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1. A novel system for stable, high-level expression from the T7 promoter

Author

Kesik-Brodacka Malgorzata, Romanik Agnieszka, Mikiewicz-Sygula Diana, Plucienniczak Grazyna, and Plucienniczak Andrzej

Subjects
T7 expression, Expression cassette, Stable expression from T7 promoter, High expression from T7 promoter, Microbiology, QR1-502
Abstract

Abstract Background The most widespread, efficient prokaryotic protein-producing system is one where the T7 phage polymerase recognizes the T7 phage promoter (T7 p/p system). Unfortunately, in this system, target protein expression gradually declines and is often undetectable following 3 to 5 subcultures. Although a number of studies have attempted to stabilize the expression levels of the T7 p/p system, none has resolved the problem adequately and thus precludes the use of this system for the production of recombinant proteins on a large scale. Results We created an expression cassette enabling stable, high-level expression in the T7p/p system. The cassette was tested with two different vector backbones and two target proteins. In all experiments, the expression system using the new cassette exhibited high and stable protein expression levels when compared to the traditional system. Conclusions Herein, we describe a universal expression cassette that enables high-level, stable target protein expression in T7 RNA polymerase-based expression systems. We also present the successful use of this cassette as a novel expression platform and demonstrate its ability to overcome the main deficiency of the T7 p/p system. Thus, we provide a method for using the T7 p/p system on an industrial scale.

Published
2012
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2. Expression of yeast deubiquitination enzyme UBP1 analogues in E. coli

Author

Chojnacka Luiza, Mikiewicz-Sygula Diana, Plucienniczak Grazyna, Mazurkiewicz-Pisarek Anna, Wojtowicz Anna, Lukasiewicz Natalia, and Plucienniczak Andrzej

Subjects
Microbiology, QR1-502
Abstract

Abstract Background It has been shown that proteins fused to ubiquitin undergo greater expression in E. coli and are easier to purify and renaturate than nonhybrid foreign proteins. However, there is no commercial source of large quantities of specific deubiquitinating proteases. This is the reason why hybrid proteins containing ubiquitin at their N-end cannot be used in large scale biotechnological processes. Results and Conclusion We have described the synthesis of the yeast deubiquination enzyme UBP1 muteins in E. coli. We have shown that an efficient overproduction of the enzyme in E. coli may be achieved after the introduction of several changes in the nucleotide sequence encoding UBP1. One of the conditions of an effective synthesis of the UBP1 muteins is the removal of the 5'-end sequence encoding the transmembrane region of the enzyme. The obtained variants of the enzyme may be successfully used for processing large amounts of hybrid proteins comprising ubiquitin or tagged ubiquitin at their N-ends.

Published
2005
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12. Biotechnological Approaches to Making Vaccine in Plants

Author

Kapusta, J., Modelska, A., Figlerowicz, M., Podkowinski, J., Pniewski, T., Lisowa, O., Berbezy, P., Helias, D., Biesiadka, J., Femiak, I., Letellier, M., Yusibov, V., Koprowski, H., Plucienniczak, A., Legocki, A. B., Summerfield, R. J., editor, Altman, Arie, editor, Ziv, Meira, editor, and Izhar, Shamay, editor

Published
1999
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14. Factors affecting the effectiveness of the manager’s work

Author

Marian Kopczewski and Marcin Plucienniczak

Subjects
negotiations, competences, Process management, Work (electrical), ComputingMilieux_THECOMPUTINGPROFESSION, lcsh:Military Science, efficiency, lcsh:U, Psychology, company, manager
Abstract

The requirements placed on modern entrepreneurs – managers – leaders of organisations – are extremely high, and their fulfilment does not guarantee exclusively successes. They guide people who need to be taught and prepared above all: to work in their occupied positions, to live in society, as well as to bring people closer together and to focus on each other. Employees can be different, strong and weak, proud and humble, curious about the world and despite their different ages, apathetic. All of them, due to the work of managers and their competences, knowledge and skills become good employees at different levels of the organisation and then managers. However, the basis of the manager’s work is also, or maybe above all, communication skills, which are based on negotiations.

Published
2019

15. Novel Expression Vectors Based on the pIGDM1 Plasmid

Author

Agnieszka Skowronek, Andrzej Plucienniczak, Diana Mikiewicz, Anna Bierczyńska-Krzysik, and Grzegorz Węgrzyn

Subjects
0106 biological sciences, Genetic Vectors, Cloning vector, Heterologous, Bioengineering, Computational biology, Biology, Molecular cloning, medicine.disease_cause, 01 natural sciences, Applied Microbiology and Biotechnology, Biochemistry, 03 medical and health sciences, Plasmid, 010608 biotechnology, Escherichia coli, medicine, Cloning, Molecular, Promoter Regions, Genetic, Molecular Biology, Gene, 030304 developmental biology, 0303 health sciences, Expression vector, Drug Resistance, Microbial, Kanamycin, Gene Expression Regulation, Bacterial, Recombinant Proteins, Klebsiella pneumoniae, Plasmids, Biotechnology, medicine.drug
Abstract

Escherichia coli is one of the most widely used hosts for the production of heterologous proteins. Within this host, the choice of cloning vector constitutes a key factor for a satisfactory amplified expression of a target gene. We aimed to develop novel, unpatented expression vectors that enable the stable maintenance and efficient overproduction of proteins in E. coli. A series of expression vectors based on the ColE1-like pIGDM1 plasmid were constructed. The vectors named pIGDMCT7RS, pIGDM4RS and pIGDMKAN carry various antibiotic resistance genes: chloramphenicol, ampicillin or kanamycin, respectively. Two derivatives contain the inducible T7 promoter while the third one bears the constitutive pms promoter from a clinical strain of Klebsiella pneumoniae. The pIGDM1-derivatives are compatible with other ColE1-like plasmids commonly used in molecular cloning. The pIGDMCT7RS and pIGDM4RS vectors contain genes encoding AGA and AGG tRNAs, which supplement the shortage of these tRNAs, increasing the efficiency of synthesis of heterologous proteins. In conclusion, pIGDMCT7RS, pIGDM4RS and pIGDMKAN vectors, with significantly improved features, including compatibility with vast majority of other plasmids, were designed and constructed. They enable a high-level expression of a desired recombinant gene and therefore constitute a potential, valuable tool for pharmaceutical companies and research laboratories for their own research or for the production of recombinant biopharmaceuticals.

Published
2019

17. Fingerprinting of Bacterial Genomes by Amplification of DNA Fragments Surrounding Rare Restriction Sites

Author

Aleksander Masny and Andrzej Plucienniczak

Subjects
Biology (General), QH301-705.5
Abstract

A method for generating limited representations of total bacterial DNA, without prior knowledge of the DNA sequence, has been developed. This method consists of three steps: digestion with two restriction enzymes, ligation of two oligonucleotide adapters corresponding to the restriction sites, and selective PCR amplification of the ligation products. The method relies on the use of two restriction enzymes with considerable differences in cleavage frequency of the investigated DNA and the ligation of two different oligonucleotides, each corresponding to one of the two cohesive ends of DNA fragments. Three subsets of DNA fragments are generated during digestion and subsequent ligation: terminated with the same oligonucleotide on both 5′ ends of DNA fragments (two subsets) and terminated with two different oligonucleotides. Suppression PCR allows only the third subset of DNA fragments to be amplified exponentially. The method allows bacterial species strain differentiation on the basis of the different DNA band patterns obtained after electrophoresis in polyacrylamide gels stained with ethidium bromide and visualized in UV light.

Published
2001
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23. Production of highly and broad-range specific monoclonal antibodies against hemagglutinin of H5-subtype avian influenza viruses and their differentiation by mass spectrometry

Author

Violetta Cecuda-Adamczewska, Grazyna Plucienniczak, Porebska Anna, Katarzyna Florys, Marcin Zielinski, Anna Bierczyńska-Krzysik, Piotr Baran, and Violetta Sączyńska

Subjects
0301 basic medicine, medicine.drug_class, Viral disease diagnosis, Hemagglutinin (influenza), Enzyme-Linked Immunosorbent Assay, Hemagglutinin Glycoproteins, Influenza Virus, Antibodies, Viral, Monoclonal antibody, medicine.disease_cause, 01 natural sciences, Mass Spectrometry, Serology, lcsh:Infectious and parasitic diseases, Influenza hemagglutinin, Immunoglobulin Fab Fragments, Mice, 03 medical and health sciences, Orthomyxoviridae Infections, Peptide mass fingerprinting, Antibody Specificity, Virology, Infectious disease control, medicine, Animals, lcsh:RC109-216, Immunoassays, Screening procedures, Immunologic techniques, Influenza A Virus, H5N1 Subtype, biology, Research, 010401 analytical chemistry, Antibodies, Monoclonal, Isotype, Influenza A virus subtype H5N1, Influenza, 0104 chemical sciences, 030104 developmental biology, Infectious Diseases, MALDI-TOF/TOF MS, biology.protein, Female, Monoclonal antibodies, Antibody, Ficin digestion
Abstract

Background The highly pathogenic avian influenza viruses of the H5 subtype, such as the H5N1 viral strains or the novel H5N8 and H5N2 reassortants, are of both veterinary and public health concern worldwide. To combat these viruses, monoclonal antibodies (mAbs) against H5 hemagglutinin (HA) play a significant role. These mAbs are effective diagnostic and therapeutic agents and powerful tools in vaccine development and basic scientific research. The aim of this study was to obtain diagnostically valuable mAbs with broad strain specificity against H5-subtype AIVs. Results We applied the hybridoma method to produce anti-HA mAbs. The cloning and screening procedures resulted in the selection of 7 mouse hybridoma cell lines and their respective antibody clones. Preliminary immunoreactivity studies showed that these newly established mAbs, all of the IgG1 isotype, had high specificity and broad-range activities against the H5 HAs. However, these studies did not allow for a clear distinction among the selected antibodies and mAb-secreting hybridoma clones. To differentiate the analyzed mAbs and determine the exact number of hybridoma clones, peptide mapping of the Fc and Fab fragments was performed using a Matrix-Assisted Laser Desorption Ionization Time of Flight (MALDI-TOF/TOF) mass spectrometer. Detailed analyses of the acquired MS and MS/MS spectra confirmed that the Fc fragments constituted highly conserved species- and isotype-immunoglobulin components, whereas the Fab fragments exhibited considerable variation in the sequences that determine antibody specificity. This approach enabled unambiguous characterization of the selected mAbs according to their peptide composition. As a result, 6 different clones were distinguished. Conclusions Our work provided a unique panel of anti-H5 HA mAbs, which meets the demand for novel, high-specificity analytical tools for use in serologic surveillance. Applications of these mAbs in areas other than diagnostics are also possible. Moreover, we demonstrated for the first time that peptide mapping of antibody fragments with mass spectrometry is an efficient method for the differentiation of antibody clones and relevant antibody-producing cell lines. The method may be successfully used to characterize mAbs at the protein level. Electronic supplementary material The online version of this article (10.1186/s12985-017-0886-2) contains supplementary material, which is available to authorized users.

Published
2018

26. Molecular dissection of the replication system of plasmid pIGRK encoding two in-frame Rep proteins with antagonistic functions

Author

Anna Bierczyńska-Krzysik, Anna Mazurkiewicz-Pisarek, Andrzej Plucienniczak, Dariusz Bartosik, Paweł Wawrzyniak, Paulina Kabaj, Piotr Kierył, Natalia Łukasiewicz, Piotr Baran, Piotr Zaleski, Agata Gościk, and Agnieszka Sobolewska-Ruta

Subjects
Microbiology (medical), lcsh:QR1-502, Replication Origin, Locus (genetics), Biology, Replication system, Microbiology, Genome, lcsh:Microbiology, In-frame proteins, 03 medical and health sciences, chemistry.chemical_compound, Overlapping genes, Plasmid, Bacterial Proteins, Start codon, Gene Duplication, Gene duplication, Cloning, Molecular, Promoter Regions, Genetic, Gene, 030304 developmental biology, Genetics, Regulation of gene expression, 0303 health sciences, 030306 microbiology, Transcription regulation, Gene Expression Regulation, Bacterial, Rep protein, DNA-Binding Proteins, Klebsiella pneumoniae, chemistry, Protein Multimerization, Plasmid replication, DNA, Research Article, Plasmids
Abstract

BackgroundGene overlapping is a frequent phenomenon in microbial genomes. Excluding so-called “trivial overlapping”, there are significant implications of such genetic arrangements, including regulation of gene expression and modification of protein activity. It is also postulated that, besides gene duplication, the appearance of overlapping genes (OGs) is one of the most important factors promoting a genome’s novelty and evolution. OGs coding for in-frame proteins with different functions are a particularly interesting case. In this study we identified and characterized two in-frame proteins encoded by OGs on plasmid pIGRK fromKlebsiella pneumoniae, a representative of the newly distinguished pHW126 plasmid family.ResultsA singlerepRlocus located within the replication system of plasmid pIGRK encodes, in the same frame, two functional polypeptides: a full-length RepR protein and a RepR’ protein (withN-terminal truncation) translated from an internal START codon. Both proteins form homodimers, and interact with diverse DNA regions within the plasmid replication origin andrepRpromoter operator. Interestingly, RepR and RepR’ have opposing functions – RepR is crucial for initiation of pIGRK replication, while RepR’ is a negative regulator of this process. Nevertheless, both proteins act cooperatively as negative transcriptional regulators of their own expression.ConclusionsRegulation of the initiation of pIGRK replication is a complex process in which a major role is played by two in-frame proteins with antagonistic functions. In-frame encoded Rep proteins are uncommon, having been described in only a few plasmids. This is the first description of such proteins in a plasmid of the pHW126 family.

Published
2019

27. Prime-Boost Vaccination With a Novel Hemagglutinin Protein Produced in Bacteria Induces Neutralizing Antibody Responses Against H5-Subtype Influenza Viruses in Commercial Chickens

Author

Iwona Sokolowska, Violetta Cecuda-Adamczewska, Grazyna Plucienniczak, Malgorzata Kesik-Brodacka, Katarzyna Florys, Violetta Sączyńska, Natalia Łukasiewicz, and Agnieszka Romanik-Chruścielewska

Subjects
0301 basic medicine, lcsh:Immunologic diseases. Allergy, chicken, Immunology, Heterologous, Hemagglutinin Glycoproteins, Influenza Virus, Biology, medicine.disease_cause, 03 medical and health sciences, 0302 clinical medicine, Antigen, recombinant vaccine, medicine, Escherichia coli, Immunology and Allergy, Animals, hemagglutinin, Neutralizing antibody, Original Research, Hemagglutination assay, Influenza A Virus, H5N1 Subtype, poultry, Immune Sera, Vaccination, H5N1, Virology, Antibodies, Neutralizing, Influenza A virus subtype H5N1, Recombinant Proteins, 030104 developmental biology, Influenza Vaccines, Influenza in Birds, biology.protein, vaccination and immunization, H5-subtype influenza viruses, Antibody, lcsh:RC581-607, influenza, Chickens, 030215 immunology
Abstract

The highly pathogenic (HP) avian influenza virus (AIV), H5N1 and reassortant H5-subtype HPAIVs, H5N2, H5N6, and H5N8, cause high mortality in domestic birds, resulting in economic losses in the poultry industry. H5N1 and H5N6 also pose significant public health risks and H5N1 viruses are a permanent pandemic threat. To control HPAIVs, eukaryotic expression systems have traditionally been exploited to produce vaccines based on hemagglutinin (HA), a protective viral antigen. In contrast, we used a bacterial expression system to produce vaccine targeting the HA protein. A fragment of the HA ectodomain from H5N1, with a multibasic cleavage site deletion, was expressed in Escherichia coli, refolded, and chromatographically purified from inclusion bodies. The resulting antigen, rH5-E. coli, was validated in terms of conformational integrity and oligomerization status. Previously, the protective efficacy of rH5-E. coli adjuvanted with aluminum hydroxide, has been positively verified by challenging the specific pathogen-free layer chickens with homologous and heterologous H5N1 HPAIVs. Protection was provided primarily by the H5 subtype-specific antibodies, as detected in the FluAC H5 test. The present studies were conducted to assess the performance of alum-adjuvanted rH5-E. coli in commercial birds. Broiler chickens were vaccinated twice with 25 μg of rH5-E. coli at 2- and 4-week intervals, while the layer chickens were vaccinated with 5- to 25-μg antigen doses at 4- and 6-week intervals. Post-vaccination sera were analyzed for anti-H5 HA antibodies, using homologous ELISA and heterologous FluAC H5 and hemagglutination inhibition (HI) tests. Prime-boost immunizations with rH5-E. coli elicited H5 HA-specific antibodies in all the chickens tested. Two antigen doses administered at 4- or 6-week intervals were sufficient to induce neutralizing antibodies against H5-subtype HAs; however, they were ineffective when applied with a 2-week delay. In the layers, 80% to 100% of individuals developed antibodies that were active in the FluAC H5 and/or HI tests. A dose-sparing effect was seen when using the longer prime-boost interval. In the broiler chickens, 62.5% positivity was achieved in the FluAC H5 and/or HI tests. The trials confirmed the vaccine potential of rH5-E. coli and provided indications for anti-influenza vaccination with respect to the chicken type and immunization scheme.

Published
2019

28. pIGWZ12 – A cryptic plasmid with a modular structure

Author

Paweł Wawrzyniak, Agnieszka Sobolewska, Piotr Kierył, Grazyna Plucienniczak, Natalia Łukasiewicz, Katarzyna Romańczuk, Andrzej Plucienniczak, Piotr Baran, Katarzyna Daniszewska, and Piotr Zaleski

Subjects
DNA Replication, DNA, Bacterial, Genetics, Genotyping Techniques, DNA Helicases, Replication Origin, Sequence Analysis, DNA, Biology, Origin of replication, medicine.disease_cause, Homology (biology), Bacterial cell structure, Open Reading Frames, Plasmid, Cryptic plasmid, Subcloning, Escherichia coli, Trans-Activators, medicine, Cloning, Molecular, Promoter Regions, Genetic, Molecular Biology, Gene, Plasmids
Abstract

We studied the detailed structure of the cryptic plasmid pIGWZ12, which was isolated from an Escherichia coli strain. pIGWZ12 is composed of two structural modules of distinct evolutionary origin. The REP module, which contains all the features necessary for replication and stable maintenance in the bacterial cell, was assigned by genotyping to the IncF family. The MOB module, which is responsible for plasmid mobilization, shows significant homology to MOBQ modules from broad-host-range plasmids belonging to the RSF1010/R1162 family. We showed that iterons located in the origin of replication are the target for specific binding by the replication initiator protein RepApIGWZ12. Furthermore, we proved that the promoter for the repA gene overlaps with the iterons, and that the latter are the sole determinant of incompatibility. We performed a mutagenesis analysis of the MOBpIGWZ12 module and characterized the roles played by all identified genes (mobA and mobC), as well as the role played by oriT in mobilization. Finally, we showed that it was possible to remove the MOB module from pIGWZ12 without any loss in plasmid replication and stability. Furthermore, the MOBpIGWZ12 module was fully functional after subcloning into another plasmid. Therefore, pIGWZ12 is yet another example of modular structure in small cryptic plasmids.

Published
2015

29. Obtaining chicken primordial germ cells used for gene transfer: in vitro and in vivo results

Author

Grazyna Plucienniczak, Marek Bednarczyk, Dorota Sawicka, Pawel Lakota, Luiza Chojnacka-Puchta, and Andrzej Plucienniczak

Subjects
Expression vectors, Male, Transgene, Cell Separation, Biology, Transfection, Animals, Genetically Modified, In vivo, Cell Movement, Genetics, Animals, Primordial germ cells, Transgenes, Gonads, Cells, Cultured, Differential centrifugation, Expression vector, Chimera, Electroporation, General Medicine, Chicken embryo, Molecular biology, In vitro, Animal Genetics • Original Paper, Germ Cells, embryonic structures, Germline chimeras, Female, Genetic Engineering, Percoll, Chickens
Abstract

Recently, several attempts have been made to create a generation of transgenic chickens via chimeric intermediates produced by primordial germ cells (PGCs) transfer. This study aimed to compare the influences of different chicken PGCs isolated from circulating blood (bPGCs) or gonads (gPGCs), purification (ACK, Percoll or trypsin) and transfection methods (electroporation or lipofection) on the expression of transgenes in vitro and the migration of modified donor cells to the recipient gonads. The highest average frequency of pEGFP-N1 plasmid-transfected bPGCs (75.8 %) was achieved with Percoll density gradient centrifugation and electroporation. After ammonium chloride-potassium (ACK) treatment and lipofection, in vitro transgene expression was only detected in 35.2 % of bPGCs. Chimeric chickens were produced from these purified, transfected and cultured cells, and the transgene was detected in the gonads of 44 and 42 % of the recipient embryos that had been injected with bPGCs and gPGCs, respectively. These data confirmed that the combination of PGC purification via Percoll centrifugation and electroporation was an effective method for producing transgenic chickens. Subsequently, we used this method with expression vectors for gene hIFNα 2a/hepatitis B virus surface antigen (HBsAg) under the control of the ovalbumin promoter to generate G0 transgenic chickens. Consequently, we observed that 4.9 % of the hens and 3.5 % of the roosters carried the hIFNα 2a gene, whereas 16.7 % of the hens and 2.4 % of the roosters carried the HBsAg gene, thus undisputedly confirming the exceptional effectiveness of the applied methods.

Published
2015

30. Biotechnological Approaches to Making Vaccine in Plants

Author

Kapusta, J., primary, Modelska, A., additional, Figlerowicz, M., additional, Podkowinski, J., additional, Pniewski, T., additional, Lisowa, O., additional, Berbezy, P., additional, Helias, D., additional, Biesiadka, J., additional, Femiak, I., additional, Letellier, M., additional, Yusibov, V., additional, Koprowski, H., additional, Plucienniczak, A., additional, and Legocki, A. B., additional

Published
1999
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32. Soluble insulin analogs combining rapid- and long-acting hypoglycemic properties - From an efficient E. coli expression system to a pharmaceutical formulation

Author

Jacek Stadnik, Diana Mikiewicz, Monika Bogiel, M. Pawlowska, Iwona Sokolowska, Agnieszka Sobolewska, Grazyna Plucienniczak, Anna Bierczyńska-Krzysik, Anna Wojtowicz-Krawiec, Andrzej Plucienniczak, Dorota Stadnik, Piotr Borowicz, Natalia Łukasiewicz, Piotr Baran, and Agnieszka Romanik-Chruścielewska

Subjects
0301 basic medicine, Reversed-Phase High Performance Liquid Chromatography, Molecular biology, medicine.medical_treatment, lcsh:Medicine, Pharmacology, Biochemistry, Inclusion bodies, law.invention, 0302 clinical medicine, Endocrinology, law, Medicine and Health Sciences, Insulin, lcsh:Science, Liquid Chromatography, Multidisciplinary, Expression vector, Chemistry, Organic Compounds, Pharmaceutics, Monosaccharides, Chromatographic Techniques, Drugs, Biological activity, Trypsin, Enzymes, Dismutases, Pharmaceutical Preparations, Physical Sciences, Recombinant DNA, medicine.drug, Research Article, Signal peptide, Drug Administration, Endocrine Disorders, Carbohydrates, Hypoglycemics, 030209 endocrinology & metabolism, DNA construction, 03 medical and health sciences, Drug Therapy, medicine, Escherichia coli, Diabetes Mellitus, Hypoglycemic Agents, Diabetic Endocrinology, Superoxide Dismutase, Organic Chemistry, lcsh:R, Chemical Compounds, Biology and Life Sciences, Proteins, Reversed Phase Chromatography, Fusion protein, Hormones, High Performance Liquid Chromatography, Research and analysis methods, 030104 developmental biology, Molecular biology techniques, Glucose, Solubility, Metabolic Disorders, Plasmid Construction, Enzymology, lcsh:Q
Abstract

The discovery of insulin led to a revolution in diabetes management. Since then, many improvements have been introduced to insulin preparations. The availability of molecular genetic techniques has enabled the creation of insulin analogs by changing the structure of the native protein in order to improve the therapeutic properties. A new expression vector pIBAINS for production of four recombinant human insulin (INS) analogs (GKR, GEKR, AKR, SR) was constructed and overexpressed in the new E. coli 20 strain as a fusion protein with modified human superoxide dismutase (SOD). The SOD gene was used as a signal peptide to enhance the expression of insulin. SOD::INS was manufactured in the form of insoluble inclusion bodies. After cleavage of the fusion protein with trypsin, the released insulin analogs were refolded and purified by reverse-phase high performance liquid chromatography (RP-HPLC). Elongation of chain A, described here for the first time, considerably improved the stability of the selected analogs. Their identity was confirmed with mass spectrometric techniques. The biological activity of the insulin derivatives was tested on rats with experimental diabetes. The obtained results proved that the new analogs described in this paper have the potential to generate prolonged hypoglycemic activity and may allow for even less frequent subcutaneous administration than once-a-day. When applied, all the analogs demonstrate a rapid onset of action. Such a combination renders the proposed biosynthetic insulin unique among already known related formulations.

Published
2017

33. A novel hemagglutinin protein produced in bacteria protects chickens against H5N1 highly pathogenic avian influenza viruses by inducing H5 subtype-specific neutralizing antibodies

Author

Zenon Minta, Monika Olszewska, Katarzyna Florys, Agnieszka Romanik, Krzysztof Śmietanka, Violetta Sączyńska, Boguslaw Szewczyk, Violetta Cecuda-Adamczewska, Grazyna Plucienniczak, Katarzyna Domańska-Blicharz, Andrzej Plucienniczak, and Malgorzata Kesik-Brodacka

Subjects
RNA viruses, 0301 basic medicine, Hemagglutination, Physiology, animal diseases, lcsh:Medicine, medicine.disease_cause, Biochemistry, Poultry, Zoonoses, Immune Physiology, Medicine and Health Sciences, Influenza A virus, Gamefowl, Public and Occupational Health, Enzyme-Linked Immunoassays, lcsh:Science, Pathology and laboratory medicine, Vaccines, Immune System Proteins, Multidisciplinary, biology, virus diseases, Agriculture, H5N1, Medical microbiology, Vaccination and Immunization, Infectious Diseases, Vertebrates, Viruses, Pathogens, Research Article, Antigenicity, Livestock, Immunology, Hemagglutinin (influenza), Research and Analysis Methods, Microbiology, Antibodies, Virus, Birds, 03 medical and health sciences, Antigen, medicine, Animals, Influenza viruses, Antigens, Viral shedding, Immunoassays, Biology and life sciences, lcsh:R, Organisms, Viral pathogens, Proteins, Virology, Influenza A virus subtype H5N1, Microbial pathogens, 030104 developmental biology, Fowl, Amniotes, Immunologic Techniques, biology.protein, lcsh:Q, Preventive Medicine, Chickens, Orthomyxoviruses
Abstract

The highly pathogenic (HP) H5N1 avian influenza viruses (AIVs) cause a mortality rate of up to 100% in infected chickens and pose a permanent pandemic threat. Attempts to obtain effective vaccines against H5N1 HPAIVs have focused on hemagglutinin (HA), an immunodominant viral antigen capable of eliciting neutralizing antibodies. The vast majority of vaccine projects have been performed using eukaryotic expression systems. In contrast, we used a bacterial expression system to produce vaccine HA protein (bacterial HA) according to our own design. The HA protein with the sequence of the H5N1 HPAIV strain was efficiently expressed in Escherichia coli, recovered in the form of inclusion bodies and refolded by dilution between two chromatographic purification steps. Antigenicity studies showed that the resulting antigen, referred to as rH5-E. coli, preserves conformational epitopes targeted by antibodies specific for H5-subtype HAs, inhibiting hemagglutination and/or neutralizing influenza viruses in vitro. The proper conformation of this protein and its ability to form functional oligomers were confirmed by a hemagglutination test. Consistent with the biochemical characteristics, prime-boost immunizations with adjuvanted rH5-E. coli protected 100% and 70% of specific pathogen-free, layer-type chickens against challenge with homologous and heterologous H5N1 HPAIVs, respectively. The observed protection was related to the positivity in the FluAC H5 test (IDVet) but not to hemagglutination-inhibiting antibody titers. Due to full protection, the effective contact transmission of the homologous challenge virus did not occur. Survivors from both challenges did not or only transiently shed the viruses, as established by viral RNA detection in oropharyngeal and cloacal swabs. Our results demonstrate that vaccination with rH5-E. coli could confer control of H5N1 HPAIV infection and transmission rates in chicken flocks, accompanied by reduced virus shedding. Moreover, the role of H5 subtype-specific neutralizing antibodies in anti-influenza immunity and a novel correlate of protection are indicated.

Published
2017

35. Expression and purification of recombinant human insulin from E. coli 20 strain

Author

Marcin Zielinski, Iwona Sokolowska, Diana Mikiewicz, Anna Bierczyńska-Krzysik, Natalia Łukasiewicz, Jarosław Antosik, Agnieszka Sobolewska-Ruta, Agnieszka Romanik-Chruścielewska, Piotr Zaleski, and Andrzej Plucienniczak

Subjects
0106 biological sciences, medicine.medical_treatment, Genetic Vectors, Gene Expression, Biology, medicine.disease_cause, 01 natural sciences, Inclusion bodies, law.invention, 03 medical and health sciences, Industrial Microbiology, Bioreactors, law, 010608 biotechnology, Diabetes mellitus, medicine, Escherichia coli, Humans, Insulin, Chromatography, High Pressure Liquid, 030304 developmental biology, Inclusion Bodies, 0303 health sciences, Expression vector, Trypsin, medicine.disease, Recombinant Proteins, Biochemistry, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Recombinant DNA, Biotechnology, medicine.drug, Protein Renaturation, Plasmids
Abstract

The number of people with diabetes is estimated to be over 370 million, in 2030 it will increase to 552 million. In Poland, the number of people with diabetes is estimated to be 3.5 million (9.1%). According to the estimates of the International Diabetes Federation, the percentage of patients in the adult Polish population will increase to around 11% over the next 20 years. Despite the appearance of insulin analogues on the pharmaceutical market, insulin delivery is still the most effective method of pharmacotherapy in cases of extremely high hyperglycemia. A new bacterial host strain (Escherichia coli 20) was obtained at the Institute of Biotechnology and Antibiotics and a new pIBAINS expression vector was constructed that provides greater efficiency in the production of recombinant human insulin. In the IBA Bioengineering Department, successful attempts were made to produce recombinant human insulin on a laboratory and quarter-technical scale, and several batches were performed on a semi-technical scale. The production process has been divided into several stages: 1. biosynthesis of insulin in the fermenter, 2. isolation, purification and dissolution of inclusion bodies, 3. protein renaturation, 4. enzymatic reaction with trypsin, 5. multi-stage purification of insulin using low-pressure and HPLC techniques. At each stage of insulin production, qualitative and quantitative analyses were performed to confirm identity and purity. In particular, the molecular weight of insulin, the amount of insulin and the content of protein impurities were studied. The results of these experiments are presented in this work.

Published
2018

36. Insight into human insulin aggregation revisited using NMR derived translational diffusion parameters

Author

Mateusz Urbańczyk, Grazyna Plucienniczak, Iwona Sokolowska, Jerzy Sitkowski, Lech Kozerski, Natalia Łukasiewicz, Wojciech Bocian, Elżbieta Bednarek, Wiktor Koźmiński, and Piotr Borowicz

Subjects
0301 basic medicine, Protein Folding, 030102 biochemistry & molecular biology, Chemistry, Ligand, Thermodynamics, Pharmaceutical formulation, Protein aggregation, Ligands, Biochemistry, Ion, Diffusion, 03 medical and health sciences, Protein Aggregates, Zinc, 030104 developmental biology, Exponential growth, Humans, Insulin, Protein folding, Diffusion (business), Nuclear Magnetic Resonance, Biomolecular, Spectroscopy, Heteronuclear single quantum coherence spectroscopy
Abstract

The NMR derived translational diffusion coefficients were performed on unlabeled and uniformly labeled 13C,15N human insulin in water, both in neat, with zinc ions only, and in pharmaceutical formulation, containing only m-cresol as phenolic ligand, glycerol and zinc ions. The results show the dominant role of the pH parameter and the concentration on aggregation. The diffusion coefficient Dav was used for monitoring the overall average state of oligomeric ensemble in solution. The analysis of the experimental data of diffusion measurements, using the direct exponential curve resolution algorithm (DECRA) allows suggesting the two main components of the oligomeric ensemble. The 3D HSQC-iDOSY, (diffusion ordered HSQC) experiments performed on 13C, 15N-fully labeled insulin at the two pH values, 4 and 7.5, allow for the first time a more detailed experimental observation of individual components in the ensemble. The discussion involves earlier static and dynamic laser light scattering experiments and recent NMR derived translational diffusion results. The results bring new informations concerning the preparation of pharmaceutical formulation and in particular a role of Zn2+ ions. They also will enable better understanding and unifying the results of studies on insulin misfolding effects performed in solution by diverse physicochemical methods at different pH and concentration.

Published
2018

37. Diversity and Global Distribution of IncL/M Plasmids Enabling Horizontal Dissemination ofβ-Lactam Resistance Genes among the Enterobacteriaceae

Author

Marcin Adamczuk, Paweł Wawrzyniak, Piotr Kierył, Marta Nieckarz, Lukasz Dziewit, Piotr Zaleski, Dariusz Bartosik, Andrzej Plucienniczak, and Renata Wolinowska

Subjects
Article Subject, Gene Transfer, Horizontal, lcsh:Medicine, medicine.disease_cause, Genome, beta-Lactam Resistance, beta-Lactamases, General Biochemistry, Genetics and Molecular Biology, Microbiology, Plasmid, Enterobacteriaceae, medicine, Replicon, Gene, Escherichia coli, Genetics, General Immunology and Microbiology, Phylogenetic tree, biology, lcsh:R, Genetic Variation, Genomics, General Medicine, biology.organism_classification, Phylogeography, Genes, Bacterial, DNA, Circular, Mobile genetic elements, Research Article, Plasmids
Abstract

Antibiotic resistance determinants are frequently associated with plasmids and other mobile genetic elements, which simplifies their horizontal transmission. Several groups of plasmids (including replicons of the IncL/M incompatibility group) were found to play an important role in the dissemination of resistance genes encodingβ-lactamases. The IncL/M plasmids are large, broad host range, and self-transmissible replicons. We have identified and characterized two novel members of this group: pARM26 (isolated from bacteria inhabiting activated sludge from a wastewater treatment plant) and pIGT15 (originating from a clinical strain ofEscherichia coli). This instigated a detailed comparative analysis of all available sequences of IncL/M plasmids encodingβ-lactamases. The core genome of these plasmids is comprised of 20 genes with conserved synteny. Phylogenetic analyses of these core genes allowed clustering of the plasmids into four separate groups, which reflect their antibiotic resistance profiles. Examination of the biogeography of the IncL/M plasmids revealed that they are most frequently found in bacteria of the family Enterobacteriaceae originating from the Mediterranean region and Western Europe and that they are able to persist in various ecological niches even in the absence of direct antibiotic selection pressure.

Published
2015

38. The factor VIII protein and its function

Author

Anna Mazurkiewicz-Pisarek, Grazyna Plucienniczak, Tomasz Ciach, and Andrzej Plucienniczak

Subjects
Models, Molecular, 0301 basic medicine, Severe bleeding, Coagulation protein, Heavy chain, Factor VIII, Chemistry, Single chain, Hemophilia A, Immunoglobulin light chain, General Biochemistry, Genetics and Molecular Biology, Factor IXa, 03 medical and health sciences, 030104 developmental biology, Biochemistry, Humans, Secretion, Function (biology)
Abstract

Factor VIII (FVIII), an essential blood coagulation protein, is a key component of the fluid phase blood coagulation system. Human factor VIII is a single chain of about 300 kDa consisting of domains described as A1-A2-B-A3-C1-C2. The protein undergoes processing prior to secretion into blood resulting in a heavy chain of 200 kDa (A1-A2-B) and a light chain of 80 kDa (A3-C1-C2) linked by metal ions. The role of factor VIII is to increase the catalytic efficiency of factor IXa in the activation of factor X. Variants of these factors lead frequently also to severe bleeding disorders.

Published
2016

39. New cloning and expression vector derived from Escherichia coli plasmid pIGWZ12; A potential vector for a two-plasmid expression system

Author

Piotr Zaleski, Marcin Zielinski, Agnieszka Sobolewska, Diana Mikiewicz, Anna Wojtowicz-Krawiec, Paweł Wawrzyniak, Andrzej Plucienniczak, Luiza Chojnacka-Puchta, and Grazyna Plucienniczak

Subjects
DNA Replication, Genetic Vectors, Restriction Mapping, Gene Dosage, Cloning vector, Biology, Origin of replication, medicine.disease_cause, Plasmid, Kanamycin, Escherichia coli, medicine, Humans, Cloning, Molecular, Molecular Biology, T-DNA Binary system, Genetics, Plasmid preparation, Cloning, Expression vector, Gene Expression Regulation, Bacterial, Sequence Analysis, DNA, Molecular biology, DNA-Binding Proteins, Electrophoresis, Polyacrylamide Gel, Plasmids, Transcription Factors
Abstract

We constructed pIGPZ, a new cloning and expression vector derived from Escherichia coli plasmid pIGWZ12::Kan. pIGPZ contains a kanamycin resistance marker, a multiple-cloning-site (MCS) region, and a promoter for constitutive expression of cloned genes. pIGPZ has the same high level of stability as the original plasmid, even in the absence of antibiotic selection. Furthermore, we show that pIGPZ is compatible with ColE1-based plasmids and a pSC101-like plasmid. All the characteristic elements of theta-replicating plasmids were found in the pIGPZ putative origin of replication. Finally, we demonstrate that pIGPZ can be used in a double-plasmid expression system by co-expressing UBP1 protease from pIGPZ with ubi-interferon alpha (IFNA13; GenBank Accession No. NM_006900.3) or ubi-human growth hormone (ubi-hGH; patent No. WO 2005/066208 A2) cloned in another plasmid. In this system, both ubi-interferon alpha and ubi-human growth hormone were deubiquitinated efficiently in E. coli cells.

Published
2012

41. PLASMIDS – VECTORS FOR GENE THERAPY

Author

Grazyna Plucienniczak, Agnieszka Sobolewska, Piotr Zaleski, and Paweł Wawrzyniak

Subjects
Microbiology (medical), Genetics, plasmids, Genetic enhancement, lcsh:QR1-502, plazmidy, Biology, Microbiology, gene therapy, lcsh:Microbiology, Plasmid, terapia genowa, vectors, wektory
Abstract

The first confirmed transfer of genetic material in human was performed in 1990. Ever since, gene therapy was considered to be one of the best promising treatments of genetic diseases. The sine qua non of successful gene therapy are efficient genetic vectors. Recently, the most frequently used vectors in clinical trials for genetic therapies are virus-based and plasmid-based. A range of features makes plasmids useful for gene therapy, however, they have also some characteristics which make it difficult to consider plasmids as ideal vectors. The main goal of this article is to address and describe these unfavourable factors. 1. Introduction. 2. Natural modification of DNA as an obstacle to the use of plasmids for gene therapy. 3. Plasmid DNA usage safety. 4. Plasmid DNA entry into eucaryotic cells. 5. Post-entry fate of plasmid DNA in eucaryotic cells. 6. pDNA-based gene therapies. 7. Alternative routes of development of pDNA-based gene therapies. 7.1. Baktofection. 7.2. Alternative Gene Therapy – AGT. 7.3. Hydrogels. 7.4. DNA minicircles. 7.5. DNA ministrings. 8. Summary 1. Wstęp. 2. Naturalna modyfikacja DNA jako przeszkoda w stosowaniu plazmidów w terapii genowej. 3. Bezpieczeństwo użycia plazmidowego DNA. 4. Wprowadzenie pDNA do komórek eukariotycznych. 5. Los plazmidowego DNA po wprowadzeniu do komórek eukariotycznych. 6. Terapie genowe bazujące na pDNA. 7. Inne kierunki rozwoju terapii genowych opartych na plazmidowym DNA. 7.1 Baktofekcja. 7.2. Alternatywna terapia genowa (Alternative Gene Therapy – AGT). 7.3. Hydrożele. 7.4. Minikoliste DNA. 7.5. Mininici DNA. 8. Podsumowanie

Published
2017

42. Immune response of rats vaccinated orally with various plant-expressed recombinant cysteine proteinase constructs when challenged with Fasciola hepatica metacercariae

Author

Katarzyna Miedzinska, Malgorzata Kesik-Brodacka, Monika Kozak Ljunggren, Andrzej B. Legocki, Agnieszka Lipiec, Magdalena Mikolajczak, Luiza Jedlina, Halina Wędrychowicz, and Andrzej Plucienniczak

Subjects
Male, 0301 basic medicine, Physiology, Administration, Oral, Biochemistry, Epitope, law.invention, Rats, Sprague-Dawley, Random Allocation, 0302 clinical medicine, Cysteine Proteases, law, Immune Physiology, Vegetables, Vaccines, DNA, Medicine and Health Sciences, Public and Occupational Health, Amino Acids, Immune Response, Flowering Plants, Vaccines, Immune System Proteins, biology, Organic Compounds, lcsh:Public aspects of medicine, Vaccination, Proteases, Plants, Lettuce, Plants, Genetically Modified, Vaccination and Immunization, Recombinant Proteins, Enzymes, Chemistry, HBcAg, Infectious Diseases, Physical Sciences, Recombinant DNA, Antibody, Research Article, Fascioliasis, lcsh:Arctic medicine. Tropical medicine, DNA, Complementary, Infectious Disease Control, lcsh:RC955-962, Immunology, 030231 tropical medicine, Antibodies, Helminth, Antibodies, Host-Parasite Interactions, Microbiology, Microbiology in the medical area, 03 medical and health sciences, Immune system, Antigen, Mikrobiologi inom det medicinska området, Animals, Sulfur Containing Amino Acids, Fasciola hepatica, Metacercariae, Cysteine, Antigens, Organic Chemistry, Organisms, Chemical Compounds, Public Health, Environmental and Occupational Health, Biology and Life Sciences, Proteins, lcsh:RA1-1270, biology.organism_classification, Virology, Rats, 030104 developmental biology, Immunoglobulin M, Antigens, Helminth, Immunoglobulin G, Enzymology, biology.protein, Preventive Medicine
Abstract

Background Cysteine proteinases of Fasciola hepatica are important candidates for vaccine antigens because of their role in fluke biology and host-parasite relationships. In our previous experiments, we found that a recombinant cysteine proteinase cloned from adult F. hepatica (CPFhW) can protect rats against liver fluke infections when it is administered intramuscularly or intranasally in the form of cDNA. We also observed considerable protection upon challenge following mucosal vaccination with inclusion bodies containing recombinant CPFhW produced in Escherichia coli. In this study, we explore oral vaccination, which may be the desired method of delivery and is potentially capable of preventing infections at the site of helminth entry. To provide antigen encapsulation and to protect the vaccine antigen from degradation in the intestinal tract, transgenic plant-based systems are used. Methodology In the present study, we aimed to evaluate the protective ability of mucosal vaccinations of 12-week-old rats with CPFhW produced in a transgenic-plant-based system. To avoid inducing tolerance and to maximise the immune response induced by oral immunisation, we used the hepatitis B virus (HBV) core protein (HBcAg) as a carrier. Animals were immunised with two doses of the antigen and challenged with 25 or 30 metacercariae of F. hepatica. Conclusions We obtained substantial protection after oral administration of the plant-produced hybrids of CPFhW and HBcAg. The highest level of protection (65.4%) was observed in animals immunised with transgenic plants expressing the mature CPFhW enzyme flanked by Gly-rich linkers and inserted into c/e1 epitope of truncated HBcAg. The immunised rats showed clear IgG1 and IgM responses to CPFhW for 4 consecutive weeks after the challenge., Author summary Infection with Fasciola hepatica, a liver fluke, is one of the most significant veterinary problems due to the worldwide distribution of this parasite, a wide spectrum of host organisms and the resulting economic loss. Human fasciolosis caused by F. hepatica is recognised by the World Health Organization as an important emerging but neglected tropical disease. Development of an effective vaccine against this disease is becoming a priority, especially as the appearance of drug-resistant strains undermine the currently employed drug-based treatments. The two primary issues when developing a vaccine are the selection of an appropriate vaccine antigen and the route of antigen administration. In our studies, we use one of the F. hepatica cysteine proteinases, which are promising antigens for vaccine construction. We evaluate the immunogenicity and protective ability of various modifications of this cysteine proteinase produced in plants. We show that substantial protection can be obtained when plant-expressed hybrid proteins are administered orally.

Published
2017

44. Expression of recombinant human bifunctional peptidylglycine α-amidating monooxygenase in CHO cells and its use for insulin analogue modification

Author

Malgorzata Kesik-Brodacka, Marcin Zielinski, Violetta Cecuda-Adamczewska, Grazyna Plucienniczak, Diana Mikiewicz, Natalia Łukasiewicz, Piotr Borowicz, Iwona Sokolowska, Lidia Gurba, Anna Wojtowicz-Krawiec, Boguslaw Szewczyk, Andrzej Plucienniczak, Alina Marciniak-Rusek, Michał Odrowąż-Sypniewski, and Piotr Baran

Subjects
0301 basic medicine, Blood Glucose, Male, medicine.medical_treatment, Drug Evaluation, Preclinical, CHO Cells, law.invention, Diabetes Mellitus, Experimental, Mixed Function Oxygenases, 03 medical and health sciences, Cricetulus, law, Diabetes mellitus, Cricetinae, medicine, Animals, Hypoglycemic Agents, Insulin, Rats, Wistar, Chromatography, High Pressure Liquid, chemistry.chemical_classification, 030102 biochemistry & molecular biology, Insulin glargine, Chinese hamster ovary cell, Monooxygenase, medicine.disease, Streptozotocin, Recombinant Proteins, 030104 developmental biology, Enzyme, Biochemistry, chemistry, Amidine-Lyases, Recombinant DNA, Chromatography, Gel, Female, Biotechnology, medicine.drug
Abstract

The availability of catalytically active peptidylglycine α-amidating monooxygenase (PAM) should provide the means to examine its potential use for the chemienzymatic synthesis of bioactive peptides for the purpose of pharmacological studies. Hypoglycemic activity is one of the most important features of insulin derivatives. Insulin glargine amide was found to show a time/effect profile which is distinctly more flat and thus more advantageous than insulin glargine itself. The aim of the study was to obtain recombinant PAM and use it for insulin analogue amidation. We stably expressed a recombinant PAM in CHO dhfr-cells in culture. Recombinant PAM was partially purified by fractional ammonium sulphate precipitation and ion-exchange chromatography. The enzyme was used to modify glycine-extended A22(G)-B31(K)-B32(R) human insulin analogue (GKR). Alpha-amidated insulin was analyzed by HPLC and mass spectrometry. Hypoglycemic activity of amidated and non-amidated insulin was compared. The pharmacodynamic effect was based on glucose concentration measurement in Wistar rats with hyperglycemia induced by streptozotocin. The overall glycemic profile up to 36 h was evaluated after subcutaneous single dosing at a range of 2.5-7.5 U/kg b.w. The experiment on rats confirmed with a statistical significance (P0.05) hypoglycemic activity of GKR-NH2 in comparison to a control group receiving 0.9% NaCl. Characteristics for GKR-NH2 profile was a rather fast beginning of action (0.5-2.0 h) and quite prolonged return to initial values. GKR-NH2 is a candidate for a hypoglycemic drug product in diabetes care. In addition, this work also provides a valuable alternative method for preparing any other recombinant bioactive peptides with C-terminal amidation.

Published
2015

45. Immune response of rats vaccinated orally with various plant-expressed recombinant cysteine proteinase constructs when challenged with Fasciola hepatica metacercariae

Author

Kesik-Brodacka, Malgorzata, Lipiec, Agnieszka, Kozak Ljunggren, Monika, Jedlina, Luiza, Miedzinska, Katarzyna, Mikolajczak, Magdalena, Plucienniczak, Andrzej, Legocki, Andrzej B., Wedrychowicz, Halina, Kesik-Brodacka, Malgorzata, Lipiec, Agnieszka, Kozak Ljunggren, Monika, Jedlina, Luiza, Miedzinska, Katarzyna, Mikolajczak, Magdalena, Plucienniczak, Andrzej, Legocki, Andrzej B., and Wedrychowicz, Halina

Abstract

Background Cysteine proteinases of Fasciola hepatica are important candidates for vaccine antigens because of their role in fluke biology and host-parasite relationships. In our previous experiments, we found that a recombinant cysteine proteinase cloned from adult F. hepatica ( CPFhW) can protect rats against liver fluke infections when it is administered intramuscularly or intranasally in the form of cDNA. We also observed considerable protection upon challenge following mucosal vaccination with inclusion bodies containing recombinant CPFhW produced in Escherichia coli. In this study, we explore oral vaccination, which may be the desired method of delivery and is potentially capable of preventing infections at the site of helminth entry. To provide antigen encapsulation and to protect the vaccine antigen from degradation in the intestinal tract, transgenic plant-based systems are used. Methodology Conclusions We obtained substantial protection after oral administration of the plant-produced hybrids of CPFhW and HBcAg. The highest level of protection (65.4%)was observed in animals immunised with transgenic plants expressing the mature CPFhW enzyme flanked by Gly-rich linkers and inserted into c/e1 epitope of truncated HBcAg. The immunised rats showed clear IgG1 and IgM responsesIn the present study, we aimed to evaluate the protective ability of mucosal vaccinations of 12-week- old rats with CPFhW produced in a transgenic-plant-based system. To avoid inducing tolerance and to maximise the immune response induced by oral immunisation, we used the hepatitis B virus (HBV) core protein ( HBcAg) as a carrier. Animals were immunised with two doses of the antigen and challenged with 25 or 30 metacercariae of F. hepatica. Conclusions We obtained substantial protection after oral administration of the plant-produced hybrids of CPFhW and HBcAg. The highest level of protection (65.4%) was observed in animals immunised with transgenic plants expressing the mature CPFhW enzyme, Funding Agencies|Polish Ministry of Scientific Research and Information Technology [PBZ-MIN-007/P04/05, PBZ-MIN-007/P04/06, PBZ-MIN-007/P04/04]

Published
2017
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46. Flow cytometric analysis of apoptosis in cryoconserved chicken primordial germ cells

Author

Marcin Zielinski, Dorota Sawicka, Marek Bednarczyk, Luiza Chojnacka-Puchta, Andrzej Plucienniczak, and Grazyna Plucienniczak

Subjects
endocrine system, Cryoprotectant, Cell Survival, Apoptosis, Biology, Biochemistry, Cryopreservation, Flow cytometry, Cryoprotective Agents, In vivo, medicine, Animals, Molecular Biology, Differential centrifugation, medicine.diagnostic_test, urogenital system, fungi, Embryo, Cell Biology, Flow Cytometry, Molecular biology, Staining, Germ Cells, embryonic structures, Percoll, Chickens
Abstract

Our research aimed to compare the effects of four cryoprotectants and four slow freezing programs on the viability and apoptosis of primordial germ cells (PGCs) in vitro. PGCs were collected from chicken embryonic blood at Hamburger and Hamilton (HH) stages 14-16 and purified by Percoll density gradient centrifugation and then subjected to cryopreservation. We applied microscopy to determine the survival of PGCs after trypan blue staining and flow cytometry to examine apoptosis and viability after annexin V kit staining. We also examined the functionality of cryopreserved PGCs in vivo. Significant differences in viability of PGCs determined via microscopy and flow cytometry were observed. The most unfavorable combination for slow freezing PGCs was program 3 and MIX H (10% DMSO and 5% glycerol in Hank’s solution supplemented with 10% FBS) as the cryoprotectant (48.43 and 15.37% live and early apoptotic PGCs, respectively). The highest average percentage of live PGCs (93.1%) and the lowest percentage of early apoptotic PGCs (6.5%) were achieved by slow freezing PGCs in the presence of DMSO F (10% DMSO in FBS) via program 1. Therefore, this method was chosen for the in vivo test. Cryopreserved (group 1) and freshly isolated (group 2) PGCs were transfectedwith a pEGFP-N1 plasmid, cultured under antibiotic selection, and then injected into 3-day-old embryos. After 5 days of incubation, we identified the EGFP marker gene in the gonads of 40 and 45% of recipients in groups 1 and 2, respectively. This is the first study to apply flow cytometry to examine the apoptosis and viability of cryopreserved PGCs. The in vitro and in vivo findings showed that the developed PGC cryoconservation method, depending on slow freezing at the rate of 2°C/min (program 1) in the presence of 10% DMSO F, is an improvement over previous cryoconservation methods and may be a useful tool for the ex situ strategy of poultry biodiversity preservation.

Published
2014

47. Structure and pharmaceutical formulation development of a new long-acting recombinant human insulin analog studied by NMR and MS

Author

Beata Jaworska, Jerzy Sitkowski, Dorota Stadnik, Lech Kozerski, Wojciech Bocian, Grazyna Plucienniczak, Weronika Surmacz-Chwedoruk, Piotr Borowicz, and Elżbieta Bednarek

Subjects
0301 basic medicine, Protein Conformation, alpha-Helical, Spectrometry, Mass, Electrospray Ionization, Magnetic Resonance Spectroscopy, medicine.medical_treatment, Drug Compounding, Clinical Biochemistry, Population, Pharmaceutical Science, Pharmaceutical formulation, 010402 general chemistry, Crystallography, X-Ray, 01 natural sciences, Oligomer, Analytical Chemistry, law.invention, 03 medical and health sciences, chemistry.chemical_compound, law, Drug Discovery, medicine, Humans, Insulin, Acetonitrile, education, Spectroscopy, education.field_of_study, Chromatography, Insulin glargine, Recombinant Proteins, 0104 chemical sciences, 030104 developmental biology, Monomer, chemistry, Delayed-Action Preparations, Recombinant DNA, Protein Conformation, beta-Strand, medicine.drug
Abstract

A monomer structure of a novel human insulin analog A22S-B3K-B31R (SK3R) has been characterized by NMR in water/acetonitrile solution and compared with the structure of human insulin (HIS) established in the same medium. The composition of the oligomer ensemble for neat insulins in water was qualitatively assessed by monitoring, derived from NMR experiment, translational diffusion coefficient Dix10-10m2s-1, whose value is a population averaged of individual coefficients for species in oligomeric ensemble. Nanospray ESI/MS experiment was used to establish the masses of oligomers in pharmaceutical formulation of the SK3R insulin. The pharmacodynamic data were established and compared to insulin glargine characterized by the same profile of action in diabetics. The oligomerization process of insulin during development of pharmaceutical formulation with routinely used excipients has been studied using translation diffusion coefficient Dix10-10m2s-1 established in water solution. These properties were compared with those of human insulin (HIS) which is a standard reference for novel recombinant insulins.

Published
2016

48. Efficient Source of Cells in Proximal Oviduct for Testing Non-Viral Expression Constructs in the Chicken Bioreactor Model and for Other in Vitro Studies

Author

Magdalena Bodnar, Aleksandra Dunislawska, Luiza Chojnacka-Puchta, Violetta Cecuda-Adamczewska, Grazyna Plucienniczak, Katarzyna Stadnicka, Tomasz Drewa, Marek Bednarczyk, Anna Bajek, and Andrzej Marszałek

Subjects
0301 basic medicine, animal structures, Population, Cell Culture Techniques, Oviducts, Biology, Interferon alpha-2, Transfection, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Bioreactors, Animals, Humans, Progenitor cell, education, Cells, Cultured, Regulation of gene expression, education.field_of_study, Expression vector, Interferon-alpha, Epithelial Cells, General Medicine, Molecular biology, In vitro, Recombinant Proteins, 030104 developmental biology, Gene Expression Regulation, Cell culture, Oviduct, Female, Chickens, Biomarkers
Abstract

This work shows the usefulness of chicken oviduct epithelial cells (COEC) in evaluating the efficacy of non-viral expression vectors carrying human therapeutic genes. Secondly, an efficient source of progenitor COEC for in vitro studies is described. Within the distal part of the oviduct, weak to moderate expression of a trans membrane glycoprotein (CD44) was observed. Single cells presenting only weak expression of CD44 were found in magnum sections. in vitro cultured oviduct cells originating from the distal oviduct were suitable for subculturing and showed a stable proliferation potential up to the 2nd passage. However, the pavimentous epithelial-like morphology of COEC was progressively lost over time and mainly a fibroblast-like monolayer was established in consecutive passages. Moreover, various commercial transfection agents including FuGENE6 and XtremeGENE9 DNA were used to optimize delivery of human interferon alfa-2a, (IFNα2a) a therapeutic protein gene under an ovalbumin promoter. The transfection efficiency of adherent COEC was estimated for up to 40% at a ratio of 6:1 of transfectant to pOVA5EIFN + GFP plasmid. Expression of IFNα2a was confirmed by western blotting in transformed COEC. In conclusion, the population of epithelial progenitor cells sourced from the distal oviduct can significantly contribute to in vitro culture of COEC, representing an efficient model to develop the production of avian bioreactors and other in vitro studies related to oviduct tissue.

Published
2016

49. Low-dose oral immunization with lyophilized tissue of herbicide-resistant lettuce expressing hepatitis B surface antigen for prototype plant-derived vaccine tablet formulation

Author

Anna Kostrzak, Piotr Bociąg, Halina Otta, Sławomir Samardakiewicz, Piotr Wójcik, Andrzej Plucienniczak, Michal R. Gdula, Olga Fedorowicz-Strońska, Bogdan Wolko, Tomasz Pniewski, Jacek Wojciechowicz, and Józef Kapusta

Subjects
Hepatitis B virus, medicine.medical_treatment, Lyophilized plant tissue, Transgenic lettuce, Dose-Response Relationship, Immunologic, Administration, Oral, Biology, S-HBsAg, medicine.disease_cause, Endoplasmic Reticulum, Anti-HBV oral vaccine, Feces, Mice, Oral immunization, Antigen, Plant Genetics • Original Paper, Immunity, medicine, Genetics, Animals, Humans, Hepatitis B Vaccines, Plant-based vaccines, Mice, Inbred BALB C, Hepatitis B Surface Antigens, Vaccines, Edible, Herbicides, Aminobutyrates, Vaccination, Kanamycin, General Medicine, Hepatitis B, Lettuce, medicine.disease, Plants, Genetically Modified, Virology, Recombinant Proteins, Immunity, Humoral, Plant Leaves, Freeze Drying, Immunization, Immunoglobulin A, Secretory, Adjuvant, medicine.drug, Herbicide Resistance
Abstract

Efficient immunization against hepatitis B virus (HBV) and other pathogens with plant-based oral vaccines requires appropriate plant expressors and the optimization of vaccine compositions and administration protocols. Previous immunization studies were mainly based on a combination of the injection of a small surface antigen of HBV (S-HBsAg) and the feeding with raw tissue containing the antigen, supplemented with an adjuvant, and coming from plants conferring resistance to kanamycin. The objective of this study was to develop a prototype oral vaccine formula suitable for human immunization. Herbicide-resistant lettuce was engineered, stably expressing through progeny generation micrograms of S-HBsAg per g of fresh weight and formed into virus-like particles (VLPs). Lyophilized tissue containing a relatively low, 100-ng VLP-assembled antigen dose, administered only orally to mice with a long, 60-day interval between prime and boost immunizations and without exogenous adjuvant, elicited mucosal and systemic humoral anti-HBs responses at the nominally protective level. Lyophilized tissue was converted into tablets, which preserved S-HBsAg content for at least one year of room temperature storage. The results of the study provide indications on immunization methodology using a durable, efficacious, and convenient plant-derived prototype oral vaccine against hepatitis B.

Published
2010

50. Nanogram Doses of Alum-Adjuvanted HBs Antigen Induce Humoral Immune Response in Mice When Orally Administered

Author

Tomasz Pniewski, Jacek Wojciechowicz, Józef Kapusta, Piotr Bociag, and Andrzej Plucienniczak

Subjects
HBsAg, Time Factors, Immunology, Administration, Oral, medicine.disease_cause, Injections, Intramuscular, Mice, Immune system, Adjuvants, Immunologic, Antigen, medicine, Animals, Immunology and Allergy, Hepatitis B Vaccines, Hepatitis B Antibodies, Antigen-presenting cell, Immunization Schedule, Hepatitis B virus, Mice, Inbred BALB C, Vaccines, Synthetic, Hepatitis B Surface Antigens, Dose-Response Relationship, Drug, business.industry, General Medicine, Hepatitis B, medicine.disease, Recombinant Proteins, Immunity, Humoral, Immunization, Alum Compounds, Female, business, Intramuscular injection
Abstract

Mucosal immunity elicited by plant-based and other orally administered vaccines can serve as the first line of defense against most pathogens infecting through mucosal surfaces, but it is also considered for systemic immunity against blood-borne diseases such as hepatitis B (HB). Previous oral immunization trials based on multiple administration of high doses of HBs antigen elicited an immune response; however, a reproducible and long-lasting immunization protocol was difficult to design. The objective of this study was to evaluate the effect of dose and timing of orally delivered alum-adsorbed antigen on the magnitude of the anti-HBs humoral response. Mice were immunized orally by gavage intubation or parenterally by intramuscular injection three times, once every 2 weeks, with doses of 5, 50, or 500 ng alum-adjuvanted HBsAg. A low dose (10 ng) of HBsAg was orally administered three times in different time intervals: 2, 4, 6, and 8 weeks. The three consecutive 5-ng oral doses of the antigen induced immune response at the protective level (>or=10 mIU/ml), significantly higher than the reaction elicited by three 50 or 500 ng doses. In contrast, intramuscular delivery of these doses did not differ significantly; however, they induced a five to six times higher immune response than oral immunization. The 8-week period between each of the three oral immunizations appeared to be favorable to the anti-HBs humoral responses compared with the shorter schedules. The results presented here clearly identify the importance of low doses of antigen administered orally in extended intervals for a significantly higher anti-HBs response. This finding provides some indications concerning the strategy of orally administered vaccines, including plant-based ones.

Published
2010

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