Your search keyword '"Transgenes physiology"' showing total 25 results

1. Generation of transgenic chickens expressing the human erythropoietin (hEPO) gene in an oviduct-specific manner: Production of transgenic chicken eggs containing human erythropoietin in egg whites.

Author

Kwon MS, Koo BC, Kim D, Nam YH, Cui XS, Kim NH, and Kim T

Subjects

Animals, Animals, Genetically Modified genetics, Chickens genetics, Erythropoietin genetics, Female, Genetic Vectors administration & dosage, Humans, Lentivirus genetics, Male, Ovalbumin genetics, Promoter Regions, Genetic, Animals, Genetically Modified metabolism, Chickens metabolism, Egg White, Erythropoietin metabolism, Oviducts metabolism, Transgenes physiology

Abstract

The transgenic chicken has been considered as a prospective bioreactor for large-scale production of costly pharmaceutical proteins. In the present study, we report successful generation of transgenic hens that lay eggs containing a high concentration of human erythropoietin (hEPO) in the ovalbumin. Using a feline immunodeficiency virus (FIV)-based pseudotyped lentivirus vector enveloped with G glycoproteins of the vesicular stomatitis virus, the replication-defective vector virus carrying the hEPO gene under the control of the chicken ovalbumin promoter was microinjected to the subgerminal cavity of freshly laid chicken eggs (stage X). Stable germline transmission of the hEPO transgene to the G1 progeny, which were non-mosaic and hemizygous for the hEPO gene under the ovalbumin promoter, was confirmed by mating of a G0 rooster with non-transgenic hens. Quantitative analysis of hEPO in the egg whites and in the blood samples taken from G1 transgenic chickens showed 4,810 ~ 6,600 IU/ml (40.1 ~ 55.0 μg/ml) and almost no detectable concentration, respectively, indicating tightly regulated oviduct-specific expression of the hEPO transgene. In terms of biological activity, there was no difference between the recombinant hEPO contained in the transgenic egg white and the commercially available counterpart, in vitro. We suggest that these results imply an important step toward efficient production of human cytokines from a transgenic animal bioreactor., Competing Interests: The authors have declared that no competing interests exist.

Published

2018

2. Ketocarotenoid Production in Soybean Seeds through Metabolic Engineering.

Author

Pierce EC, LaFayette PR, Ortega MA, Joyce BL, Kopsell DA, and Parrott WA

Subjects

Canthaxanthin biosynthesis, Cloning, Molecular, DNA, Bacterial genetics, Gene Expression Regulation, Plant, Genes, Plant genetics, Plants, Genetically Modified genetics, Plants, Genetically Modified growth & development, Seeds genetics, Seeds growth & development, Glycine max genetics, Glycine max growth & development, Carotenoids biosynthesis, Metabolic Engineering, Metabolic Networks and Pathways genetics, Plants, Genetically Modified metabolism, Seeds metabolism, Glycine max metabolism, Transgenes physiology

Abstract

The pink or red ketocarotenoids, canthaxanthin and astaxanthin, are used as feed additives in the poultry and aquaculture industries as a source of egg yolk and flesh pigmentation, as farmed animals do not have access to the carotenoid sources of their wild counterparts. Because soybean is already an important component in animal feed, production of these carotenoids in soybean could be a cost-effective means of delivery. In order to characterize the ability of soybean seed to produce carotenoids, soybean cv. Jack was transformed with the crtB gene from Pantoea ananatis, which codes for phytoene synthase, an enzyme which catalyzes the first committed step in the carotenoid pathway. The crtB gene was engineered together in combinations with ketolase genes (crtW from Brevundimonas sp. strain SD212 and bkt1 from Haematococcus pluvialis) to produce ketocarotenoids; all genes were placed under the control of seed-specific promoters. HPLC results showed that canthaxanthin is present in the transgenic seeds at levels up to 52 μg/g dry weight. Transgenic seeds also accumulated other compounds in the carotenoid pathway, such as astaxanthin, lutein, β-carotene, phytoene, α-carotene, lycopene, and β-cryptoxanthin, whereas lutein was the only one of these detected in non-transgenic seeds. The accumulation of astaxanthin, which requires a β-carotene hydroxylase in addition to a β-carotene ketolase, in the transgenic seeds suggests that an endogenous soybean enzyme is able to work in combination with the ketolase transgene. Soybean seeds that accumulate ketocarotenoids could potentially be used in animal feed to reduce or eliminate the need for the costly addition of these compounds.

Published

2015

3. Transcriptional Response of Human Neurospheres to Helper-Dependent CAV-2 Vectors Involves the Modulation of DNA Damage Response, Microtubule and Centromere Gene Groups.

Author

Piersanti S, Burla R, Licursi V, Brito C, La Torre M, Alves PM, Simao D, Mottini C, Salinas S, Negri R, Tagliafico E, Kremer EJ, and Saggio I

Subjects

Animals, Brain metabolism, Cells, Cultured, Centromere metabolism, Dogs, Gene Expression Regulation, Gene Transfer Techniques, Genetic Therapy methods, Genetic Vectors physiology, HEK293 Cells, Humans, Microtubules metabolism, Neurons cytology, Spheroids, Cellular cytology, Adenoviruses, Canine physiology, Centromere genetics, DNA Damage genetics, Microtubules genetics, Neurons metabolism, Spheroids, Cellular metabolism, Transgenes physiology

Abstract

Brain gene transfer using viral vectors will likely become a therapeutic option for several disorders. Helper-dependent (HD) canine adenovirus type 2 vectors (CAV-2) are well suited for this goal. These vectors are poorly immunogenic, efficiently transduce neurons, are retrogradely transported to afferent structures in the brain and lead to long-term transgene expression. CAV-2 vectors are being exploited to unravel behavior, cognition, neural networks, axonal transport and therapy for orphan diseases. With the goal of better understanding and characterizing HD-CAV-2 for brain therapy, we analyzed the transcriptomic modulation induced by HD-CAV-2 in human differentiated neurospheres derived from midbrain progenitors. This 3D model system mimics several aspects of the dynamic nature of human brain. We found that differentiated neurospheres are readily transduced by HD-CAV-2 and that transduction generates two main transcriptional responses: a DNA damage response and alteration of centromeric and microtubule probes. Future investigations on the biochemistry of processes highlighted by probe modulations will help defining the implication of HD-CAV-2 and CAR receptor binding in enchaining these functional pathways. We suggest here that the modulation of DNA damage genes is related to viral DNA, while the alteration of centromeric and microtubule probes is possibly enchained by the interaction of the HD-CAV-2 fibre with CAR.

Published

2015

4. Chromatin function modifying elements in an industrial antibody production platform--comparison of UCOE, MAR, STAR and cHS4 elements.

Author

Saunders F, Sweeney B, Antoniou MN, Stephens P, and Cain K

Subjects

Animals, CHO Cells, Cricetulus, DNA Methylation, Epigenesis, Genetic genetics, Gene Silencing, Genetic Vectors, Humans, In Situ Hybridization, Fluorescence, Mice, Promoter Regions, Genetic genetics, Antibody Formation genetics, Chromatin genetics, Chromosomal Proteins, Non-Histone genetics, Immunoglobulin Heavy Chains genetics, Immunoglobulin Light Chains genetics, Regulatory Elements, Transcriptional genetics, Transgenes physiology

Abstract

The isolation of stably transfected cell lines suitable for the manufacture of biotherapeutic protein products can be an arduous process relying on the identification of a high expressing clone; this frequently involves transgene amplification and maintenance of the clones' expression over at least 60 generations. Maintenance of expression, or cell line stability, is highly dependent upon the nature of the genomic environment at the site of transgene integration, where epigenetic mechanisms lead to variable expression and silencing in the vast majority of cases. We have assessed four chromatin function modifying elements (A2UCOE, MAR X_S29, STAR40 and cHS4) for their ability to negate chromatin insertion site position effects and their ability to express and maintain monoclonal antibody expression. Each element was analysed by insertion into different positions within a vector, either flanking or between heavy chain (HC) and light chain (LC) antibody expression cassettes. Our results clearly show that the A2UCOE is the most beneficial element in this system, with stable cell pools and clones increasing antibody yields 6.5-fold and 6.75-fold respectively. Stability analysis demonstrated that the reduction in antibody expression, seen with cells transfected with the control vector over 120 generations, was mitigated in the clones containing A2UCOE-augmented transgenes. Analysis also showed that the A2UCOE reduced the amount of transgene promoter DNA methylation, which contributed to the maintenance of starting levels of expression.

Published

2015

5. Expression and functional characterization of Smyd1a in myofibril organization of skeletal muscles.

Author

Gao J, Li J, Li BJ, Yagil E, Zhang J, and Du SJ

Subjects

Animals, Animals, Genetically Modified genetics, Animals, Genetically Modified growth & development, Blotting, Western, Cell Differentiation, DNA-Binding Proteins metabolism, Embryo, Nonmammalian cytology, Gene Expression Regulation, Developmental, Gene Knockdown Techniques, In Situ Hybridization, Mice, Morphogenesis, Muscle Development, Muscle Proteins metabolism, Muscle, Skeletal cytology, Phenotype, RNA, Messenger genetics, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Transcription Factors metabolism, Transgenes physiology, Zebrafish growth & development, DNA-Binding Proteins genetics, Embryo, Nonmammalian metabolism, Histone-Lysine N-Methyltransferase physiology, Muscle Proteins genetics, Muscle, Skeletal metabolism, Myofibrils metabolism, Transcription Factors genetics, Zebrafish genetics, Zebrafish Proteins physiology

Abstract

Background: Smyd1, the founding member of the Smyd family including Smyd-1, 2, 3, 4 and 5, is a SET and MYND domain containing protein that plays a key role in myofibril assembly in skeletal and cardiac muscles. Bioinformatic analysis revealed that zebrafish genome contains two highly related smyd1 genes, smyd1a and smyd1b. Although Smyd1b function is well characterized in skeletal and cardiac muscles, the function of Smyd1a is, however, unknown., Methodology/principal Findings: To investigate the function of Smyd1a in muscle development, we isolated smyd1a from zebrafish, and characterized its expression and function during muscle development via gene knockdown and transgenic expression approaches. The results showed that smyd1a was strongly expressed in skeletal muscles of zebrafish embryos. Functional analysis revealed that knockdown of smyd1a alone had no significant effect on myofibril assembly in zebrafish skeletal muscles. However, knockdown of smyd1a and smyd1b together resulted in a complete disruption of myofibril organization in skeletal muscles, a phenotype stronger than knockdown of smyd1a or smyd1b alone. Moreover, ectopic expression of zebrafish smyd1a or mouse Smyd1 transgene could rescue the myofibril defects from the smyd1b knockdown in zebrafish embryos., Conclusion/significance: Collectively, these data indicate that Smyd1a and Smyd1b share similar biological activity in myofibril assembly in zebrafish embryos. However, Smyd1b appears to play a major role in this process.

Published

2014

6. TAILOR: transgene activation and inactivation using lox and rox in zebrafish.

Author

Park JT and Leach SD

Subjects

Animals, Escherichia coli Proteins genetics, Integrases genetics, Integrases metabolism, Microscopy, Confocal, Mifepristone, Recombinases genetics, Substrate Specificity, Transgenes physiology, Zebrafish metabolism, Escherichia coli Proteins metabolism, Gene Expression Regulation physiology, Gene Transfer Techniques, Recombinases metabolism, Transgenes genetics, Zebrafish genetics

Abstract

The ability to achieve precisely tailored activation and inactivation of gene expression represents a critical utility for vertebrate model organisms. In this regard, Cre and other site-specific DNA recombinases have come to play a central role in achieving temporally regulated and cell type-specific genetic manipulation. In zebrafish, both Cre and Flp recombinases have been applied for inducible activation, inactivation and inversion of inserted genomic elements. Here we describe the addition of Dre, a heterospecific Cre-related site-specific recombinase, to the zebrafish genomic toolbox. Combining Dre-based recombination in zebrafish with established Cre/lox technology, we have established an effective strategy for transgene activation and inactivation using lox and rox (TAILOR). Using stable transgenic lines expressing tamoxifen-inducible CreER(T2) and RU486-inducible DrePR fusions, we demonstrate that Cre and Dre retain non-overlapping specificities for their respective lox and rox target sites in larval zebrafish, and that their combinatorial and sequential activation can achieve precisely timed transgene activation and inactivation. In addition to TAILOR, the successful application of Dre/rox technology in zebrafish will facilitate a variety of additional downstream genetic applications, including sequential lineage labeling, complex genomic rearrangements and the precise temporal and spatial control of gene expression through the intersection of partially overlapping promoter activities.

Published

2013

7. Tightly regulated and homogeneous transgene expression in human adipose-derived mesenchymal stem cells by lentivirus with tet-off system.

Author

Moriyama H, Moriyama M, Sawaragi K, Okura H, Ichinose A, Matsuyama A, and Hayakawa T

Subjects

Blotting, Western, Cytomegalovirus genetics, DNA Primers genetics, Doxycycline pharmacology, Escherichia coli, Flow Cytometry, Gene Expression Regulation drug effects, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Humans, Lentivirus genetics, Mesenchymal Stem Cells physiology, Microscopy, Fluorescence, Peptide Elongation Factor 1 genetics, Promoter Regions, Genetic genetics, Tetracycline, Transgenes genetics, Transgenes physiology, Adipose Tissue cytology, Cell Differentiation physiology, Gene Transfer Techniques, Genetic Vectors genetics, Mesenchymal Stem Cells metabolism

Abstract

Genetic modification of human adipose tissue-derived multilineage progenitor cells (hADMPCs) is highly valuable for their exploitation in therapeutic applications. Here, we have developed a novel single tet-off lentiviral vector platform. This vector combines (1) a modified tetracycline (tet)-response element composite promoter, (2) a multi-cistronic strategy to express an improved version of the tet-controlled transactivator and the blasticidin resistance gene under the control of a ubiquitous promoter, and (3) acceptor sites for easy recombination cloning of the gene of interest. In the present study, we used the cytomegalovirus (CMV) or the elongation factor 1 α (EF-1α) promoter as the ubiquitous promoter, and EGFP was introduced as the gene of interest. hADMPCs transduced with a lentiviral vector carrying either the CMV promoter or the EF-1α promoter were effectively selected by blasticidin without affecting their stem cell properties, and EGFP expression was strictly regulated by doxycycline (Dox) treatment in these cells. However, the single tet-off lentiviral vector carrying the EF-1α promoter provided more homogenous expression of EGFP in hADMPCs. Intriguingly, differentiated cells from these Dox-responsive cell lines constitutively expressed EGFP only in the absence of Dox. This single tet-off lentiviral vector thus provides an important tool for applied research on hADMPCs.

Published

2013

8. Noninvasive assessment of gene transfer and expression by in vivo functional and morphologic imaging in a rabbit tumor model.

Author

Ravoori MK, Han L, Singh SP, Dixon K, Duggal J, Liu P, Uthamanthil R, Gupta S, Wright KC, and Kundra V

Subjects

Animals, Blotting, Western, Carcinoma, Adenosquamous genetics, Carcinoma, Adenosquamous therapy, Drug Administration Routes, Gamma Cameras, Genes, Reporter physiology, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Image Processing, Computer-Assisted, Injections, Intra-Arterial, Injections, Intralesional, Necrosis, Octreotide pharmacokinetics, Rabbits, Radiopharmaceuticals pharmacokinetics, Receptors, Somatostatin metabolism, Tissue Distribution, Tomography, Emission-Computed, Single-Photon, Transgenes physiology, Tumor Burden, Tumor Cells, Cultured, Adenoviridae genetics, Carcinoma, Adenosquamous pathology, Gene Transfer Techniques, Genetic Therapy, Genetic Vectors administration & dosage, Octreotide analogs & derivatives, Receptors, Somatostatin genetics

Abstract

Purpose: To evaluate the importance of morphology in quantifying expression after in vivo gene transfer and to compare gene expression after intra-arterial (IA) and intra-tumoral (IT) delivery of adenovirus expressing a SSTR2-based reporter gene in a large animal tumor model., Materials and Methods: Tumor directed IA or IT delivery of adenovirus containing a human somatostatin receptor type 2A (Ad-CMV-HA-SSTR2A) gene chimera or control adenovirus (Ad-CMV-GFP) was performed in VX2 tumors growing in both rabbit thighs. Three days later, ¹¹¹In-octreotide was administered intravenously after CT imaging using a clinical scanner. ¹¹¹In-octreotide uptake in tumors was evaluated the following day using a clinical gamma-camera. Gene expression was normalized to tumor weight with and without necrosis. This procedure was repeated on nine additional rabbits to investigate longitudinal gene expression both 5 days and 2 weeks after adenovirus delivery. CT images were used to evaluate tumor morphology and excised tissue samples were analyzed to determine ¹¹¹In-octreotide biodistribution ex vivo., Results: VX2 tumors infected with Ad-CMV-HA-SSTR2 had greater ¹¹¹In-octreotide uptake than with control virus (P<0.05). Intra-arterial and intra-tumoral routes resulted in similar levels of gene expression. Longitudinally, expression appeared to wane at 2 weeks versus 5 days after delivery. Areas of necrosis did not demonstrate significant uptake ex vivo. Morphology identified areas of necrosis on contrast enhanced CT and upon excluding necrosis, in vivo biodistribution analysis resulted in greater percent injected dose per gram (P<0.01) and corresponded better with ex vivo biodistribution(r = 0.72, P<0.01, Coefficient of the x-variable = .72) at 2 weeks than without excluding necrosis (P<0.01)., Conclusion: Tumor specificity and high transgene expression can be achieved in tumors via both tumor directed intra-arterial and intra-tumoral delivery in a large animal tumor model. Using clinical machines, morphologic imaging contributes to functional imaging for quantifying SSTR2-based reporter expression in vivo.

Published

2013

9. Biochemical and functional analysis of Drosophila-sciara chimeric sex-lethal proteins.

Author

Ruiz MF, Sarno F, Zorrilla S, Rivas G, and Sánchez L

Subjects

Animals, Animals, Genetically Modified, Blotting, Western, Drosophila classification, Drosophila genetics, Drosophila Proteins genetics, Electrophoretic Mobility Shift Assay, Female, Gene Expression Regulation, Developmental, Male, Protein Structure, Tertiary, RNA Precursors genetics, RNA, Messenger genetics, RNA-Binding Proteins genetics, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Dosage Compensation, Genetic, Drosophila metabolism, Drosophila Proteins metabolism, RNA Precursors metabolism, RNA Splicing genetics, RNA-Binding Proteins metabolism, Transgenes physiology

Abstract

Background: The Drosophila SXL protein controls sex determination and dosage compensation. It is a sex-specific factor controlling splicing of its own Sxl pre-mRNA (auto-regulation), tra pre-mRNA (sex determination) and msl-2 pre-mRNA plus translation of msl-2 mRNA (dosage compensation). Outside the drosophilids, the same SXL protein has been found in both sexes so that, in the non-drosophilids, SXL does not appear to play the key discriminating role in sex determination and dosage compensation that it plays in Drosophila. Comparison of SXL proteins revealed that its spatial organisation is conserved, with the RNA-binding domains being highly conserved, whereas the N- and C-terminal domains showing significant variation. This manuscript focuses on the evolution of the SXL protein itself and not on regulation of its expression., Methodology: Drosophila-Sciara chimeric SXL proteins were produced. Sciara SXL represents the non-sex-specific function of ancient SXL in the non-drosophilids from which presumably Drosophila SXL evolved. Two questions were addressed. Did the Drosophila SXL protein have affected their functions when their N- and C-terminal domains were replaced by the corresponding ones of Sciara? Did the Sciara SXL protein acquire Drosophila sex-specific functions when the Drosophila N- and C-terminal domains replaced those of Sciara? The chimeric SXL proteins were analysed in vitro to study their binding affinity and cooperative properties, and in vivo to analyse their effect on sex determination and dosage compensation by producing Drosophila flies that were transgenic for the chimeric SXL proteins., Conclusions: The sex-specific properties of extant Drosophila SXL protein depend on its global structure rather than on a specific domain. This implies that the modifications, mainly in the N- and C-terminal domains, that occurred in the SXL protein during its evolution within the drosophilid lineage represent co-evolutionary changes that determine the appropriate folding of SXL to carry out its sex-specific functions.

Published

2013

10. Interaction between NANOS2 and the CCR4-NOT deadenylation complex is essential for male germ cell development in mouse.

Author

Suzuki A, Saba R, Miyoshi K, Morita Y, and Saga Y

Subjects

Animals, Biomarkers, Tumor genetics, Biomarkers, Tumor metabolism, Blotting, Western, Embryo, Mammalian cytology, Gene Expression Profiling, HeLa Cells, Humans, Immunoprecipitation, Male, Mice, Mice, Knockout, Mice, Transgenic, Oligonucleotide Array Sequence Analysis, RNA, Messenger genetics, RNA-Binding Proteins, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Ribonucleases genetics, Testis embryology, Testis metabolism, Transcription Factors genetics, Transgenes physiology, Carrier Proteins physiology, Embryo, Mammalian metabolism, RNA, Messenger metabolism, Ribonucleases metabolism, Spermatozoa growth & development, Spermatozoa metabolism, Transcription Factors metabolism

Abstract

Nanos is one of the evolutionarily conserved proteins implicated in germ cell development and we have previously shown that it interacts with the CCR4-NOT deadenylation complex leading to the suppression of specific RNAs. However, the molecular mechanism and physiological significance of this interaction have remained elusive. In our present study, we identify CNOT1, a component of the CCR4-NOT deadenylation complex, as a direct factor mediating the interaction with NANOS2. We find that the first 10 amino acids (AAs) of NANOS2 are required for this binding. We further observe that a NANOS2 mutant lacking these first 10 AAs (NANOS2-ΔN10) fails to rescue defects in the Nanos2-null mouse. Our current data thus indicate that the interaction with the CCR4-NOT deadenylation complex is essential for NANOS2 function. In addition, we further demonstrate that NANOS2-ΔN10 can associate with specific mRNAs as well as wild-type NANOS2, suggesting the existence of other NANOS2-associated factor(s) that determine the specificity of RNA-binding independently of the CCR4-NOT deadenylation complex.

Published

2012

11. DNA barcoding simplifies environmental risk assessment of genetically modified crops in biodiverse regions.

Author

Nzeduru CV, Ronca S, and Wilkinson MJ

Subjects

Animals, Bacillus thuringiensis genetics, Crops, Agricultural classification, Insecta parasitology, Lepidoptera parasitology, Plants, Genetically Modified classification, Transgenes genetics, Transgenes physiology, Crops, Agricultural genetics, DNA Barcoding, Taxonomic methods, Plants, Genetically Modified genetics, Risk Assessment methods

Abstract

Transgenes encoding for insecticidal crystal (Cry) proteins from the soil-dwelling bacterium Bacillus Thuringiensis have been widely introduced into Genetically Modified (GM) crops to confer protection against insect pests. Concern that these transgenes may also harm beneficial or otherwise valued insects (so-called Non Target Organisms, NTOs) represents a major element of the Environmental Risk Assessments (ERAs) used by all countries prior to commercial release. Compiling a comprehensive list of potentially susceptible NTOs is therefore a necessary part of an ERA for any Cry toxin-containing GM crop. In partly-characterised and biodiverse countries, NTO identification is slowed by the need for taxonomic expertise and time to enable morphological identifications. This limitation represents a potentially serious barrier to timely adoption of GM technology in some developing countries. We consider Bt Cry1A cowpea (Vigna unguiculata) in Nigeria as an exemplar to demonstrate how COI barcoding can provide a simple and cost-effective means of addressing this problem. Over a period of eight weeks, we collected 163 insects from cowpea flowers across the agroecological and geographic range of the crop in Nigeria. These individuals included 32 Operational Taxonomic Units (OTUs) spanning four Orders and that could mostly be assigned to genus or species level. They included 12 Lepidopterans and two Coleopterans (both potentially sensitive to different groups of Cry proteins). Thus, barcode-assisted diagnoses were highly harmonised across groups (typically to genus or species level) and so were insensitive to expertise or knowledge gaps. Decisively, the entire study was completed within four months at a cost of less than 10,000 US$. The broader implications of the findings for food security and the capacity for safe adoption of GM technology are briefly explored.

Published

2012

12. Optimizing NTS-polyplex as a tool for gene transfer to cultured dopamine neurons.

Author

Hernandez-Baltazar D, Martinez-Fong D, and Trudeau LE

Subjects

Animals, Cell Survival, Cells, Cultured, Dopaminergic Neurons cytology, Immunoenzyme Techniques, Mice, Neurotensin metabolism, Parkinson Disease genetics, Parkinson Disease therapy, Receptors, Neurotensin metabolism, Transgenes physiology, Dopaminergic Neurons metabolism, Gene Transfer Techniques, Genetic Therapy, Genetic Vectors administration & dosage, Nanoparticles chemistry, Neurotensin chemistry, Plasmids genetics

Abstract

The study of signal transduction in dopamine (DA)-containing neurons as well as the development of new therapeutic approaches for Parkinson's disease requires the selective expression of transgenes in such neurons. Here we describe optimization of the use of the NTS-polyplex, a gene carrier system taking advantage of neurotensin receptor internalization, to transfect mouse DA neurons in primary culture. The plasmids DsRed2 (4.7 kbp) and VGLUT2-Venus (11 kbp) were used to compare the ability of this carrier system to transfect plasmids of different sizes. We examined the impact of age of the neurons (1, 3, 5 and 8 days after seeding), of culture media used during the transfection (Neurobasal with B27 vs. conditioned medium) and of three molar ratios of plasmid DNA to carrier. While the NTS-polyplex successfully transfected both plasmids in a control N1E-115 cell line, only the pDsRed2 plasmid could be transfected in primary cultured DA neurons. We achieved 20% transfection efficiency of pDsRed2 in DA neurons, with 80% cell viability. The transfection was demonstrated pharmacologically to be dependent on activation of neurotensin receptors and to be selective for DA neurons. The presence of conditioned medium for transfection was found to be required to insure cell viability. Highest transfection efficiency was achieved in the most mature neurons. In contrast, transfection with the VGLUT2-Venus plasmid produced cell damage, most likely due to the high molar ratios required, as evidenced by a 15% cell viability of DA neurons at the three molar ratios tested (1:36, 1:39 and 1:42). We conclude that, when used at molar ratios lower than 1:33, the NTS-polyplex can selectively transfect mature cultured DA neurons with only low levels of toxicity. Our results provide evidence that the NTS-polyplex has good potential for targeted gene delivery in cultured DA neurons, an in vitro system of great use for the screening of new therapeutic approaches for Parkinson's disease.

Published

2012

13. Impact of age at administration, lysosomal storage, and transgene regulatory elements on AAV2/8-mediated rat liver transduction.

Author

Cotugno G, Annunziata P, Barone MV, Karali M, Banfi S, and Auricchio A

Subjects

Age Factors, Animals, Blotting, Western, DNA, Recombinant genetics, Dependovirus, Enzyme-Linked Immunosorbent Assay, Genetic Vectors genetics, Glycosaminoglycans metabolism, Green Fluorescent Proteins metabolism, Liver Diseases genetics, Liver Diseases metabolism, Lysosomes metabolism, Oligonucleotides genetics, Rats, Reverse Transcriptase Polymerase Chain Reaction, Transgenes physiology, Genetic Therapy methods, Liver Diseases therapy, Regulatory Elements, Transcriptional genetics, Transduction, Genetic methods, Transgenes genetics

Abstract

Liver-directed gene transfer is being investigated for the treatment of systemic or liver-specific diseases. Recombinant vectors based on adeno-associated virus serotype 8 (AAV2/8) efficiently transduce liver cells allowing long term transgene expression after a single administration in animal models and in patients.We evaluated the impact on AAV2/8-mediated rat liver transduction of the following variables: i) age at vector administration, ii) presence of lysosomal storage in liver cells, and iii) regulatory elements included in the transgene expression cassette. We found that systemic administration of AAV2/8 to newborn rats results in vector genome dilution and reduced transduction efficacy when compared to adult injected animals, presumably due to hepatocyte proliferation. Accumulation of glycosaminoglycans in lysosomes does not impact on levels and distribution of AAV2/8-mediated liver transduction. Transgene expression occurs in hepatocytes but not in Kupffer or liver endothelial cells when the liver-specific thyroxine-binding-globulin promoter is used. However, extra-hepatic transduction is observed in the spleen and kidney of animals injected at birth. The use of target sequences for the hematopoietic-specific microRNA miR142-3p does not improve liver transduction efficacy neither reduce immune responses to the lysosomal enzyme arylsulfatase B. The inclusion of a variant of the Woodchuck hepatitis virus post-transcriptional regulatory element (WPRE-m) decreases AAV2/8-mediated liver transduction levels.As AAV2/8-mediated liver gene transfer is entering in the clinical arena, these data will provide relevant information to the design of efficient AAV2/8-based therapeutic strategies.

Published

2012

14. A rapid Flp-In system for expression of secreted H5N1 influenza hemagglutinin vaccine immunogen in mammalian cells.

Author

Lu H, Khurana S, Verma N, Manischewitz J, King L, Beigel JH, and Golding H

Subjects

Animals, Cell Line, Gene Expression physiology, Genetic Vectors, Hemagglutinin Glycoproteins, Influenza Virus metabolism, Humans, Influenza A Virus, H5N1 Subtype immunology, Influenza A Virus, H5N1 Subtype metabolism, Influenza Vaccines chemical synthesis, Influenza Vaccines immunology, Mammals, Neutralization Tests, Rabbits, Transfection, Transgenes genetics, Transgenes physiology, Cloning, Molecular methods, Hemagglutinin Glycoproteins, Influenza Virus immunology, Influenza Vaccines genetics

Abstract

Background: Continuing transmissions of highly pathogenic H5N1 viruses in poultry and humans underscores the need for a rapid response to potential pandemic in the form of vaccine. Recombinant technologies for production of immunogenic hemagglutinin (HA) could provide an advantage over the traditional inactivated vaccine manufacturing process. Generation of stably transfected mammalian cells secreting properly folded HA proteins is important for scalable controlled manufacturing., Methodology/principal Findings: We have developed a Flp-In based 293 stable cell lines through targeted site-specific recombination for expression of secreted hemagglutinin (HA) proteins and evaluated their immunogenicity. H5N1 globular domain HA1(1-330) and HA0(1-500) proteins were purified from the supernatants of 293 Flp-In stable cell lines. Both proteins were properly folded as confirmed by binding to H5N1-neutralizing conformation-dependent human monoclonal antibodies. The HA0 (with unmodified cleavage site) was monomeric, while the HA1 contained oligomeric forms. Upon rabbit immunization, both HA proteins elicited neutralizing antibodies against the homologous virus (A/Vietnam/1203/2004, clade 1) as well as cross-neutralizing antibodies against heterologous H5N1 clade 2 strains, including A/Indonesia/5/2005. These results exceeded the human antibody responses against the inactivated sub-virion H5N1 vaccine., Conclusions/significance: Our data suggest that the 293 Flp-In system could serve as a platform for rapid expression of HA immunogens in mammalian cells from emerging influenza strains.

Published

2011

15. IL-2 suppression of IL-12p70 by a recombinant HSV-1 expressing IL-2 induces T-cell auto-reactivity and CNS demyelination.

Author

Zandian M, Mott KR, Allen SJ, Chen S, Arditi M, and Ghiasi H

Subjects

Animals, Autoimmunity genetics, Demyelinating Autoimmune Diseases, CNS chemically induced, Demyelinating Autoimmune Diseases, CNS pathology, Down-Regulation drug effects, Female, Gene Expression physiology, Genetic Vectors genetics, Genetic Vectors metabolism, Genetic Vectors pharmacology, Herpesvirus 1, Human metabolism, Interleukin-12 metabolism, Interleukin-12 physiology, Interleukin-2 metabolism, Lymphocyte Activation drug effects, Lymphocyte Activation genetics, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Mice, Transgenic, Recombinant Proteins genetics, Recombinant Proteins metabolism, Recombinant Proteins pharmacology, T-Lymphocytes metabolism, Transgenes physiology, Autoimmunity drug effects, Demyelinating Autoimmune Diseases, CNS genetics, Herpesvirus 1, Human genetics, Interleukin-12 antagonists & inhibitors, Interleukin-2 genetics, Interleukin-2 pharmacology, T-Lymphocytes immunology

Abstract

To evaluate the role of cellular infiltrates in CNS demyelination in immunocompetent mice, we have used a model of multiple sclerosis (MS) in which different strains of mice are infected with a recombinant HSV-1 expressing IL-2. Histologic examination of the mice infected with HSV-IL-2 demonstrates that natural killer cells, dendritic cells, B cells, and CD25 (IL-2rα) do not play any role in the HSV-IL-2-induced demyelination. T cell depletion, T cell knockout and T cell adoptive transfer experiments suggest that both CD8(+) and CD4(+) T cells contribute to HSV-IL-2-induced CNS demyelination with CD8(+) T cells being the primary inducers. In the adoptive transfer studies, all of the transferred T cells irrespective of their CD25 status at the time of transfer were positive for expression of FoxP3 and depletion of FoxP3 blocked CNS demyelination by HSV-IL-2. The expression levels of IL-12p35 relative to IL-12p40 differed in BM-derived macrophages infected with HSV-IL-2 from those infected with wild-type HSV-1. HSV-IL-2-induced demyelination was blocked by injecting HSV-IL-2-infected mice with IL-12p70 DNA. This study demonstrates that suppression of the IL-12p70 function of macrophages by IL-2 causes T cells to become auto-aggressive. Interruption of this immunoregulatory axis results in demyelination of the optic nerve, the spinal cord and the brain by autoreactive T cells in the HSV-IL-2 mouse model of MS.

Published

2011

16. A modular cloning system for standardized assembly of multigene constructs.

Author

Weber E, Engler C, Gruetzner R, Werner S, and Marillonnet S

Subjects

Agrobacterium tumefaciens genetics, Algorithms, Base Sequence, Green Fluorescent Proteins genetics, Models, Biological, Molecular Sequence Data, Plant Tumors genetics, Plant Tumors microbiology, Research Design, Nicotiana genetics, Nicotiana microbiology, Transgenes physiology, Validation Studies as Topic, Cloning, Molecular methods, Genetic Engineering methods, Genetic Engineering standards, Recombinant Fusion Proteins genetics

Abstract

The field of synthetic biology promises to revolutionize biotechnology through the design of organisms with novel phenotypes useful for medicine, agriculture and industry. However, a limiting factor is the ability of current methods to assemble complex DNA molecules encoding multiple genetic elements in various predefined arrangements. We present here a hierarchical modular cloning system that allows the creation at will and with high efficiency of any eukaryotic multigene construct, starting from libraries of defined and validated basic modules containing regulatory and coding sequences. This system is based on the ability of type IIS restriction enzymes to assemble multiple DNA fragments in a defined linear order. We constructed a 33 kb DNA molecule containing 11 transcription units made from 44 individual basic modules in only three successive cloning steps. This modular cloning (MoClo) system can be readily automated and will be extremely useful for applications such as gene stacking and metabolic engineering.

Published

2011

17. Study of muscle cell dedifferentiation after skeletal muscle injury of mice with a Cre-Lox system.

Author

Mu X, Peng H, Pan H, Huard J, and Li Y

Subjects

Animals, Cell Dedifferentiation genetics, Cell Tracking methods, Integrases metabolism, Male, Mice, Mice, Inbred C57BL, Mice, SCID, Mice, Transgenic, Muscle Fibers, Skeletal metabolism, Muscle Fibers, Skeletal pathology, Muscle, Skeletal metabolism, Muscle, Skeletal pathology, Organ Specificity genetics, Regeneration physiology, beta-Galactosidase genetics, beta-Galactosidase metabolism, Cell Dedifferentiation physiology, Integrases genetics, Muscle Fibers, Skeletal physiology, Muscle, Skeletal injuries, Transgenes physiology

Abstract

Background: Dedifferentiation of muscle cells in the tissue of mammals has yet to be observed. One of the challenges facing the study of skeletal muscle cell dedifferentiation is the availability of a reliable model that can confidentially distinguish differentiated cell populations of myotubes and non-fused mononuclear cells, including stem cells that can coexist within the population of cells being studied., Methodology/principal Findings: In the current study, we created a Cre/Lox-β-galactosidase system, which can specifically tag differentiated multinuclear myotubes and myotube-generated mononuclear cells based on the activation of the marker gene, β-galactosidase. By using this system in an adult mouse model, we found that β-galactosidase positive mononuclear cells were generated from β-galactosidase positive multinuclear myofibers upon muscle injury. We also demonstrated that these mononuclear cells can develop into a variety of different muscle cell lineages, i.e., myoblasts, satellite cells, and muscle derived stem cells., Conclusions/significance: These novel findings demonstrated, for the first time, that cellular dedifferentiation of skeletal muscle cells actually occurs in mammalian skeletal muscle following traumatic injury in vivo.

Published

2011

18. Nestin-GFP transgene reveals neural precursor cells in adult skeletal muscle.

Author

Birbrair A, Wang ZM, Messi ML, Enikolopov GN, and Delbono O

Subjects

Aging metabolism, Aging physiology, Animals, Cell Differentiation genetics, Cell Differentiation physiology, Cell Tracking methods, Cells, Cultured, Female, Flow Cytometry, Green Fluorescent Proteins metabolism, Green Fluorescent Proteins physiology, Intermediate Filament Proteins metabolism, Intermediate Filament Proteins physiology, Male, Mice, Mice, Inbred C57BL, Mice, Transgenic, Muscle, Skeletal metabolism, Nerve Tissue Proteins metabolism, Nerve Tissue Proteins physiology, Nestin, Neural Stem Cells physiology, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Recombinant Fusion Proteins physiology, Green Fluorescent Proteins genetics, Intermediate Filament Proteins genetics, Muscle, Skeletal cytology, Nerve Tissue Proteins genetics, Neural Stem Cells cytology, Neural Stem Cells metabolism, Transgenes physiology

Abstract

Background: Therapy for neural lesions or degenerative diseases relies mainly on finding transplantable active precursor cells. Identifying them in peripheral tissues accessible for biopsy, outside the central nervous system, would circumvent the serious immunological and ethical concerns impeding cell therapy., Methodology/principal Findings: In this study, we isolated neural progenitor cells in cultured adult skeletal muscle from transgenic mice in which nestin regulatory elements control GFP expression. These cells also expressed the early neural marker Tuj1 and light and heavy neurofilament but not S100β, indicating that they express typical neural but not Schwann cell markers. GFP+/Tuj1+ cells were also negative for the endothelial and pericyte markers CD31 and α-smooth muscle actin, respectively. We established their a) functional response to glutamate in patch-clamp recordings; b) interstitial mesenchymal origin; c) replicative capacity; and d) the environment necessary for their survival after fluorescence-activated cell sorting., Conclusions/significance: We propose that the decline in nestin-GFP expression in muscle progenitor cells and its persistence in neural precursor cells in muscle cultures provide an invaluable tool for isolating a population of predifferentiated neural cells with therapeutic potential.

Published

2011

19. Forced notch signaling inhibits commissural axon outgrowth in the developing chick central nerve system.

Author

Shi M, Liu Z, Lv Y, Zheng M, Du F, Zhao G, Huang Y, Chen J, Han H, and Ding Y

Subjects

Animals, Chick Embryo, Neurons, Receptors, Notch genetics, Transgenes physiology, Axons, Central Nervous System growth & development, Neurites, Receptors, Notch metabolism, Signal Transduction

Abstract

Background: A collection of in vitro evidence has demonstrated that Notch signaling plays a key role in the growth of neurites in differentiated neurons. However, the effects of Notch signaling on axon outgrowth in an in vivo condition remain largely unknown., Methodology/principal Findings: In this study, the neural tubes of HH10-11 chick embryos were in ovo electroporated with various Notch transgenes of activating or inhibiting Notch signaling, and then their effects on commissural axon outgrowth across the floor plate midline in the chick developing central nerve system were investigated. Our results showed that forced expression of Notch intracellular domain, constitutively active form of RBPJ, or full-length Hes1 in the rostral hindbrain, diencephalon and spinal cord at stage HH10-11 significantly inhibited commissural axon outgrowth. On the other hand, inhibition of Notch signaling by ectopically expressing a dominant-negative form of RBPJ promoted commissural axonal growth along the circumferential axis. Further results revealed that these Notch signaling-mediated axon outgrowth defects may be not due to the alteration of axon guidance since commissural axon marker TAG1 was present in the axons in floor plate midline, and also not result from the changes in cell fate determination of commissural neurons since the expression of postmitotic neuron marker Tuj1 and specific commissural markers TAG1 and Pax7 was unchanged., Conclusions/significance: We first used an in vivo system to provide evidence that forced Notch signaling negatively regulates commissural axon outgrowth.

Published

2011

20. Trade-off between toxicity and signal detection orchestrated by frequency- and density-dependent genes.

Author

Arthaud L, Rokia-Mille SB, Raad H, Dombrovsky A, Prevost N, Capovilla M, and Robichon A

Subjects

Aldehyde Dehydrogenase genetics, Aldehyde Dehydrogenase metabolism, Animals, Animals, Genetically Modified, Behavior, Animal, Cells, Cultured, Cyclic GMP-Dependent Protein Kinases genetics, Cyclic GMP-Dependent Protein Kinases metabolism, Environment, Genotype, Drosophila melanogaster genetics, Genes, Insect, Transgenes physiology

Abstract

Behaviors in insects are partly highly efficient Bayesian processes that fulfill exploratory tasks ending with the colonization of new ecological niches. The foraging (for) gene in Drosophila encodes a cGMP-dependent protein kinase (PKG). It has been extensively described as a frequency-dependent gene and its transcripts are differentially expressed between individuals, reflecting the population density context. Some for transcripts, when expressed in a population at high density for many generations, concomitantly trigger strong dispersive behavior associated with foraging activity. Moreover, genotype-by-environment interaction (GEI) analysis has highlighted a dormant role of for in energetic metabolism in a food deprivation context. In our current report, we show that alleles of for encoding different cGMP-dependent kinase isoforms influence the oxidation of aldehyde groups of aromatic molecules emitted by plants via Aldh-III and a phosphorylatable adaptor. The enhanced efficiency of oxidation of aldehyde odorants into carboxyl groups by the action of for lessens their action and toxicity, which should facilitate exploration and guidance in a complex odor environment. Our present data provide evidence that optimal foraging performance requires the fast metabolism of volatile compounds emitted by plants to avoid neurosensory saturation and that the frequency-dependent genes that trigger dispersion influence these processes.

Published

2011

21. Non-integrative lentivirus drives high-frequency cre-mediated cassette exchange in human cells.

Author

Torres R, García A, Payá M, and Ramirez JC

Subjects

Blotting, Western, Cells, Cultured, Flow Cytometry, Humans, Kidney cytology, Kidney metabolism, Promoter Regions, Genetic, Transgenes physiology, Integrases metabolism, Lentivirus genetics, Plasmids genetics, Recombination, Genetic

Abstract

Recombinase mediated cassette exchange (RMCE) is a two-step process leading to genetic modification in a specific genomic target sequence. The process involves insertion of a docking genetic cassette in the genome followed by DNA transfer of a second cassette flanked by compatible recombination signals and expression of the recombinase. Major technical drawbacks are cell viability upon transfection, toxicity of the enzyme, and the ability to target efficiently cell types of different origins. To overcome such drawbacks, we developed an RMCE assay that uses an integrase-deficient lentivirus (IDLV) vector in the second step combined with promoterless trapping of double selectable markers. Additionally, recombinase expression is self-limiting as a result of the exchangeable reaction, thus avoiding toxicity. Our approach provides proof-of-principle of a simple and novel strategy with expected wide applicability modelled on a human cell line with randomly integrated copies of a genetic landing pad. This strategy does not present foreseeable limitations for application to other cell systems modified by homologous recombination. Safety, efficiency, and simplicity are the major advantages of our system, which can be applied in low-to-medium throughput strategies for screening of cDNAs, non-coding RNAs during functional genomic studies, and drug screening.

Published

2011

22. A transgenic mouse line expressing cre recombinase in undifferentiated postmitotic mouse retinal bipolar cell precursors.

Author

Nickerson PE, Ronellenfitch K, McEwan J, Kim H, McInnes RR, and Chow RL

Subjects

Animals, Cells, Cultured, Female, Humans, Integrases, Male, Mice, Mice, Inbred C3H, Mice, Inbred C57BL, Mice, Transgenic, Neurons cytology, Neurons metabolism, Retina cytology, Retinal Bipolar Cells cytology, Stem Cells cytology, Cell Differentiation, Homeodomain Proteins physiology, Mitosis physiology, Retina metabolism, Retinal Bipolar Cells metabolism, Stem Cells metabolism, Transcription Factors physiology, Transgenes physiology

Abstract

Approaches for manipulating cell type-specific gene expression during development depend on the identification of novel genetic tools. Here, we report the generation of a transgenic mouse line that utilizes Vsx2 upstream sequences to direct Cre recombinase to developing retinal bipolar cells. In contrast to the endogenous Vsx2 expression pattern, transgene expression was not detected in proliferating retinal progenitor cells and was restricted to post-mitotic bipolar cells. Cre immunolabeling was detected in rod bipolar cells and a subset of ON and OFF cone bipolar cells. Expression was first observed at postnatal day 3 and was detectable between 24 hours and 36 hours after the last S-phase of the cell cycle. The appearance of Cre-immunolabeled cells preceded the expression of bipolar cell type-specific markers such as PKCα and Cabp5 suggesting that transgene expression is initiated prior to terminal differentiation. In the presence of a constitutive conditional reporter transgene, reporter fluorescence was detected in Cre-expressing bipolar cells in the mature retina as expected, but was also observed in Cre-negative Type 2 bipolar cells and occasionally in Cre-negative photoreceptor cells. Together these findings reveal a new transgenic tool for directing gene expression to post-mitotic retinal precursors that are mostly committed to a bipolar cell fate.

Published

2011

23. Targeting the NG2/CSPG4 proteoglycan retards tumour growth and angiogenesis in preclinical models of GBM and melanoma.

Author

Wang J, Svendsen A, Kmiecik J, Immervoll H, Skaftnesmo KO, Planagumà J, Reed RK, Bjerkvig R, Miletic H, Enger PØ, Rygh CB, and Chekenya M

Subjects

Animals, Antigens genetics, Brain Neoplasms metabolism, Brain Neoplasms pathology, Cell Adhesion, Cell Movement, Glioblastoma metabolism, Glioblastoma pathology, Humans, Immunoenzyme Techniques, Magnetic Resonance Imaging, Melanoma metabolism, Melanoma pathology, Mice, Mice, Inbred NOD, Mice, SCID, Proteoglycans genetics, RNA, Small Interfering genetics, Rats, Rats, Nude, Transgenes physiology, Antigens metabolism, Brain Neoplasms prevention & control, Cell Proliferation, Disease Models, Animal, Glioblastoma prevention & control, Melanoma prevention & control, Neovascularization, Pathologic, Proteoglycans antagonists & inhibitors, Proteoglycans metabolism

Abstract

Aberrant expression of the progenitor marker Neuron-glia 2 (NG2/CSPG4) or melanoma proteoglycan on cancer cells and angiogenic vasculature is associated with an aggressive disease course in several malignancies including glioblastoma multiforme (GBM) and melanoma. Thus, we investigated the mechanism of NG2 mediated malignant progression and its potential as a therapeutic target in clinically relevant GBM and melanoma animal models. Xenografting NG2 overexpressing GBM cell lines resulted in increased growth rate, angiogenesis and vascular permeability compared to control, NG2 negative tumours. The effect of abrogating NG2 function was investigated after intracerebral delivery of lentivirally encoded shRNAs targeting NG2 in patient GBM xenografts as well as in established subcutaneous A375 melanoma tumours. NG2 knockdown reduced melanoma proliferation and increased apoptosis and necrosis. Targeting NG2 in two heterogeneous GBM xenografts significantly reduced tumour growth and oedema levels, angiogenesis and normalised vascular function. Vascular normalisation resulted in increased tumour invasion and decreased apoptosis and necrosis. We conclude that NG2 promotes tumour progression by multiple mechanisms and represents an amenable target for cancer molecular therapy.

Published

2011

24. Nestin-Cre mice are affected by hypopituitarism, which is not due to significant activity of the transgene in the pituitary gland.

Author

Galichet C, Lovell-Badge R, and Rizzoti K

Subjects

Adrenocorticotropic Hormone metabolism, Animals, Central Nervous System metabolism, Growth Hormone metabolism, Hypopituitarism genetics, Luteinizing Hormone metabolism, Mice, Mice, Transgenic, Nestin, Prolactin metabolism, Promoter Regions, Genetic genetics, Radioimmunoassay, Rats, Thyrotropin metabolism, Transgenes genetics, Hypopituitarism metabolism, Integrases genetics, Integrases metabolism, Intermediate Filament Proteins genetics, Nerve Tissue Proteins genetics, Pituitary Gland metabolism, Transgenes physiology

Abstract

Nestin-Cre mice express Cre recombinase under control of the rat nestin promoter and central nervous system (CNS) enhancer. While endogenous Nestin is expressed in some other tissues including the pituitary gland, Nestin-Cre mice induce recombination predominantly in the CNS. For this reason, they have been widely used to explore gene function or cell fate in the latter. Pituitary hormonal deficiencies, or hypopituitarism, are associated with a wide range of symptoms and with a significant morbidity. These can have a neural and/or a pituitary origin as the gland's secretions are controlled by the hypothalamus. We report here that Nestin-Cre mice themselves are affected by mild hypopituitarism. Hence, physiological consequences are expected, especially in combination with defects resulting from Cre mediated deletion of any gene under investigation. To further investigate the origin of this phenotype, we re-examined the activity of the transgene. We compared it with expression of Nestin itself in the context of the hypothalamo-pituitary axis, especially in the light of a recent report showing pituitary Nestin-Cre activity, which contrasts with previous data. Our results disagree with those of this recent study and do not support the claim that Nestin positive cells are present in the pituitary anlagen, the Rathke's pouch (RP). Moreover we did not observe any significant activity in the post-natal pituitary, in agreement with the initial report.

Published

2010

25. Expanding the repertoire of Modified Vaccinia Ankara-based vaccine vectors via genetic complementation strategies.

Author

Garber DA, O'Mara LA, Zhao J, Gangadhara S, An I, and Feinberg MB

Subjects

Animals, Blotting, Southern, CD4-Positive T-Lymphocytes immunology, CD8-Positive T-Lymphocytes immunology, Chick Embryo cytology, Chick Embryo metabolism, Chickens, DNA Replication, Female, Fibroblasts cytology, Flow Cytometry, Immunization, Secondary, Macaca mulatta, Male, Mice, Mice, Inbred C57BL, Neutralization Tests, Transgenes physiology, Uracil-DNA Glycosidase genetics, Uracil-DNA Glycosidase immunology, Vaccinia virus genetics, Viral Vaccines genetics, Virus Replication, gag Gene Products, Human Immunodeficiency Virus immunology, gag Gene Products, Human Immunodeficiency Virus metabolism, Antibodies, Viral immunology, Genetic Complementation Test, Genetic Vectors immunology, HIV Antibodies immunology, Vaccinia virus immunology, Viral Vaccines immunology

Abstract

Background: Modified Vaccinia virus Ankara (MVA) is a safe, highly attenuated orthopoxvirus that is being developed as a recombinant vaccine vector for immunization against a number of infectious diseases and cancers. However, the expression by MVA vectors of large numbers of poxvirus antigens, which display immunodominance over vectored antigens-of-interest for the priming of T cell responses, and the induction of vector-neutralizing antibodies, which curtail the efficacy of subsequent booster immunizations, remain as significant impediments to the overall utility of such vaccines. Thus, genetic approaches that enable the derivation of MVA vectors that are antigenically less complex may allow for rational improvement of MVA-based vaccines., Principal Findings: We have developed a genetic complementation system that enables the deletion of essential viral genes from the MVA genome, thereby allowing us to generate MVA vaccine vectors that are antigenically less complex. Using this system, we deleted the essential uracil-DNA-glycosylase (udg) gene from MVA and propagated this otherwise replication-defective variant on a complementing cell line that constitutively expresses the poxvirus udg gene and that was derived from a newly identified continuous cell line that is permissive for growth of wild type MVA. The resulting virus, MVADeltaudg, does not replicate its DNA genome or express late viral gene products during infection of non-complementing cells in culture. As proof-of-concept for immunological 'focusing', we demonstrate that immunization of mice with MVADeltaudg elicits CD8+ T cell responses that are directed against a restricted repertoire of vector antigens, as compared to immunization with parental MVA. Immunization of rhesus macaques with MVADeltaudg-gag, a udg(-) recombinant virus that expresses an HIV subtype-B consensus gag transgene, elicited significantly higher frequencies of Gag-specific CD8 and CD4 T cells following both primary (2-4-fold) and booster (2-fold) immunizations as compared to the udg(+) control virus MVA-gag, as determined by intracellular cytokine assay. In contrast, levels of HIV Gag-specific antibodies were elicited similarly in macaques following immunization with MVADeltaudg-gag and MVA-gag. Furthermore, both udg(-) and udg(+) MVA vectors induced comparatively similar titers of MVA-specific neutralizing antibody responses following immunization of mice (over a 4-log range: 10(4)-10(8) PFU) and rhesus macaques. These results suggest that the generation of MVA-specific neutralizing antibody responses are largely driven by input MVA antigens, rather than those that are synthesized de novo during infection, and that the processes governing the generation of antiviral antibody responses are more readily saturated by viral antigen than are those that elicit CD8+ T cell responses., Significance: Our identification of a spontaneously-immortalized (but not transformed) chicken embryo fibroblast cell line (DF-1) that is fully permissive for MVA growth and that can be engineered to stably express MVA genes provides the basis for a genetic system for MVA. DF-1 cells (and derivatives thereof) constitute viable alternatives, for the manufacture of MVA-based vaccines, to primary CEFs -- the conventional cell substrate for MVA vaccines that is not amenable to genetic complementation strategies due to these cells' finite lifespan in culture. The establishment of a genetic system for MVA, as illustrated here to allow udg deletion, enables the generation of novel replication-defective MVA mutants and expands the repertoire of genetic viral variants that can now be explored as improved vaccine vectors.

Published

2009