future studies using fluorescent protein tags to probe dynamics of highly ordered protein complexes.

Published

2015

31. Going Viral with Fluorescent Proteins

Author

Erik L. Snapp and Lindsey M. Costantini

Subjects

Models, Molecular, Viral protein, Extramural, Immunology, Optical Imaging, Computational biology, Biology, medicine.disease_cause, Bioinformatics, Microbiology, Luminescent Proteins, Cellular Microenvironment, Insect Science, Virology, medicine, Fluorescent protein, Viral Fusion Proteins, Cellular localization, Gems

Abstract

Many longstanding questions about dynamics of virus-cell interactions can be answered by combining fluorescence imaging techniques with fluorescent protein (FP) tagging strategies. Successfully creating a FP fusion with a cellular or viral protein of interest first requires selecting the appropriate FP. However, while viral architecture and cellular localization often dictate the suitability of a FP, a FP's chemical and physical properties must also be considered. Here, we discuss the challenges of and offer suggestions for identifying the optimal FPs for studying the cell biology of viruses.

Published

2015

32. A palette of fluorescent proteins optimized for diverse cellular environments

Author

Mikhail Baloban, Megan A. Rizzo, Lindsey M. Costantini, Feng Guo, Erik L. Snapp, Michele L. Markwardt, and Vladislav V. Verkhusha

Subjects

Green Fluorescent Proteins, General Physics and Astronomy, Biology, Article, General Biochemistry, Genetics and Molecular Biology, Madin Darby Canine Kidney Cells, Green fluorescent protein, 03 medical and health sciences, Dogs, 0302 clinical medicine, Bacterial Proteins, Live cell imaging, Cell Line, Tumor, Organelle, Animals, Humans, Secretory pathway, Cellular compartment, Fluorescent Dyes, 030304 developmental biology, 0303 health sciences, Multidisciplinary, Staining and Labeling, Cell Membrane, Optical Imaging, Biological membrane, General Chemistry, Protein subcellular localization prediction, Transmembrane protein, Cell biology, Luminescent Proteins, Microscopy, Fluorescence, 030217 neurology & neurosurgery, HeLa Cells

Abstract

To perform quantitative live cell imaging, investigators require fluorescent reporters that accurately report protein localization and levels, while minimally perturbing the cell. Yet, within the biochemically distinct environments of cellular organelles, popular fluorescent proteins (FPs), including EGFP, can be unreliable for quantitative imaging, resulting in the underestimation of protein levels and incorrect localization. Specifically, within the secretory pathway, significant populations of FPs misfold and fail to fluoresce due to non-native disulphide bond formation. Furthermore, transmembrane FP-fusion constructs can disrupt organelle architecture due to oligomerizing tendencies of numerous common FPs. Here, we describe a powerful set of bright and inert FPs optimized for use in multiple cellular compartments, especially oxidizing environments and biological membranes. Also, we provide new insights into the use of red FPs in the secretory pathway. Our monomeric ‘oxFPs’ finally resolve long-standing, underappreciated and important problems of cell biology and should be useful for a number of applications. Quantitative live cell imaging of protein trafficking suffers from misfolding and inappropriate disulphide bond formation of fluorescent proteins in the secretory pathway. Here, the authors present an optimized collection of fluorescent proteins suitable for use in oxidizing subcellular compartments.

Published

2015

33. Golgi Inheritance in Mammalian Cells Is Mediated through Endoplasmic Reticulum Export Activities

Author

Theresa H. Ward, Rachid Sougrat, Wei Liu, Jennifer Lippincott-Schwartz, Erik L. Snapp, and Nihal Altan-Bonnet

Subjects

Recombinant Fusion Proteins, Golgi Apparatus, Golgi reassembly, Biology, Endoplasmic Reticulum, Models, Biological, GTP Phosphohydrolases, symbols.namesake, Animals, Golgi inheritance, Telophase, Molecular Biology, Mitosis, Secretory pathway, Ionophores, Ionomycin, Nocodazole, Endoplasmic reticulum, Articles, Cell Biology, Cell plate, Golgi apparatus, Galactosyltransferases, Rats, Cell biology, Luminescent Proteins, Microscopy, Fluorescence, symbols, ADP-Ribosylation Factor 1, Cattle, Cell Division

Abstract

Golgi inheritance during mammalian cell division occurs through the disassembly, partitioning, and reassembly of Golgi membranes. The mechanisms responsible for these processes are poorly understood. To address these mechanisms, we have examined the identity and dynamics of Golgi proteins within mitotic membranes using live cell imaging and electron microscopy techniques. Mitotic Golgi fragments, seen in prometaphase and telophase, were found to localize adjacent to endoplasmic reticulum (ER) export domains, and resident Golgi transmembrane proteins cycled rapidly into and out of these fragments. Golgi proteins within mitotic Golgi haze—seen during metaphase—were found to redistribute with ER markers into fragments when the ER was fragmented by ionomycin treatment. The temperature-sensitive misfolding mutant ts045VSVG protein, when localized to the Golgi at the start of mitosis, became trapped in the ER at the end of mitosis in cells shifted to 40°C. Finally, reporters for Arf1 and Sar1 activity revealed that Arf1 and Sar1 undergo sequential inactivation during mitotic Golgi breakdown and sequential reactivation upon Golgi reassembly at the end of mitosis. Together, these findings support a model of mitotic Golgi inheritance that involves inhibition and subsequent reactivation of cellular activities controlling the cycling of Golgi components into and out of the ER.

Published

2006

34. Stable Binding of ATF6 to BiP in the Endoplasmic Reticulum Stress Response

Author

Ron Prywes, Jingshi Shen, Jennifer Lippincott-Schwartz, and Erik L. Snapp

Subjects

Protein Folding, genetic structures, Gene Expression, macromolecular substances, Plasma protein binding, Endoplasmic Reticulum, Mice, chemistry.chemical_compound, Adenosine Triphosphate, Chlorocebus aethiops, Animals, Humans, Endoplasmic Reticulum Chaperone BiP, Molecular Biology, Transcription factor, Heat-Shock Proteins, biology, ATF6, Endoplasmic reticulum, Cell Biology, Activating Transcription Factor 6, DNA-Binding Proteins, Dithiothreitol, Biochemistry, chemistry, Chaperone (protein), COS Cells, Mutation, NIH 3T3 Cells, biology.protein, Unfolded protein response, Biophysics, Protein folding, Adenosine triphosphate, HeLa Cells, Molecular Chaperones, Protein Binding, Transcription Factors

Abstract

Endoplasmic reticulum (ER) stress-induced activation of ATF6, an ER membrane-bound transcription factor, requires a dissociation step from its inhibitory regulator, BiP. It has been generally postulated that dissociation of the BiP-ATF6 complex is a result of the competitive binding of misfolded proteins generated during ER stress. Here we present evidence against this model and for an active regulatory mechanism for dissociation of the complex. Contradictory to the competition model that is based on dynamic binding of BiP to ATF6, our data reveal relatively stable binding. First, the complex was easily isolated, in contrast to many chaperone complexes that require chemical cross-linking. Second, ATF6 bound at similar levels to wild-type BiP and a BiP mutant form that binds substrates stably because of a defect in its ATPase activity. Third, ER stress specifically induced the dissociation of BiP from ER stress transducers while the competition model would predict dissociation from any specific substrate. Fourth, the ATF6-BiP complex was resistant to ATP-induced dissociation in vitro when isolated without detergents, suggesting that cofactors stabilize the complex. In favor of an active dissociation model, one specific region within the ATF6 lumenal domain was identified as a specific ER stress-responsive sequence required for ER stress-triggered BiP release. Together, our results do not support a model in which competitive binding of misfolded proteins causes dissociation of the BiP-ATF6 complex in stressed cells. We propose that stable BiP binding is essential for ATF6 regulation and that ER stress dissociates BiP from ATF6 by actively restarting the BiP ATPase cycle.

Published

2005

35. The Fusome Mediates Intercellular Endoplasmic Reticulum Connectivity inDrosophilaOvarian Cysts

Author

David Frescas, Erik L. Snapp, Takako Iida, Jennifer Lippincott-Schwartz, and Mary A. Lilly

Subjects

Recombinant Fusion Proteins, Endoplasmic reticulum, Ovary, Mitosis, Cell Differentiation, Intracellular Membranes, Articles, Cell Biology, Biology, Endoplasmic Reticulum, Spindle apparatus, Cell biology, Drosophila melanogaster, Cytoplasm, Organelle, Animals, Female, Cleavage furrow, Oocyte differentiation, Cytoskeleton, Molecular Biology, Biomarkers

Abstract

Drosophila ovarian cysts arise through a series of four synchronous incomplete mitotic divisions. After each round of mitosis, a membranous organelle, the fusome, grows along the cleavage furrow and the remnants of the mitotic spindle to connect all cystocytes in a cyst. The fusome is essential for the pattern and synchrony of the mitotic cyst divisions as well as oocyte differentiation. Using live cell imaging, greenfluorescent protein–tagged proteins, and photobleaching techniques, we demonstrate that fusomal endomembranes are part of a single continuous endoplasmic reticulum (ER) that is shared by all cystocytes in dividing ovarian cysts. Membrane and lumenal proteins of the common ER freely and rapidly diffuse between cystocytes. The fusomal ER mediates intercellular ER connectivity by linking the cytoplasmic ER membranes of all cystocytes within a cyst. Before entry into meiosis and onset of oocyte differentiation (between region 1 and region 2A), ER continuity between cystocytes is lost. Furthermore, analyses of hts and Dhc64c mutants indicate that intercellular ER continuity within dividing ovarian cysts requires the fusome cytoskeletal component and suggest a possible role for the common ER in synchronizing mitotic cyst divisions.

Published

2004

36. Endoplasmic Reticulum Export Sites and Golgi Bodies Behave as Single Mobile Secretory Units in Plant Cells[W]

Author

Luis L. P. daSilva, Jennifer Lippincott-Schwartz, Federica Brandizzi, Erik L. Snapp, Chris Hawes, and Jürgen Denecke

Subjects

Genetic Markers, Recombinant Fusion Proteins, Golgi Apparatus, Plant Science, Biology, Endoplasmic Reticulum, chemistry.chemical_compound, symbols.namesake, Transformation, Genetic, Tobacco, COPII, Research Articles, Secretory pathway, Golgi membrane, Vesicular-tubular cluster, Endoplasmic reticulum, Biological Transport, Cell Biology, COPI, Brefeldin A, Golgi apparatus, Cell biology, Plant Leaves, chemistry, Agrobacterium tumefaciens, symbols, COP-Coated Vesicles, Fluorescence Recovery After Photobleaching

Abstract

In contrast with animals, plant cells contain multiple mobile Golgi stacks distributed over the entire cytoplasm. However, the distribution and dynamics of protein export sites on the plant endoplasmic reticulum (ER) surface have yet to be characterized. A widely accepted model for ER-to-Golgi transport is based on the sequential action of COPII and COPI coat complexes. The COPII complex assembles by the ordered recruitment of cytosolic components on the ER membrane. Here, we have visualized two early components of the COPII machinery, the small GTPase Sar1p and its GTP exchanging factor Sec12p in live tobacco (Nicotiana tabacum) leaf epidermal cells. By in vivo confocal laser scanning microscopy and fluorescence recovery after photobleaching experiments, we show that Sar1p cycles on mobile punctate structures that track with the Golgi bodies in close proximity but contain regions that are physically separated from the Golgi bodies. By contrast, Sec12p is uniformly distributed along the ER network and does not accumulate in these structures, consistent with the fact that Sec12p does not become part of a COPII vesicle. We propose that punctate accumulation of Sar1p represents ER export sites (ERES). The sites may represent a combination of Sar1p-coated ER membranes, nascent COPII membranes, and COPII vectors in transit, which have yet to lose their coats. ERES can be induced by overproducing Golgi membrane proteins but not soluble bulk-flow cargos. Few punctate Sar1p loci were observed that are independent of Golgi bodies, and these may be nascent ERES. The vast majority of ERES form secretory units that move along the surface of the ER together with the Golgi bodies, but movement does not influence the rate of cargo transport between these two organelles. Moreover, we could demonstrate using the drug brefeldin A that formation of ERES is strictly dependent on a functional retrograde transport route from the Golgi apparatus.

Published

2004

37. The organization of engaged and quiescent translocons in the endoplasmic reticulum of mammalian cells

Author

Jennifer Lippincott-Schwartz, Gretchen A. Reinhart, Ramanujan S. Hegde, Erik L. Snapp, and Brigitte A. Bogert

Subjects

Sec61, Signal recognition particle, Membrane Glycoproteins, FRET, TRAP, protein translocation, TRAM, Endoplasmic reticulum, Translation (biology), Cell Biology, Biology, Endoplasmic Reticulum, Kidney, Translocon, Article, Cell Line, Transport protein, Cell biology, Protein Transport, Dogs, Förster resonance energy transfer, Animals, Signal recognition particle receptor

Abstract

Protein translocons of the mammalian endoplasmic reticulum are composed of numerous functional components whose organization during different stages of the transport cycle in vivo remains poorly understood. We have developed generally applicable methods based on fluorescence resonance energy transfer (FRET) to probe the relative proximities of endogenously expressed translocon components in cells. Examination of substrate-engaged translocons revealed oligomeric assemblies of the Sec61 complex that were associated to varying degrees with other essential components including the signal recognition particle receptor TRAM and the TRAP complex. Remarkably, these components not only remained assembled but also had a similar, yet distinguishable, organization both during and after nascent chain translocation. The persistence of preassembled and complete translocons between successive rounds of transport may facilitate highly efficient translocation in vivo despite temporal constraints imposed by ongoing translation and a crowded cellular environment.

Published

2004

38. Formation of stacked ER cisternae by low affinity protein interactions

Author

Jennifer Lippincott-Schwartz, Nica Borgese, Sara Francesca Colombo, Erik L. Snapp, Ramanujan S. Hegde, Emanuela Pedrazzini, Francesca Lombardo, and Maura Francolini

Subjects

Recombinant Fusion Proteins, Green Fluorescent Proteins, Biology, Endoplasmic Reticulum, Models, Biological, Article, endoplasmic reticulum, photobleaching, cytochrome b5, GFP, FRAP, Cell Line, Protein–protein interaction, Green fluorescent protein, Chlorocebus aethiops, Animals, Point Mutation, Luminescent Proteins, COS cells, Endoplasmic reticulum, Membrane Proteins, Intracellular Membranes, Cell Biology, Endoplasmic Reticulum, Smooth, Protein Structure, Tertiary, Cell biology, Membrane protein, Cytoplasm, COS Cells, Biogenesis

Abstract

The endoplasmic reticulum (ER) can transform from a network of branching tubules into stacked membrane arrays (termed organized smooth ER [OSER]) in response to elevated levels of specific resident proteins, such as cytochrome b(5). Here, we have tagged OSER-inducing proteins with green fluorescent protein (GFP) to study OSER biogenesis and dynamics in living cells. Overexpression of these proteins induced formation of karmellae, whorls, and crystalloid OSER structures. Photobleaching experiments revealed that OSER-inducing proteins were highly mobile within OSER structures and could exchange between OSER structures and surrounding reticular ER. This indicated that binding interactions between proteins on apposing stacked membranes of OSER structures were not of high affinity. Addition of GFP, which undergoes low affinity, antiparallel dimerization, to the cytoplasmic domains of non–OSER-inducing resident ER proteins was sufficient to induce OSER structures when overexpressed, but addition of a nondimerizing GFP variant was not. These results point to a molecular mechanism for OSER biogenesis that involves weak homotypic interactions between cytoplasmic domains of proteins. This mechanism may underlie the formation of other stacked membrane structures within cells.

Published

2003

39. Approaches to imaging unfolded secretory protein stress in living cells

Author

Elena N. Fazio, Patrick Lajoie, and Erik L. Snapp

Subjects

Endoplasmic reticulum, fungi, Medicine (miscellaneous), Cell Biology, Biology, Article, Green fluorescent protein, Cell biology, Secretory protein, Live cell imaging, Unfolded protein response, Protein folding, Signal transduction, Secretory pathway

Abstract

The endoplasmic reticulum (ER) is the point of entry of proteins into the secretory pathway. Nascent peptides interact with the ER quality control machinery that ensures correct folding of the nascent proteins. Failure to properly fold proteins can lead to loss of protein function and cytotoxic aggregation of misfolded proteins that can lead to cell death. To cope with increases in the ER unfolded secretory protein burden, cells have evolved the Unfolded Protein Response (UPR). The UPR is the primary signaling pathway that monitors the state of the ER folding environment. When the unfolded protein burden overwhelms the capacity of the ER quality control machinery, a state termed ER stress, sensor proteins detect accumulation of misfolded peptides and trigger the UPR transcriptional response. The UPR, which is conserved from yeast to mammals, consists of an ensemble of complex signaling pathways that aims at adapting the ER to the new misfolded protein load. To determine how different factors impact the ER folding environment, various tools and assays have been developed. In this review, we discuss recent advances in live cell imaging reporters and model systems that enable researchers to monitor changes in the unfolded secretory protein burden and activation of the UPR and its associated signaling pathways.

Published

2014

40. Allosteric inhibition of the IRE1α RNase preserves cell viability and function during endoplasmic reticulum stress

Author

Maike Thamsen, Deborah Caswell, Likun Wang, Dustin J. Maly, Kurt F. Weiberth, Hector Macias, Sanjay B. Hari, Scott A. Oakes, Aeid Igbaria, Barun Bhhatarai, Shuhei Morita, Eric S. Wang, Michael S. German, Micah J. Gliedt, Bradley J. Backes, Kris Prado, Erik L. Snapp, Arinjay K. Mitra, Douglas B. Gould, Rajarshi Ghosh, Feroz R. Papa, B. Gayani K. Perera, Stephan C. Schürer, and Marcel V. Alavi

Subjects

Male, XBP1, RNase P, Endoribonuclease, Apoptosis, Cell fate determination, Biology, Protein Serine-Threonine Kinases, Medical and Health Sciences, Article, General Biochemistry, Genetics and Molecular Biology, Retina, Cell Line, Enzyme activator, Islets of Langerhans, Mice, Ribonucleases, Allosteric Regulation, Endoribonucleases, Genetics, Animals, Humans, 2.1 Biological and endogenous factors, Viability assay, Aetiology, Protein Kinase Inhibitors, Biochemistry, Genetics and Molecular Biology(all), Endoplasmic reticulum, Biological Sciences, Protein-Serine-Threonine Kinases, Endoplasmic Reticulum Stress, Cell biology, Rats, Enzyme Activation, Unfolded protein response, Developmental Biology

Abstract

SummaryDepending on endoplasmic reticulum (ER) stress levels, the ER transmembrane multidomain protein IRE1α promotes either adaptation or apoptosis. Unfolded ER proteins cause IRE1α lumenal domain homo-oligomerization, inducing trans autophosphorylation that further drives homo-oligomerization of its cytosolic kinase/endoribonuclease (RNase) domains to activate mRNA splicing of adaptive XBP1 transcription factor. However, under high/chronic ER stress, IRE1α surpasses an oligomerization threshold that expands RNase substrate repertoire to many ER-localized mRNAs, leading to apoptosis. To modulate these effects, we developed ATP-competitive IRE1α Kinase-Inhibiting RNase Attenuators—KIRAs—that allosterically inhibit IRE1α’s RNase by breaking oligomers. One optimized KIRA, KIRA6, inhibits IRE1α in vivo and promotes cell survival under ER stress. Intravitreally, KIRA6 preserves photoreceptor functional viability in rat models of ER stress-induced retinal degeneration. Systemically, KIRA6 preserves pancreatic β cells, increases insulin, and reduces hyperglycemia in Akita diabetic mice. Thus, IRE1α powerfully controls cell fate but can itself be controlled with small molecules to reduce cell degeneration.

Published

2014

41. A sphingolipid-dependent diffusion barrier confines ER stress to the yeast mother cell

Author

Stéphanie Buvelot Frei, Annina Denoth-Lippuner, Lori Clay, Fabrice Caudron, Barbara Boettcher, Yves Barral, and Erik L. Snapp

Subjects

Protein Folding, Saccharomyces cerevisiae Proteins, Time Factors, Cell division, QH301-705.5, Nuclear Envelope, Science, Saccharomyces cerevisiae, S. cerevisiae, Cell Cycle Proteins, Endoplasmic Reticulum, Septin, Permeability, asymmetric cell division, General Biochemistry, Genetics and Molecular Biology, Diffusion, Asymmetric cell division, Guanine Nucleotide Exchange Factors, Biology (General), diffusion barrier, Cell Cycle Protein, Sphingolipids, General Immunology and Microbiology, biology, General Neuroscience, Endoplasmic reticulum, Microfilament Proteins, aging, Intracellular Membranes, Cell Biology, General Medicine, Endoplasmic Reticulum Stress, biology.organism_classification, Cell biology, rab GTP-Binding Proteins, Unfolded protein response, Medicine, sphingolipid, ER stress, Bacterial outer membrane, Cell Division, Septins, Research Article

Abstract

In many cell types, lateral diffusion barriers compartmentalize the plasma membrane and, at least in budding yeast, the endoplasmic reticulum (ER). However, the molecular nature of these barriers, their mode of action and their cellular functions are unclear. Here, we show that misfolded proteins of the ER remain confined into the mother compartment of budding yeast cells. Confinement required the formation of a lateral diffusion barrier in the form of a distinct domain of the ER-membrane at the bud neck, in a septin-, Bud1 GTPase- and sphingolipid-dependent manner. The sphingolipids, but not Bud1, also contributed to barrier formation in the outer membrane of the dividing nucleus. Barrier-dependent confinement of ER stress into the mother cell promoted aging. Together, our data clarify the physical nature of lateral diffusion barriers in the ER and establish the role of such barriers in the asymmetric segregation of proteotoxic misfolded proteins during cell division and aging., eLife, 3, ISSN:2050-084X

Published

2014

42. Author response: A sphingolipid-dependent diffusion barrier confines ER stress to the yeast mother cell

Author

Erik L. Snapp, Barbara Boettcher, Fabrice Caudron, Stéphanie Buvelot Frei, Annina Denoth-Lippuner, Lori Clay, and Yves Barral

Subjects

medicine.anatomical_structure, Diffusion barrier, Chemistry, Cell, medicine, Unfolded protein response, Sphingolipid, Yeast, Cell biology

Published

2014

43. Dynamics and retention of misfolded proteins in native ER membranes

Author

Theresa H Roberts, Erik L. Snapp, Eric D. Siggia, Anne K. Kenworthy, Jan Ellenberg, John F. Presley, Jennifer Lippincott-Schwartz, Sarah Nehls, Nelson B. Cole, and Kristien J. M. Zaal

Subjects

Protein Folding, Glycosylation, Recombinant Fusion Proteins, Green Fluorescent Proteins, Biology, Endoplasmic Reticulum, chemistry.chemical_compound, Adenosine Triphosphate, JUNQ and IPOD, Viral Envelope Proteins, Genes, Reporter, Animals, Protein oligomerization, Membrane Glycoproteins, Tunicamycin, Endoplasmic reticulum, Temperature, Fluorescence recovery after photobleaching, Biological Transport, Cell Biology, Anti-Bacterial Agents, Cell biology, Dithiothreitol, Luminescent Proteins, Membrane, chemistry, COS Cells, Unfolded protein response, Indicators and Reagents, Protein folding

Abstract

When co-translationally inserted into endoplasmic reticulum (ER) membranes, newly synthesized proteins encounter the lumenal environment of the ER, which contains chaperone proteins that facilitate the folding reactions necessary for protein oligomerization, maturation and export from the ER. Here we show, using a temperature-sensitive variant of vesicular stomatitis virus G protein tagged with green fluorescent protein (VSVG-GFP), and fluorescence recovery after photobleaching (FRAP), the dynamics of association of folded and misfolded VSVG complexes with ER chaperones. We also investigate the potential mechanisms underlying protein retention in the ER. Misfolded VSVG-GFP complexes at 40 degrees C are highly mobile in ER membranes and do not reside in post-ER compartments, indicating that they are not retained in the ER by immobilization or retrieval mechanisms. These complexes are immobilized in ATP-depleted or tunicamycin-treated cells, in which VSVG-chaperone interactions are no longer dynamic. These results provide insight into the mechanisms of protein retention in the ER and the dynamics of protein-folding complexes in native ER membranes.

Published

2000

44. Cytoskeletal Association Is Important for Differential Targeting of Glucose Transporter Isoforms in Leishmania

Author

Scott M. Landfear and Erik L. Snapp

Subjects

Monosaccharide Transport Proteins, Octoxynol, Detergents, Protein Sorting Signals, Flagellum, Cell Fractionation, Article, 03 medical and health sciences, Microtubule, parasitic diseases, Animals, Cytoskeleton, Cell body membrane, 030304 developmental biology, Glucose Transporter Type 2, 0303 health sciences, Binding Sites, biology, Membrane transport protein, 030302 biochemistry & molecular biology, Glucose transporter, Membrane Proteins, Cell Biology, Leishmania enriettii, Rats, Cell biology, Cytosol, Solubility, Biochemistry, Membrane protein, Flagella, biology.protein, Epitopes, B-Lymphocyte

Abstract

The major glucose transporter of the parasitic protozoan Leishmania enriettii exists in two isoforms, one of which (iso-1) localizes to the flagellar membrane, while the other (iso-2) localizes to the plasma membrane of the cell body, the pellicular membrane. These two isoforms differ only in their cytosolic NH2-terminal domains. Using immunoblots and immunofluorescence microscopy of detergent-extracted cytoskeletons, we have demonstrated that iso-2 associates with the microtubular cytoskeleton that underlies the cell body membrane, whereas the flagellar membrane isoform iso-1 does not associate with the cytoskeleton. Deletion mutants that remove the first 25 or more amino acids from iso-1 are retargeted from the flagellum to the pellicular membrane, suggesting that these deletions remove a signal required for flagellar targeting. Unlike the full-length iso-1 protein, these deletion mutants associate with the cytoskeleton. Our results suggest that cytoskeletal binding serves as an anchor to localize the iso-2 transporter within the pellicular membrane, and that the flagellar targeting signal of iso-1 diverts this transporter into the flagellar membrane and away from the pellicular microtubules.

Published

1997

45. Fluorescent Proteins in Cellular Organelles: Serious Pitfalls and Some Solutions

Author

Lindsey M. Costantini and Erik L. Snapp

Subjects

Glycosylation, animal structures, Protein Conformation, health care facilities, manpower, and services, education, Computational biology, Biology, Fluorescence, Organelle, Genetics, Animals, Humans, Disulfides, Molecular Biology, health care economics and organizations, Organelles, education.field_of_study, ComputingMilieux_PERSONALCOMPUTING, Cell Biology, General Medicine, Recombinant Proteins, Cell biology, Luminescent Proteins, Editorial, ComputingMethodologies_PATTERNRECOGNITION, embryonic structures, Warning label, Oxidation-Reduction, DNACB Bits

Abstract

Fluorescent proteins (FPs) have been powerful tools for cell biologists for over 15 years. The large variety of FPs available rarely comes with an instruction manual or a warning label. The potential pitfalls of the use of FPs in cellular organelles represent a significant concern for investigators. FPs generally did not evolve in the often distinctive physicochemical environments of subcellular organelles. In organelles, FPs can misfold, go dark, and even distort organelle morphology. In this minireview, we describe the issues associated with FPs in organelles and provide solutions to enable investigators to better exploit FP technology in cells.

Published

2013

46. Human liver cell trafficking mutants: characterization and whole exome sequencing

Author

Erik L. Snapp, David C. Spray, Allan W. Wolkoff, Fei Yuan, Barry Potvin, Pamela Stanley, Phyllis M. Novikoff, and Sylvia O. Suadicani

Subjects

Mutant, lcsh:Medicine, Gene Expression, Cell Communication, medicine.disease_cause, Biochemistry, Intracellular Receptors, Molecular Cell Biology, Exome, RNA, Small Interfering, lcsh:Science, Cells, Cultured, chemistry.chemical_classification, Mutation, Multidisciplinary, Liver cell, Liver Neoplasms, Transferrin, Gap Junctions, High-Throughput Nucleotide Sequencing, Endocytosis, Cell biology, Protein Transport, symbols, Cytochemistry, Membranes and Sorting, Research Article, Signal Transduction, Carcinoma, Hepatocellular, Blotting, Western, Transferrin receptor, Receptors, Cell Surface, Biology, Molecular Genetics, symbols.namesake, Genetic Mutation, medicine, Genetics, Humans, Secretion, lcsh:R, Cell Membrane, Proteins, Golgi apparatus, Molecular biology, chemistry, rab GTP-Binding Proteins, lcsh:Q, Gene Function, Membrane Composition

Abstract

The HuH7 liver cell mutant Trf1 is defective in membrane trafficking and is complemented by the casein kinase 2α subunit CK2α’’. Here we identify characteristic morphologies, trafficking and mutational changes in six additional HuH7 mutants Trf2-Trf7. Trf1 cells were previously shown to be severely defective in gap junction functions. Using a Lucifer yellow transfer assay, remarkable attenuation of gap junction communication was revealed in each of the mutants Trf2-Trf7. Electron microscopy and light microscopy of thiamine pyrophosphatase showed that several mutants exhibited fragmented Golgi apparatus cisternae compared to parental HuH7 cells. Intracellular trafficking was investigated using assays of transferrin endocytosis and recycling and VSV G secretion. Surface binding of transferrin was reduced in all six Trf2-Trf7 mutants, which generally correlated with the degree of reduced expression of the transferrin receptor at the cell surface. The mutants displayed the same transferrin influx rates as HuH7, and for efflux rate, only Trf6 differed, having a slower transferrin efflux rate than HuH7. The kinetics of VSV G transport along the exocytic pathway were altered in Trf2 and Trf5 mutants. Genetic changes unique to particular Trf mutants were identified by exome sequencing, and one was investigated in depth. The novel mutation Ile34Phe in the GTPase RAB22A was identified in Trf4. RNA interference knockdown of RAB22A or overexpression of RAB22AI34F in HuH7 cells caused phenotypic changes characteristic of the Trf4 mutant. In addition, the Ile34Phe mutation reduced both guanine nucleotide binding and hydrolysis activities of RAB22A. Thus, the RAB22A Ile34Phe mutation appears to contribute to the Trf4 mutant phenotype.

Published

2013

47. Photobleaching Methods to Study Golgi Complex Dynamics in Living Cells

Author

Erik L. Snapp

Subjects

Recombinant Fusion Proteins, Green Fluorescent Proteins, Golgi Apparatus, Biology, Endoplasmic Reticulum, Transfection, Article, Green fluorescent protein, Diffusion, symbols.namesake, Organelle, Animals, Humans, Secretory pathway, Microscopy, Confocal, Photobleaching, Endoplasmic reticulum, Fluorescence recovery after photobleaching, Golgi apparatus, Transport protein, Cell biology, Protein Transport, Microscopy, Fluorescence, symbols, Fluorescence Recovery After Photobleaching, HeLa Cells

Abstract

The Golgi complex (GC) is a highly dynamic organelle that constantly receives and exports proteins and lipids from both the endoplasmic reticulum and the plasma membrane. While protein trafficking can be monitored with traditional biochemical methods, these approaches average the behaviors of millions of cells, provide modest temporal information and no spatial information. Photobleaching methods enable investigators to monitor protein trafficking in single cells or even single GC stacks with subsecond precision. Furthermore, photobleaching can be exploited to monitor the behaviors of resident GC proteins to provide insight into mechanisms of retention and trafficking. In this chapter, general photobleaching approaches with laser scanning confocal microscopes are described. Importantly, the problems associated with many fluorescent proteins (FPs) and their uses in the secretory pathway are discussed and appropriate choices are suggested. For example, Enhanced Green Fluorescent Protein (EGFP) and most red FPs are extremely problematic. Finally, options for data analyses are described.

Published

2013

48. ERdj3 Regulates BiP Occupancy in Living Cells

Author

Erik L. Snapp and Feng Guo

Subjects

genetic structures, macromolecular substances, Plasma protein binding, Biology, Endoplasmic Reticulum, Madin Darby Canine Kidney Cells, Substrate Specificity, Dogs, Cell Line, Tumor, Heat shock protein, Animals, Humans, Transgenes, Endoplasmic Reticulum Chaperone BiP, Heat-Shock Proteins, Endoplasmic reticulum, Membrane Proteins, Fluorescence recovery after photobleaching, Cell Biology, HSP40 Heat-Shock Proteins, Translocon, Cell biology, Secretory protein, Membrane protein, Chaperone (protein), Mutation, biology.protein, SEC Translocation Channels, Molecular Chaperones, Protein Binding, Research Article

Abstract

Co-chaperones regulate chaperone activities and are likely to impact a protein folding environment as much as the chaperone, itself. As co-chaperones are expressed substoichiometrically, the ability of co-chaperones to encounter a chaperone represents a critical parameter for chaperone activity. ERdj3, an abundant soluble endoplasmic reticulum (ER) co-chaperone of the Hsp70 BiP, stimulates BiP's ATPase to increase BiP's affinity for client (or substrate) proteins. We investigated ERdj3 availability, how ERdj3 levels impact BiP availability, and the significance of J proteins for regulating BiP binding of clients in living cells. FRAP analysis revealed overexpressed ERdj3-sfGFP dramatically decreases BiP-GFP mobility in a client-dependent manner. In contrast, ERdj3-GFP mobility remains low regardless of client protein levels. Native gels and co-immunoprecipitations established ERdj3 associates with a large complex including Sec61α. Translocon binding likely ensures rapid encounters between emerging nascent peptides and stimulates BiP activity in critical early stages of secretory protein folding. Importantly, mutant BiP exhibited significantly increased mobility when it could not interact with any ERdjs. Thus, ERdjs appear to play dual roles of increasing BiP affinity for clients and regulating delivery of clients to BiP. Our data suggest BiP engagement of clients will be enhanced in ER subdomains enriched in ERdj proteins.

Published

2013

49. Detecting Soluble PolyQ Oligomers and Investigating Their Impact on Living Cells Using Split-GFP

Author

Patrick Lajoie and Erik L. Snapp

Subjects

Huntingtin Protein, Huntingtin, Recombinant Fusion Proteins, Green Fluorescent Proteins, Mutant, Nerve Tissue Proteins, Biology, Article, Inclusion bodies, Cell Line, Cell biology, Green fluorescent protein, Complementation, Microscopy, Fluorescence, Solubility, Biochemistry, Protein-fragment complementation assay, Cytoplasm, Animals, Humans, Protein Multimerization

Abstract

Aberrant expansion of the number of polyglutamine (polyQ) repeats in mutant proteins is the hallmark of various diseases. These pathologies include Huntington's disease (HD), a neurological disorder caused by expanded polyQ stretch within the huntingtin (Htt) protein. The expansions increase the propensity of the Htt protein to oligomerize. In the cytoplasm of living cells, the mutant form of Htt (mHtt) is present as soluble monomers and oligomers as well as insoluble aggregates termed inclusion bodies (IBs). Detecting and assessing the relative toxicity of these various forms of mHtt has proven difficult. To enable direct visualization of mHtt soluble oligomers in living cells, we established a split superfolder green fluorescent protein (sfGFP) complementation assay. In this assay, exon 1 variants of Htt (Htt(ex1)) containing non-pathological or HD-associated polyQ lengths were fused to two different nonfluorescent fragments of sfGFP. If the Htt proteins oligomerize and the sfGFP fragments come into close proximity, they can associate and complement each other to form a complete and fluorescent sfGFP reporter. Importantly, the irreversible nature of the split-sfGFP complementation allowed us to trap otherwise transient interactions and artificially increase mHtt oligomerization. When coupled with a fluorescent apoptosis reporter, this assay can correlate soluble mHtt oligomer levels and cell death leading to a better characterization of the toxic potential of various forms of mHtt in living cells.

Published

2013

50. Polymeric Mutants Of ±1-Antitrypsin Impair Protein Mobility Within The Endoplasmic Reticulum And Enhance Susceptibility To The Unfolded Protein Response

Author

Elena Miranda, Stefan J. Marciniak, Adriana Ordóñez, Erik L. Snapp, and David A. Lomas

Subjects

Chemistry, Endoplasmic reticulum, Mutant, Unfolded protein response, STIM1, Cell biology

Published

2012