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11 results on '"Marjomäki, Varpu"'

1. Structural Insight into CVB3-VLP Non-Adjuvanted Vaccine

Author

Hankaniemi, Minna M, Baikoghli, Mo A, Stone, Virginia M, Xing, Li, Väätäinen, Outi, Soppela, Saana, Sioofy-Khojine, Amirbabak, Saarinen, Niila VV, Ou, Tingwei, Anson, Brandon, Hyöty, Heikki, Marjomäki, Varpu, Flodström-Tullberg, Malin, Cheng, R Holland, Hytönen, Vesa P, and Laitinen, Olli H

Subjects
Biomedical and Clinical Sciences, Immunology, Biotechnology, Immunization, Prevention, Heart Disease, Vaccine Related, Infectious Diseases, Cardiovascular, 3.4 Vaccines, Prevention of disease and conditions, and promotion of well-being, Infection, Good Health and Well Being, Coxsackievirus B, vaccine, virus-like particle, Microbiology, Medical microbiology
Abstract

Coxsackievirus B (CVB) enteroviruses are common pathogens that can cause acute and chronic myocarditis, dilated cardiomyopathy, aseptic meningitis, and they are hypothesized to be a causal factor in type 1 diabetes. The licensed enterovirus vaccines and those currently in clinical development are traditional inactivated or live attenuated vaccines. Even though these vaccines work well in the prevention of enterovirus diseases, new vaccine technologies, like virus-like particles (VLPs), can offer important advantages in the manufacturing and epitope engineering. We have previously produced VLPs for CVB3 and CVB1 in insect cells. Here, we describe the production of CVB3-VLPs with enhanced production yield and purity using an improved purification method consisting of tangential flow filtration and ion exchange chromatography, which is compatible with industrial scale production. We also resolved the CVB3-VLP structure by Cryo-Electron Microscopy imaging and single particle reconstruction. The VLP diameter is 30.9 nm on average, and it is similar to Coxsackievirus A VLPs and the expanded enterovirus cell-entry intermediate (the 135s particle), which is ~2 nm larger than the mature virion. High neutralizing and total IgG antibody levels, the latter being a predominantly Th2 type (IgG1) phenotype, were detected in C57BL/6J mice immunized with non-adjuvanted CVB3-VLP vaccine. The structural and immunogenic data presented here indicate the potential of this improved methodology to produce highly immunogenic enterovirus VLP-vaccines in the future.

Published
2020

2. Structural characterization of site-modified nanocapsid with monodispersed gold clusters.

Author

Stark, Marie C, Baikoghli, Mo A, Lahtinen, Tanja, Malola, Sami, Xing, Li, Nguyen, Michelle, Nguyen, Marina, Sikaroudi, Aria, Marjomäki, Varpu, Häkkinen, Hannu, and Cheng, R Holland

Subjects
Hepatitis E virus, Gold, Maleimides, Recombinant Proteins, Capsid Proteins, Cryoelectron Microscopy, Microscopy, Electron, Transmission, Metal Nanoparticles, Microscopy, Electron, Transmission
Abstract

Hepatitis E Virus-like particles self-assemble in to noninfectious nanocapsids that are resistant to proteolytic/acidic mucosal delivery conditions. Previously, the nanocapsid was engineered to specifically bind and enter breast cancer cells, where successful tumor targeting was demonstrated in animal models. In the present study, the nanocapsid surface was modified with a solvent-exposed cysteine to conjugate monolayer protected gold nanoclusters (AuNC). Unlike commercially available gold nanoparticles, AuNCs monodisperse in water and are composed of a discrete number of gold atoms, forming a crystalline gold core. Au102 pMBA44 (Au102) was an ideal conjugate given its small 2.5 nm size and detectability in cryoEM. Au102 was bound directly to nanocapsid surface cysteines via direct ligand exchange. In addition, Au102 was functionalized with a maleimide linker (Au102_C6MI) for maleimide-thiol conjugation to nanocapsid cysteines. The AuNC-bound nanocapsid constructs were conjugated in various conditions. We found Au102_C6MI to bind nanocapsid more efficiently, while Au102 remained more soluble over time. Nanocapsids conjugated to Au102_C6MI were imaged in cryoEM for single particle reconstruction to localize AuNC position on the nanocapsid surface. We resolved five unique high intensity volumes that formed a ring-shaped density at the 5-fold symmetry center. This finding was further supported by independent rigid modeling.

Published
2017

3. Structural characterization of site-modified nanocapsid with monodispersed gold clusters

Author

Stark, Marie C, Baikoghli, Mo A, Lahtinen, Tanja, Malola, Sami, Xing, Li, Nguyen, Michelle, Nguyen, Marina, Sikaroudi, Aria, Marjomäki, Varpu, Häkkinen, Hannu, and Cheng, R Holland

Subjects
Medical Biotechnology, Biomedical and Clinical Sciences, Chemical Sciences, Bioengineering, Women's Health, Cancer, Breast Cancer, Nanotechnology, Generic health relevance, Good Health and Well Being, Capsid Proteins, Cryoelectron Microscopy, Gold, Hepatitis E virus, Maleimides, Metal Nanoparticles, Microscopy, Electron, Transmission, Recombinant Proteins
Abstract

Hepatitis E Virus-like particles self-assemble in to noninfectious nanocapsids that are resistant to proteolytic/acidic mucosal delivery conditions. Previously, the nanocapsid was engineered to specifically bind and enter breast cancer cells, where successful tumor targeting was demonstrated in animal models. In the present study, the nanocapsid surface was modified with a solvent-exposed cysteine to conjugate monolayer protected gold nanoclusters (AuNC). Unlike commercially available gold nanoparticles, AuNCs monodisperse in water and are composed of a discrete number of gold atoms, forming a crystalline gold core. Au102 pMBA44 (Au102) was an ideal conjugate given its small 2.5 nm size and detectability in cryoEM. Au102 was bound directly to nanocapsid surface cysteines via direct ligand exchange. In addition, Au102 was functionalized with a maleimide linker (Au102_C6MI) for maleimide-thiol conjugation to nanocapsid cysteines. The AuNC-bound nanocapsid constructs were conjugated in various conditions. We found Au102_C6MI to bind nanocapsid more efficiently, while Au102 remained more soluble over time. Nanocapsids conjugated to Au102_C6MI were imaged in cryoEM for single particle reconstruction to localize AuNC position on the nanocapsid surface. We resolved five unique high intensity volumes that formed a ring-shaped density at the 5-fold symmetry center. This finding was further supported by independent rigid modeling.

Published
2017

4. Additives for vaccine storage to improve thermal stability of adenoviruses from hours to months.

Author

Pelliccia, Maria, Andreozzi, Patrizia, Paulose, Jayson, D'Alicarnasso, Marco, Cagno, Valeria, Donalisio, Manuela, Civra, Andrea, Broeckel, Rebecca M, Haese, Nicole, Jacob Silva, Paulo, Carney, Randy P, Marjomäki, Varpu, Streblow, Daniel N, Lembo, David, Stellacci, Francesco, Vitelli, Vincenzo, and Krol, Silke

Subjects
Animals, Mice, Gold, Polyethylene Glycols, Sucrose, Excipients, Feasibility Studies, Models, Animal, Drug Stability, Drug Storage, Models, Biological, Half-Life, Time Factors, Metal Nanoparticles, Cold Temperature, Adenovirus Vaccines, Immunogenicity, Vaccine, Immunogenicity, Vaccine, Models, Animal, Biological
Abstract

Up to 80% of the cost of vaccination programmes is due to the cold chain problem (that is, keeping vaccines cold). Inexpensive, biocompatible additives to slow down the degradation of virus particles would address the problem. Here we propose and characterize additives that, already at very low concentrations, improve the storage time of adenovirus type 5. Anionic gold nanoparticles (10-8-10-6 M) or polyethylene glycol (PEG, molecular weight ∼8,000 Da, 10-7-10-4 M) increase the half-life of a green fluorescent protein expressing adenovirus from ∼48 h to 21 days at 37 °C (from 7 to >30 days at room temperature). They replicate the known stabilizing effect of sucrose, but at several orders of magnitude lower concentrations. PEG and sucrose maintained immunogenicity in vivo for viruses stored for 10 days at 37 °C. To achieve rational design of viral-vaccine stabilizers, our approach is aided by simplified quantitative models based on a single rate-limiting step.

Published
2016

5. Additives for vaccine storage to improve thermal stability of adenoviruses from hours to months

Author

Pelliccia, Maria, Andreozzi, Patrizia, Paulose, Jayson, D’Alicarnasso, Marco, Cagno, Valeria, Donalisio, Manuela, Civra, Andrea, Broeckel, Rebecca M, Haese, Nicole, Jacob Silva, Paulo, Carney, Randy P, Marjomäki, Varpu, Streblow, Daniel N, Lembo, David, Stellacci, Francesco, Vitelli, Vincenzo, and Krol, Silke

Subjects
Vaccine Related, Prevention, Immunization, Biotechnology, Infectious Diseases, Bioengineering, Infection, Adenovirus Vaccines, Animals, Cold Temperature, Drug Stability, Drug Storage, Excipients, Feasibility Studies, Gold, Half-Life, Immunogenicity, Vaccine, Metal Nanoparticles, Mice, Models, Animal, Models, Biological, Polyethylene Glycols, Sucrose, Time Factors
Abstract

Up to 80% of the cost of vaccination programmes is due to the cold chain problem (that is, keeping vaccines cold). Inexpensive, biocompatible additives to slow down the degradation of virus particles would address the problem. Here we propose and characterize additives that, already at very low concentrations, improve the storage time of adenovirus type 5. Anionic gold nanoparticles (10-8-10-6 M) or polyethylene glycol (PEG, molecular weight ∼8,000 Da, 10-7-10-4 M) increase the half-life of a green fluorescent protein expressing adenovirus from ∼48 h to 21 days at 37 °C (from 7 to >30 days at room temperature). They replicate the known stabilizing effect of sucrose, but at several orders of magnitude lower concentrations. PEG and sucrose maintained immunogenicity in vivo for viruses stored for 10 days at 37 °C. To achieve rational design of viral-vaccine stabilizers, our approach is aided by simplified quantitative models based on a single rate-limiting step.

Published
2016

6. Permeability changes of integrin-containing multivesicular structures triggered by picornavirus entry.

Author

Soonsawad, Pan, Paavolainen, Lassi, Upla, Paula, Weerachatyanukul, Wattana, Rintanen, Nina, Espinoza, Juan, McNerney, Gregory, Marjomäki, Varpu, and Cheng, R Holland

Subjects
Cell Line, Tumor, Cell Membrane, Cytoplasm, Endosomes, Humans, Picornaviridae, Picornaviridae Infections, Integrin alpha2beta1, Microscopy, Confocal, Permeability, Electron Microscope Tomography, Multivesicular Bodies, Cell Line, Tumor, Microscopy, Confocal, General Science & Technology
Abstract

Cellular uptake of clustered α2β1-integrin induces the formation of membrane compartments that subsequently mature into a multivesicular body (MVB). Enhanced internalization mediated by clustered integrins was observed upon infection by the picornavirus echovirus 1 (EVI). We elucidated the structural features of virus-induced MVBs (vMVBs) in comparison to antibody-induced control MVBs (mock infection) by means of high-pressure cryo fixation of cells followed by immuno electron tomography during early entry of the virus. Three-dimensional tomograms revealed a marked increase in the size and complexity of these vMVBs and the intraluminal vesicles (ILVs) at 2 and 3.5 hours post infection (p.i.), in contrast to the control MVBs without virus. Breakages in the membranes of vMVBs were detected from tomograms after 2 and especially after 3.5 h suggesting that these breakages could facilitate the genome release to the cytoplasm. The in situ neutral-red labeling of viral genome showed that virus uncoating starts as early as 30 min p.i., while an increase of permeability was detected in the vMVBs between 1 and 3 hours p.i., based on a confocal microscopy assay. Altogether, the data show marked morphological changes in size and permeability of the endosomes in the infectious entry pathway of this non-enveloped enterovirus and suggest that the formed breakages facilitate the transfer of the genome to the cytoplasm for replication.

Published
2014

7. Compensation of missing wedge effects with sequential statistical reconstruction in electron tomography.

Author

Paavolainen, Lassi, Acar, Erman, Tuna, Uygar, Peltonen, Sari, Moriya, Toshio, Soonsawad, Pan, Marjomäki, Varpu, Cheng, R Holland, and Ruotsalainen, Ulla

Subjects
Artifacts, Algorithms, Image Processing, Computer-Assisted, Electron Microscope Tomography, Image Processing, Computer-Assisted, General Science & Technology
Abstract

Electron tomography (ET) of biological samples is used to study the organization and the structure of the whole cell and subcellular complexes in great detail. However, projections cannot be acquired over full tilt angle range with biological samples in electron microscopy. ET image reconstruction can be considered an ill-posed problem because of this missing information. This results in artifacts, seen as the loss of three-dimensional (3D) resolution in the reconstructed images. The goal of this study was to achieve isotropic resolution with a statistical reconstruction method, sequential maximum a posteriori expectation maximization (sMAP-EM), using no prior morphological knowledge about the specimen. The missing wedge effects on sMAP-EM were examined with a synthetic cell phantom to assess the effects of noise. An experimental dataset of a multivesicular body was evaluated with a number of gold particles. An ellipsoid fitting based method was developed to realize the quantitative measures elongation and contrast in an automated, objective, and reliable way. The method statistically evaluates the sub-volumes containing gold particles randomly located in various parts of the whole volume, thus giving information about the robustness of the volume reconstruction. The quantitative results were also compared with reconstructions made with widely-used weighted backprojection and simultaneous iterative reconstruction technique methods. The results showed that the proposed sMAP-EM method significantly suppresses the effects of the missing information producing isotropic resolution. Furthermore, this method improves the contrast ratio, enhancing the applicability of further automatic and semi-automatic analysis. These improvements in ET reconstruction by sMAP-EM enable analysis of subcellular structures with higher three-dimensional resolution and contrast than conventional methods.

Published
2014

8. Compensation of Missing Wedge Effects with Sequential Statistical Reconstruction in Electron Tomography

Author

Paavolainen, Lassi, Acar, Erman, Tuna, Uygar, Peltonen, Sari, Moriya, Toshio, Soonsawad, Pan, Marjomäki, Varpu, Cheng, R Holland, and Ruotsalainen, Ulla

Subjects
Physical Sciences, Condensed Matter Physics, Bioengineering, Biomedical Imaging, Generic health relevance, Algorithms, Artifacts, Electron Microscope Tomography, Image Processing, Computer-Assisted, General Science & Technology
Abstract

Electron tomography (ET) of biological samples is used to study the organization and the structure of the whole cell and subcellular complexes in great detail. However, projections cannot be acquired over full tilt angle range with biological samples in electron microscopy. ET image reconstruction can be considered an ill-posed problem because of this missing information. This results in artifacts, seen as the loss of three-dimensional (3D) resolution in the reconstructed images. The goal of this study was to achieve isotropic resolution with a statistical reconstruction method, sequential maximum a posteriori expectation maximization (sMAP-EM), using no prior morphological knowledge about the specimen. The missing wedge effects on sMAP-EM were examined with a synthetic cell phantom to assess the effects of noise. An experimental dataset of a multivesicular body was evaluated with a number of gold particles. An ellipsoid fitting based method was developed to realize the quantitative measures elongation and contrast in an automated, objective, and reliable way. The method statistically evaluates the sub-volumes containing gold particles randomly located in various parts of the whole volume, thus giving information about the robustness of the volume reconstruction. The quantitative results were also compared with reconstructions made with widely-used weighted backprojection and simultaneous iterative reconstruction technique methods. The results showed that the proposed sMAP-EM method significantly suppresses the effects of the missing information producing isotropic resolution. Furthermore, this method improves the contrast ratio, enhancing the applicability of further automatic and semi-automatic analysis. These improvements in ET reconstruction by sMAP-EM enable analysis of subcellular structures with higher three-dimensional resolution and contrast than conventional methods.

Published
2014

9. Permeability Changes of Integrin-Containing Multivesicular Structures Triggered by Picornavirus Entry

Author

Soonsawad, Pan, Paavolainen, Lassi, Upla, Paula, Weerachatyanukul, Wattana, Rintanen, Nina, Espinoza, Juan, McNerney, Gregory, Marjomäki, Varpu, and Cheng, R Holland

Subjects
Medical Microbiology, Biomedical and Clinical Sciences, Biological Sciences, Emerging Infectious Diseases, Infectious Diseases, Biotechnology, 2.1 Biological and endogenous factors, 2.2 Factors relating to the physical environment, Aetiology, Infection, Good Health and Well Being, Cell Line, Tumor, Cell Membrane, Cytoplasm, Electron Microscope Tomography, Endosomes, Humans, Integrin alpha2beta1, Microscopy, Confocal, Multivesicular Bodies, Permeability, Picornaviridae, Picornaviridae Infections, General Science & Technology
Abstract

Cellular uptake of clustered α2β1-integrin induces the formation of membrane compartments that subsequently mature into a multivesicular body (MVB). Enhanced internalization mediated by clustered integrins was observed upon infection by the picornavirus echovirus 1 (EVI). We elucidated the structural features of virus-induced MVBs (vMVBs) in comparison to antibody-induced control MVBs (mock infection) by means of high-pressure cryo fixation of cells followed by immuno electron tomography during early entry of the virus. Three-dimensional tomograms revealed a marked increase in the size and complexity of these vMVBs and the intraluminal vesicles (ILVs) at 2 and 3.5 hours post infection (p.i.), in contrast to the control MVBs without virus. Breakages in the membranes of vMVBs were detected from tomograms after 2 and especially after 3.5 h suggesting that these breakages could facilitate the genome release to the cytoplasm. The in situ neutral-red labeling of viral genome showed that virus uncoating starts as early as 30 min p.i., while an increase of permeability was detected in the vMVBs between 1 and 3 hours p.i., based on a confocal microscopy assay. Altogether, the data show marked morphological changes in size and permeability of the endosomes in the infectious entry pathway of this non-enveloped enterovirus and suggest that the formed breakages facilitate the transfer of the genome to the cytoplasm for replication.

Published
2014

10. Calpains promote α2β1 integrin turnover in nonrecycling integrin pathway

Author

Rintanen, Nina, Karjalainen, Mikko, Alanko, Jonna, Paavolainen, Lassi, Mäki, Anita, Nissinen, Liisa, Lehkonen, Moona, Kallio, Katri, Cheng, R Holland, Upla, Paula, Ivaska, Johanna, and Marjomäki, Varpu

Subjects
Biochemistry and Cell Biology, Biological Sciences, Calpain, Cell Line, Tumor, Cell Membrane, Enterovirus B, Human, Focal Adhesions, Humans, Integrin alpha2beta1, Protein Transport, Signal Transduction, Medical and Health Sciences, Developmental Biology, Biochemistry and cell biology
Abstract

Collagen receptor integrins recycle between the plasma membrane and endosomes and facilitate formation and turnover of focal adhesions. In contrast, clustering of α2β1 integrin with antibodies or the human pathogen echovirus 1 (EV1) causes redistribution of α2 integrin to perinuclear multivesicular bodies, α2-MVBs. We show here that the internalized clustered α2 integrin remains in α2-MVBs and is not recycled back to the plasma membrane. Instead, receptor clustering and internalization lead to an accelerated down-regulation of α2β1 integrin compared to the slow turnover of unclustered α2 integrin. EV1 infection or integrin degradation is not associated with proteasomal or autophagosomal processes and shows no significant association with lysosomal pathway. In contrast, degradation is dependent on calpains, such that it is blocked by calpain inhibitors. We show that active calpain is present in α2-MVBs, internalized clustered α2β1 integrin coprecipitates with calpain-1, and calpain enzymes can degrade α2β1 integrin. In conclusion, we identified a novel virus- and clustering-specific pathway that diverts α2β1 integrin from its normal endo/exocytic traffic to a nonrecycling, calpain-dependent degradative endosomal route.

Published
2012

11. Calpains promote α2β1 integrin turnover in nonrecycling integrin pathway.

Author

Rintanen, Nina, Karjalainen, Mikko, Alanko, Jonna, Paavolainen, Lassi, Mäki, Anita, Nissinen, Liisa, Lehkonen, Moona, Kallio, Katri, Cheng, R Holland, Upla, Paula, Ivaska, Johanna, and Marjomäki, Varpu

Subjects
Cell Line, Tumor, Cell Membrane, Focal Adhesions, Humans, Enterovirus B, Human, Calpain, Integrin alpha2beta1, Signal Transduction, Protein Transport, Cell Line, Tumor, Enterovirus B, Human, Biological Sciences, Medical and Health Sciences, Developmental Biology
Abstract

Collagen receptor integrins recycle between the plasma membrane and endosomes and facilitate formation and turnover of focal adhesions. In contrast, clustering of α2β1 integrin with antibodies or the human pathogen echovirus 1 (EV1) causes redistribution of α2 integrin to perinuclear multivesicular bodies, α2-MVBs. We show here that the internalized clustered α2 integrin remains in α2-MVBs and is not recycled back to the plasma membrane. Instead, receptor clustering and internalization lead to an accelerated down-regulation of α2β1 integrin compared to the slow turnover of unclustered α2 integrin. EV1 infection or integrin degradation is not associated with proteasomal or autophagosomal processes and shows no significant association with lysosomal pathway. In contrast, degradation is dependent on calpains, such that it is blocked by calpain inhibitors. We show that active calpain is present in α2-MVBs, internalized clustered α2β1 integrin coprecipitates with calpain-1, and calpain enzymes can degrade α2β1 integrin. In conclusion, we identified a novel virus- and clustering-specific pathway that diverts α2β1 integrin from its normal endo/exocytic traffic to a nonrecycling, calpain-dependent degradative endosomal route.

Published
2012

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