Your search keyword '"Kristin Stirnnagel"' showing total 13 results

1. Identification of an Intermediate Step in Foamy Virus Fusion

Author

Aurélie Dupont, Ivo M. Glück, Dorothee Ponti, Kristin Stirnnagel, Sylvia Hütter, Florian Perrotton, Nicole Stanke, Stefanie Richter, Dirk Lindemann, and Don C. Lamb

Subjects

foamy virus, viral fusion, retrovirus, envelope glycoprotein, capsid, single virus tracking, Microbiology, QR1-502

Abstract

Viral glycoprotein-mediated membrane fusion is an essential step for productive infection of host cells by enveloped viruses; however, due to its rarity and challenges in detection, little is known about the details of fusion events at the single particle level. Here, we have developed dual-color foamy viruses (FVs) composed of eGFP-tagged prototype FV (PFV) Gag and mCherry-tagged Env of either PFV or macaque simian FV (SFVmac) origin that have been optimized for detection of the fusion process. Using our recently developed tracking imaging correlation (TrIC) analysis, we were able to detect the fusion process for both PFV and SFVmac Env containing virions. PFV Env-mediated fusion was observed both at the plasma membrane as well as from endosomes, whereas SFVmac Env-mediated fusion was only observed from endosomes. PFV Env-mediated fusion was observed to happen more often and more rapidly than as for SFVmac Env. Strikingly, using the TrIC method, we detected a novel intermediate state where the envelope and capsids are still tethered but separated by up to 400 nm before final separation of Env and Gag occurred.

Published

2020

2. Structure of a Spumaretrovirus Gag Central Domain Reveals an Ancient Retroviral Capsid.

Author

Neil J Ball, Giuseppe Nicastro, Moumita Dutta, Dominic J Pollard, David C Goldstone, Marta Sanz-Ramos, Andres Ramos, Erik Müllers, Kristin Stirnnagel, Nicole Stanke, Dirk Lindemann, Jonathan P Stoye, William R Taylor, Peter B Rosenthal, and Ian A Taylor

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

The Spumaretrovirinae, or foamy viruses (FVs) are complex retroviruses that infect many species of monkey and ape. Despite little sequence homology, FV and orthoretroviral Gag proteins perform equivalent functions, including genome packaging, virion assembly, trafficking and membrane targeting. However, there is a paucity of structural information for FVs and it is unclear how disparate FV and orthoretroviral Gag molecules share the same function. To probe the functional overlap of FV and orthoretroviral Gag we have determined the structure of a central region of Gag from the Prototype FV (PFV). The structure comprises two all α-helical domains NtDCEN and CtDCEN that although they have no sequence similarity, we show they share the same core fold as the N- (NtDCA) and C-terminal domains (CtDCA) of archetypal orthoretroviral capsid protein (CA). Moreover, structural comparisons with orthoretroviral CA align PFV NtDCEN and CtDCEN with NtDCA and CtDCA respectively. Further in vitro and functional virological assays reveal that residues making inter-domain NtDCEN-CtDCEN interactions are required for PFV capsid assembly and that intact capsid is required for PFV reverse transcription. These data provide the first information that relates the Gag proteins of Spuma and Orthoretrovirinae and suggests a common ancestor for both lineages containing an ancient CA fold.

Published

2016

3. Tracking Image Correlation: Combining Single-Particle Tracking and Image Correlation

Author

Kristin Stirnnagel, Aurélie Dupont, Dirk Lindemann, and Don C. Lamb

Subjects

Digital image correlation, Cross-correlation, Cell Survival, Biophysics, Color, Reproducibility of Results, Colocalization, Biological Transport, Nanotechnology, Biology, Tracking (particle physics), Microspheres, Cytosol, Imaging, Three-Dimensional, Cell Biophysics, Position (vector), Microscopy, Trajectory, Humans, Spumavirus, Particle, Biological system, Fluorescent Dyes, HeLa Cells

Abstract

The interactions and coordination of biomolecules are crucial for most cellular functions. The observation of protein interactions in live cells may provide a better understanding of the underlying mechanisms. After fluorescent labeling of the interacting partners and live-cell microscopy, the colocalization is generally analyzed by quantitative global methods. Recent studies have addressed questions regarding the individual colocalization of moving biomolecules, usually by using single-particle tracking (SPT) and comparing the fluorescent intensities in both color channels. Here, we introduce a new method that combines SPT and correlation methods to obtain a dynamical 3D colocalization analysis along single trajectories of dual-colored particles. After 3D tracking, the colocalization is computed at each particle’s position via the local 3D image cross correlation of the two detection channels. For every particle analyzed, the output consists of the 3D trajectory, the time-resolved 3D colocalization information, and the fluorescence intensity in both channels. In addition, the cross-correlation analysis shows the 3D relative movement of the two fluorescent labels with an accuracy of 30 nm. We apply this method to the tracking of viral fusion events in live cells and demonstrate its capacity to obtain the time-resolved colocalization status of single particles in dense and noisy environments.

Published

2013

4. Structure of a Spumaretrovirus Gag Central Domain Reveals an Ancient Retroviral Capsid

Author

Giuseppe Nicastro, Ian A. Taylor, Nicole Stanke, Moumita Dutta, Jonathan P. Stoye, Peter B. Rosenthal, Erik Müllers, David C. Goldstone, William R. Taylor, Andres Ramos, Dominic J. Pollard, Kristin Stirnnagel, Marta Sanz-Ramos, Neil J. Ball, and Dirk Lindemann

Subjects

0301 basic medicine, RNA viruses, Protein Structure Comparison, Protein Conformation, viruses, medicine.disease_cause, Pathology and Laboratory Medicine, Biochemistry, Viral Packaging, Protein structure, Immunodeficiency Viruses, 1108 Medical Microbiology, Materials Physics, Macromolecular Structure Analysis, Medicine and Health Sciences, Biology (General), Spumavirus, Peptide sequence, AMINO-TERMINAL DOMAIN, biology, Physics, NONHUMAN-PRIMATES, CRYOELECTRON MICROSCOPY, 3. Good health, Cell biology, Capsid, Virion assembly, 1107 Immunology, Medical Microbiology, Viral Pathogens, SIZE-DISTRIBUTION ANALYSIS, Viruses, Physical Sciences, MAJOR HOMOLOGY REGION, Pathogens, Sedimentation, Life Sciences & Biomedicine, Sequence Analysis, 0605 Microbiology, Research Article, Protein Structure, VELOCITY ANALYTICAL ULTRACENTRIFUGATION, Viral protein, QH301-705.5, Immunology, Blotting, Western, Materials Science, Gene Products, gag, PROTOTYPE FOAMY VIRUS, Viral Structure, Real-Time Polymerase Chain Reaction, Research and Analysis Methods, Microbiology, Cell Line, 03 medical and health sciences, REVERSE TRANSCRIPTION, Sequence Motif Analysis, Virology, Retroviruses, Genetics, medicine, Viral Core, Animals, Humans, Amino Acid Sequence, Nucleic acid structure, Molecular Biology Techniques, Sequencing Techniques, RESTRICTION FACTOR, Nuclear Magnetic Resonance, Biomolecular, Molecular Biology, Microbial Pathogens, Science & Technology, DIPOLAR COUPLINGS, Virus Assembly, Lentivirus, Organisms, Biology and Life Sciences, Proteins, HIV, RC581-607, biology.organism_classification, Reverse transcriptase, Viral Replication, 030104 developmental biology, HIV-1, Parasitology, Capsid Proteins, Immunologic diseases. Allergy

Abstract

The Spumaretrovirinae, or foamy viruses (FVs) are complex retroviruses that infect many species of monkey and ape. Despite little sequence homology, FV and orthoretroviral Gag proteins perform equivalent functions, including genome packaging, virion assembly, trafficking and membrane targeting. However, there is a paucity of structural information for FVs and it is unclear how disparate FV and orthoretroviral Gag molecules share the same function. To probe the functional overlap of FV and orthoretroviral Gag we have determined the structure of a central region of Gag from the Prototype FV (PFV). The structure comprises two all α-helical domains NtDCEN and CtDCEN that although they have no sequence similarity, we show they share the same core fold as the N- (NtDCA) and C-terminal domains (CtDCA) of archetypal orthoretroviral capsid protein (CA). Moreover, structural comparisons with orthoretroviral CA align PFV NtDCEN and CtDCEN with NtDCA and CtDCA respectively. Further in vitro and functional virological assays reveal that residues making inter-domain NtDCEN—CtDCEN interactions are required for PFV capsid assembly and that intact capsid is required for PFV reverse transcription. These data provide the first information that relates the Gag proteins of Spuma and Orthoretrovirinae and suggests a common ancestor for both lineages containing an ancient CA fold., Author Summary Foamyviruses (FVs) or Spuma-retroviruses derive their name from the cytopathic effects they cause in cell culture. However, infection in humans is benign and FVs have entered the human population through zoonosis from apes resulting in the emergence of Prototype FV (PFV). Like all retroviruses, FVs contain gag, pol and env structural genes and replicate through reverse-transcription and host genome integration. Gag, the major structural protein, is required for genome packaging, virion assembly, trafficking and egress. However, although functionally equivalent, FV and orthoretroviral Gag share little sequence homology and it is unclear how they perform the same function. Therefore, to understand more about relationship between FV and orthoretroviral replication we have carried out structural studies of PFV-Gag. Here we present the structure of CA domains from a central region PFV-Gag and show that despite little sequence similarity they share the same fold as the CA domains of orthoretroviral Gag. These data provide the first information relating the Spuma and Orthoretrovirinae Gag proteins. We discuss our findings in terms of evolutionary divergence of spuma and orthoretroviral lineages.

Published

2016

5. A Small-molecule-controlled System for Efficient Pseudotyping of Prototype Foamy Virus Vectors

Author

Anka Swiersy, Ho Yu-Ping, Kristin Stirnnagel, Dirk Lindemann, and Schnabel Viktor

Subjects

Pharmacology, chemistry.chemical_classification, biology, viruses, biology.organism_classification, Virology, Virus, chemistry, Capsid, Vesicular stomatitis virus, Drug Discovery, Genetics, Pseudotyping, Tissue tropism, Molecular Medicine, Vector (molecular biology), Glycoprotein, Spumavirus, Molecular Biology

Abstract

Foamy virus (FV) vector systems have recently demonstrated their power as efficient gene transfer tools for different target tissues. Unfortunately, FVs cannot be naturally pseudotyped by heterologous viral glycoproteins due to an unusual particle morphogenesis involving a FV Env-dependent particle release process. Therefore, current FV vector systems are constrained to the broad host cell range provided by the cognate viral glycoprotein. We evaluated different approaches for pseudotyping of FV vectors, in which the specific FV Gag–Env interaction, essential for particle egress, is substituted by a small-molecule controlled heterodimerization (HD) system. In one system developed, one HD-domain (HDD) is fused to a membrane-targeting domain (MTD), such as the human immunodeficiency virus (HIV) Gag matrix (MA) subunit, with a second fused to the FV capsid protein. Coexpression of both components with different heterologous viral glycoproteins allowed an efficient, dimerizer-dependent pseudotyping of FV capsids. With this system FV vesicular stomatitis virus glycoprotein (VSV-G) pseudotype titers greater than 1 × 106 IU/ml were obtained, at levels comparable to authentic FV vector particles. As a proof-of-principle we demonstrate that Pac2 cells, naturally resistant to FV vectors, become permissive to FV VSV-G pseudotypes. Similar to other retroviral vectors, this FV pseudotyping system now enables adaptation of cell-specific targeting approaches for FVs.

Published

2012

6. Novel Functions of Prototype Foamy Virus Gag Glycine- Arginine-Rich Boxes in Reverse Transcription and Particle Morphogenesis

Author

Tobias Uhlig, Uwe Fiebig, Kristin Stirnnagel, Erik Müllers, Hanswalter Zentgraf, and Dirk Lindemann

Subjects

Molecular Sequence Data, Immunology, Mutant, Glycine, Gene Products, gag, Biology, Arginine, Virus Replication, Microbiology, Cell Line, chemistry.chemical_compound, Transcription (biology), Virology, Humans, Amino Acid Sequence, Spumavirus, Virus Assembly, Structure and Assembly, C-terminus, Virion, RNA, Reverse Transcription, biology.organism_classification, Molecular biology, Reverse transcriptase, Viral replication, chemistry, Insect Science, RNA, Viral, DNA, HeLa Cells

Abstract

Prototype foamy virus (PFV) Gag lacks the characteristic orthoretroviral Cys-His motifs that are essential for various steps of the orthoretroviral replication cycle, such as RNA packaging, reverse transcription, infectivity, integration, and viral assembly. Instead, it contains three glycine-arginine-rich boxes (GR boxes) in its C terminus that putatively represent a functional equivalent. We used a four-plasmid replication-deficient PFV vector system, with uncoupled RNA genome packaging and structural protein translation, to analyze the effects of deletion and various substitution mutations within each GR box on particle release, particle-associated protein composition, RNA packaging, DNA content, infectivity, particle morphology, and intracellular localization. The degree of viral particle release by all mutants was similar to that of the wild type. Only minimal effects on Pol encapsidation, exogenous reverse transcriptase (RT) activity, and genomic viral RNA packaging were observed. In contrast, particle-associated DNA content and infectivity were drastically reduced for all deletion mutants and were undetectable for all alanine substitution mutants. Furthermore, GR box I mutants had significant changes in particle morphology, and GR box II mutants lacked the typical nuclear localization pattern of PFV Gag. Finally, it could be shown that GR boxes I and III, but not GR box II, can functionally complement each other. It therefore appears that, similar to the orthoretroviral Cys-His motifs, the PFV Gag GR boxes are important for RNA encapsidation, genome reverse transcription, and virion infectivity as well as for particle morphogenesis.

Published

2011

7. Efficient Transient Genetic Manipulation In Vitro and In Vivo by Prototype Foamy Virus-mediated Nonviral RNA Transfer

Author

Benedetta Artegiani, Sara Bragado Alonso, Sylvia Hütter, Martin V. Hamann, Kristin Stirnnagel, Erik Müllers, Dirk Lindemann, Nicole Stanke, and Federico Calegari

Subjects

Transgene, Genetic Vectors, Biology, In Vitro Techniques, Viral vector, Transduction (genetics), Mice, Genome editing, Transduction, Genetic, Cell Line, Tumor, Drug Discovery, Genetics, Animals, Humans, Vector (molecular biology), Transgenes, Spumavirus, Molecular Biology, Subgenomic mRNA, Pharmacology, Gene Transfer Techniques, RNA, RNA-Directed DNA Polymerase, Fibroblasts, biology.organism_classification, Virology, Cell biology, HEK293 Cells, Molecular Medicine, Original Article

Abstract

Vector systems based on different retroviruses are widely used to achieve stable integration and expression of transgenes. More recently, transient genetic manipulation systems were developed that are based on integration- or reverse transcription-deficient retroviruses. Lack of viral genome integration is desirable not only for reducing tumorigenic potential but also for applications requiring transient transgene expression such as reprogramming or genome editing. However, all existing transient retroviral vector systems rely on virus-encoded encapsidation sequences for the transfer of heterologous genetic material. We discovered that the transient transgene expression observed in target cells transduced by reverse transcriptase-deficient foamy virus (FV) vectors is the consequence of subgenomic RNA encapsidation into FV particles. Based on this initial observation, we describe here the establishment of FV vectors that enable the efficient transient expression of various transgenes by packaging, transfer, and de novo translation of nonviral RNAs both in vitro and in vivo. Transient transgene expression levels were comparable to integrase-deficient vectors but, unlike the latter, declined to background levels within a few days. Our results show that this new FV vector system provides a useful, novel tool for efficient transient genetic manipulation of target tissues by transfer of nonviral RNAs.

Published

2014

8. Heparan Sulfate Is an Attachment Factor for Foamy Virus Entry

Author

Conrad Weber, Carsten Scheller, Tatiana Wiktorowicz, Dirk Lindemann, Nicole Armbruster, Kristin Stirnnagel, Kathrin Plochmann, Anne Horn, Jennifer Krieg, Axel Rethwilm, and Eva Gschmack

Subjects

Immunology, Cell, Virus Attachment, Biology, Microbiology, Extracellular matrix, Glycosaminoglycan, chemistry.chemical_compound, Mice, Viral entry, Virology, Cricetinae, medicine, Animals, Humans, Heparin, Cell Membrane, Cellular receptor, Heparan sulfate, Virus Internalization, Molecular biology, Virus-Cell Interactions, medicine.anatomical_structure, chemistry, Cell culture, Insect Science, Cats, Disease Progression, Receptors, Virus, Spumavirus, HT1080, Heparitin Sulfate, Retroviridae Infections

Abstract

The cellular receptor of foamy viruses (FVs) is unknown. The broad spectrum of permissive cells suggests that the cellular receptor is a molecular structure with almost ubiquitous prevalence. Here, we investigated the ability of heparan sulfate (HS), a glycosaminoglycan (GAG) present on the extracellular matrix of many cells, to bind FV particles and to permit prototype FV (PFV) and feline FV (FFV) entry. Permissivity of different cell lines for FV entry correlated with the amount of heparan sulfate present on the cell surface. The resulting 50% cell culture infectious doses (CCID 50 s) were distributed over a range of 4 logs, which means that the most susceptible cell line tested (HT1080) was more than 10,000 times more susceptible for PFV infection than the least susceptible cell line (CRL-2242). HS surface expression varied over a range of 2 logs. HS expression and FV susceptibility were positively correlated ( P < 0.001). Enzymatic digestion of heparan sulfate on HT1080 cells diminished permissivity for PFV entry by a factor of at least 500. Using fast protein liquid chromatography (FPLC), we demonstrated binding of FV vector particles to a gel filtration column packed with heparin, a molecule structurally related to heparan sulfate, allowing for the purification of infectious particles. Both PFV and FFV infection were inhibited by soluble heparin. Our results show that FVs bind to HS and that this interaction is a pivotal step for viral entry, suggesting that HS is a cellular attachment factor for FVs.

Published

2012

9. Prototype foamy virus gag nuclear localization: a novel pathway among retroviruses

Author

Kristin Stirnnagel, Sylvia Kaulfuss, Dirk Lindemann, and Erik Müllers

Subjects

viruses, Immunology, Active Transport, Cell Nucleus, Gene Products, gag, Biology, Protein Sorting Signals, Virus Replication, Microbiology, Cell Line, Virology, medicine, NLS, Humans, Spumavirus, Mitosis, Cell Nucleus, Binding Sites, biology.organism_classification, Molecular biology, Chromatin, Virus-Cell Interactions, Cell nucleus, medicine.anatomical_structure, Viral replication, Microscopy, Fluorescence, Insect Science, Mutant Proteins, Nuclear transport, Nuclear localization sequence

Abstract

Gag nuclear localization has long been recognized as a hallmark of foamy virus (FV) infection. Two required motifs, a chromatin-binding site (CBS) and a nuclear localization signal (NLS), both located in glycine-arginine-rich box II (GRII), have been described. However, the underlying mechanisms of Gag nuclear translocation are largely unknown. We analyzed prototype FV (PFV) Gag nuclear localization using a novel live-cell fluorescence microscopy assay. Furthermore, we characterized the nuclear localization route of Gag mutants tagged with the simian vacuolating virus 40-NLS (SV40-NLS) and also dissected the respective contributions of the CBS and the NLS. We found that PFV Gag does not translocate to the nucleus of interphase cells by NLS-mediated nuclear import and does not possess a functional NLS. PFV Gag nuclear localization occurred only by tethering to chromatin during mitosis. This mechanism was found for endogenously expressed Gag as well as for Gag delivered by infecting viral particles. Thereby, the CBS was absolutely essential, while the NLS was dispensable. Gag CBS-dependent nuclear localization was neither essential for infectivity nor necessary for Pol encapsidation. Interestingly, Gag localization was independent of the presence of Pol, Env, and viral RNA. The addition of a heterologous SV40-NLS resulted in the nuclear import of PFV Gag in interphase cells, rescued the nuclear localization deficiency but not the infectivity defect of a PFV Gag ΔGRII mutant, and did not enhance FV's ability to infect G 1 /S-phase-arrested cells. Thus, PFV Gag nuclear localization follows a novel pathway among orthoretroviral Gag proteins.

Published

2011

10. Abstract 5341: GlioMath-DD: A multidisciplinary approach to study glioma evolution and identify targets for individualized therapies

Author

Kathrin Geiger, Andreas Deutsch, Wolfgang E. Nagel, Leoni A. Kunz-Schughart, Achim Temme, Ralf Wiedemuth, Barbara Klink, Khalil Abou-El-Ardat, Kristin Stirnnagel, Evelin Schröck, Gabriele Schackert, Alvaro Köhn-Luque, Alexander Krüger, Mirjam Ingargiola, Michael Seifert, and Andreas Beyer

Subjects

Oncology, Cancer Research, Lower grade, medicine.medical_specialty, business.industry, Brain tumor, Astrocytoma, Cancer, Comparative Genome Hybridization, medicine.disease, Bioinformatics, Glioma, Internal medicine, medicine, Low-Grade Glioma, Copy-number variation, business

Abstract

Glioblastoma multiforme (GBM) is the most prevalent malignant primary brain tumor in adults. GBM is classified as primary if it is assumed to have arisen de novo or as secondary if it progressed from lower grade astrocytoma. Previous studies have found that primary and secondary GBMs have distinct molecular and mutational profiles. Both have a grim prognosis with survival times of about a year with therapy. Although much progress in delineating the temporal order of mutations and copy number aberrations in the progression of lower grade gliomas was made in the past years, none of the studies have actively followed individual tumors through their progression. Whereas this method can detect aberrations that are prevalent in gliomas, it can miss events that are important in a subset of gliomas or are necessary for progression. The GlioMath-DD consortium is an interdisciplinary collaboration of several groups at the Technische Universität Dresden (TU-Dresden) aiming to study the progression of gliomas and to come up with a mathematical model for gliomagenesis. The work involves analyzing pairs of gliomas obtained from patients who had presented with a low grade glioma and who later had a recurrence of a higher grade glioma. All tumors were checked by pathologists and then high quality DNA and RNA material extracted and used for analysis. The tumors are analyzed for copy number variations (CNV) by array comparative genome hybridization (aCGH), while gene expression changes and small mutations are analyzed using high-throughput sequencing (RNA- and Exome-seq). The data gleaned from these experiments and from in vitro models of cell growth and spheroid formation will be used by bioinformaticians and mathematicians to infer key signaling networks and formulate a mathematical model of glioma progression. The ultimate aim of this work that spans two and a half years is to create a comprehensive model of glioma promotion and progression. Furthermore, it will pinpoint driver mutations and aberrations that contribute to this progression and eventually isolate biomarkers for diagnosis and therapy. During the conference, we will present preliminary genetic data of our ongoing study. Acknowledgements: The GlioMath-DD project (coordinator: Andreas Deutsch; SAB-Number 100098214) is funded by the European Social Fund (ESF) and the Free State of Saxony Citation Format: Evelin Schröck, Khalil Abou-El-Ardat, Ralf Wiedemuth, Michael Seifert, Alvaro Köhn-Luque, Mirjam Ingargiola, Kristin Stirnnagel, Alexander Krüger, Wolfgang Nagel, Kathrin Geiger, Andreas Beyer, Leoni A. Kunz-Schughart, Gabriele Schackert, Achim Temme, Barbara Klink, Andreas Deutsch. GlioMath-DD: A multidisciplinary approach to study glioma evolution and identify targets for individualized therapies. [abstract]. In: Proceedings of the 105th Annual Meeting of the American Association for Cancer Research; 2014 Apr 5-9; San Diego, CA. Philadelphia (PA): AACR; Cancer Res 2014;74(19 Suppl):Abstract nr 5341. doi:10.1158/1538-7445.AM2014-5341

Published

2014

11. Differential pH-dependent cellular uptake pathways among foamy viruses elucidated using dual-colored fluorescent particles

Author

Don C. Lamb, Dorothee Schupp, Dirk Lindemann, Aurélie Dupont, Kristin Stirnnagel, Volodymyr Kudryavtsev, Erik Müllers, and Juliane Reh

Subjects

Signal peptide, lcsh:Immunologic diseases. Allergy, viruses, Recombinant Fusion Proteins, Intracellular targeting, Entry, Virus, Fluorescence, Cell Line, Retrovirus, Live-cell imaging, Viral Envelope Proteins, Live cell imaging, Virology, Humans, Spumavirus, chemistry.chemical_classification, Syncytium, biology, Staining and Labeling, Research, Time-lapse microscopy, Hydrogen-Ion Concentration, Virus Internalization, biology.organism_classification, Molecular biology, Cell biology, Luminescent Proteins, Infectious Diseases, chemistry, Capsid, Capsid Proteins, Foamy virus, Disassembly, Glycoprotein, lcsh:RC581-607

Abstract

Background It is thought that foamy viruses (FVs) enter host cells via endocytosis because all FV glycoproteins examined display pH-dependent fusion activities. Only the prototype FV (PFV) glycoprotein has also significant fusion activity at neutral pH, suggesting that its uptake mechanism may deviate from other FVs. To gain new insights into the uptake processes of FV in individual live host cells, we developed fluorescently labeled infectious FVs. Results N-terminal tagging of the FV envelope leader peptide domain with a fluorescent protein resulted in efficient incorporation of the fluorescently labeled glycoprotein into secreted virions without interfering with their infectivity. Double-tagged viruses consisting of an eGFP-tagged PFV capsid (Gag-eGFP) and mCherry-tagged Env (Ch-Env) from either PFV or macaque simian FV (SFVmac) were observed during early stages of the infection pathway. PFV Env, but not SFVmac Env, containing particles induced strong syncytia formation on target cells. Both virus types showed trafficking of double-tagged virions towards the cell center. Upon fusion and subsequent capsid release into the cytosol, accumulation of naked capsid proteins was observed within four hours in the perinuclear region, presumably representing the centrosomes. Interestingly, virions harboring fusion-defective glycoproteins still promoted virus attachment and uptake, but failed to show syncytia formation and perinuclear capsid accumulation. Biochemical and initial imaging analysis indicated that productive fusion events occur predominantly within 4–6 h after virus attachment. Non-fused or non-fusogenic viruses are rapidly cleared from the cells by putative lysosomal degradation. Quantitative monitoring of the fraction of individual viruses containing both Env and capsid signals as a function of time demonstrated that PFV virions fused within the first few minutes, whereas fusion of SFVmac virions was less pronounced and observed over the entire 90 minutes measured. Conclusions The characterized double-labeled FVs described here provide new mechanistic insights into FV early entry steps, demonstrating that productive viral fusion occurs early after target cell attachment and uptake. The analysis highlights apparent differences in the uptake pathways of individual FV species. Furthermore, the infectious double-labeled FVs promise to provide important tools for future detailed analyses on individual FV fusion events in real time using advanced imaging techniques.

Published

2012

12. Tracking Image Cross-Correlation for Elucidating the Fusion Process of Viruses

Author

Don C. Lamb, Kristin Stirnnagel, Florian Perrotton, Aurélie Dupont, Erik Müllers, Dorothee Schupp, and Dirk Lindemann

Subjects

0303 health sciences, Fusion, biology, Biophysics, Colocalization, Lipid bilayer fusion, biology.organism_classification, Endocytosis, Virology, Virus, 3. Good health, Cell biology, 03 medical and health sciences, 0302 clinical medicine, Retrovirus, Capsid, Viral entry, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Promising as a gene carrier, the Foamy virus (FV) is an atypical retrovirus that shares similarities with HIV and the hepatitis B virus. Despite numerous biochemical studies, its entry pathway remains unclear, namely whether entry occurs through fusion at the plasma membrane or after endocytosis. To investigate this issue, dual-color fluorescent viruses were engineered with a GFP-labeled capsid and a mCherry-labeled envelope. Thus, the release of the capsid from the envelope would result in a loss of colocalization of the two colors at the single virus level. Using 3D single virus tracing, we followed the entry of the fluorescent viruses in living cells. In such experiments, a compromise is made between low phototoxicity for the cells and sufficient signal-to-noise ratio for tracking. Therefore, it is often difficult to rely on the fluorescence intensity to estimate colocalization. Cross-correlation approaches are highly sensitive to colocalization and coordinated motion but none of the existing methods are applicable to single particle tracking. We developed a novel approach, Tracking Image Cross-correlation (TrIC), which combines image cross-correlation and single particle tracking. The image cross-correlation analysis yields the colocalization status of the particle as well as the average distance between the two labels. The combination of this dynamical colocalization information with the instantaneous velocity of the particle and its position within the cell allows us to clarify the Foamy virus entry pathway. We compared two types of FVs and demonstrated that the prototype FV can enter the cell by either endocytosis or membrane fusion whereas the simian FV was only observed to fuse after endocytosis. Interestingly, our analysis revealed an intermediate stage during the fusion process where the capsid and envelope separate by ∼400nm but are still attached for ∼5 minutes before fusion is completed.

13. Analysis of Prototype Foamy Virus particle-host cell interaction with autofluorescent retroviral particles

Author

Juliane Reh, Daniel Lüftenegger, Petra Schwille, Arend Große, Hanswalter Zentgraf, Heiko Keller, Annett Stange, Kristin Stirnnagel, Erik Müllers, Helmut Hanenberg, Anka Swiersy, Salvatore Chiantia, Dirk Lindemann, Nicole Stanke, and Technische Universität Dresden

Subjects

lcsh:Immunologic diseases. Allergy, Simian foamy virus, Virus, Green fluorescent protein, Cell Line, Transduction (genetics), Viral Proteins, ddc:570, Virology, Animals, Humans, ddc:610, Zebrafish, Recombination, Genetic, biology, Staining and Labeling, Research, oamy virus, particle-host cell interaction, Wild type, biology.organism_classification, Molecular biology, Virus, Virologie, Virologie, retrovirale Partikel, Luminescent Proteins, Infectious Diseases, Capsid, Microscopy, Fluorescence, Cell culture, Host-Pathogen Interactions, lcsh:RC581-607, Intracellular

Abstract

Background The foamy virus (FV) replication cycle displays several unique features, which set them apart from orthoretroviruses. First, like other B/D type orthoretroviruses, FV capsids preassemble at the centrosome, but more similar to hepadnaviruses, FV budding is strictly dependent on cognate viral glycoprotein coexpression. Second, the unusually broad host range of FV is thought to be due to use of a very common entry receptor present on host cell plasma membranes, because all cell lines tested in vitro so far are permissive. Results In order to take advantage of modern fluorescent microscopy techniques to study FV replication, we have created FV Gag proteins bearing a variety of protein tags and evaluated these for their ability to support various steps of FV replication. Addition of even small N-terminal HA-tags to FV Gag severely impaired FV particle release. For example, release was completely abrogated by an N-terminal autofluorescent protein (AFP) fusion, despite apparently normal intracellular capsid assembly. In contrast, C-terminal Gag-tags had only minor effects on particle assembly, egress and particle morphogenesis. The infectivity of C-terminal capsid-tagged FV vector particles was reduced up to 100-fold in comparison to wild type; however, infectivity was rescued by coexpression of wild type Gag and assembly of mixed particles. Specific dose-dependent binding of fluorescent FV particles to target cells was demonstrated in an Env-dependent manner, but not binding to target cell-extracted- or synthetic- lipids. Screening of target cells of various origins resulted in the identification of two cell lines, a human erythroid precursor- and a zebrafish- cell line, resistant to FV Env-mediated FV- and HIV-vector transduction. Conclusions We have established functional, autofluorescent foamy viral particles as a valuable new tool to study FV - host cell interactions using modern fluorescent imaging techniques. Furthermore, we succeeded for the first time in identifying two cell lines resistant to Prototype Foamy Virus Env-mediated gene transfer. Interestingly, both cell lines still displayed FV Env-dependent attachment of fluorescent retroviral particles, implying a post-binding block potentially due to lack of putative FV entry cofactors. These cell lines might ultimately lead to the identification of the currently unknown ubiquitous cellular entry receptor(s) of FVs.