Your search keyword '"Hafner-Bratkovic I"' showing total 9 results

1. The POM monoclonals: a comprehensive set of antibodies to non-overlapping prion protein epitopes

Author

Polymenidou, M, Moos, R, Scott, M, Sigurdson, C, Shi, Y Z, Yajima, B, Hafner-Bratkovic, I, Jerala, R, Hornemann, S, Wuthrich, K, Bellon, A, Vey, M, Garen, G, James, M N G, Kav, N, Aguzzi, A; https://orcid.org/0000-0002-0344-6708, Polymenidou, M, Moos, R, Scott, M, Sigurdson, C, Shi, Y Z, Yajima, B, Hafner-Bratkovic, I, Jerala, R, Hornemann, S, Wuthrich, K, Bellon, A, Vey, M, Garen, G, James, M N G, Kav, N, and Aguzzi, A; https://orcid.org/0000-0002-0344-6708

Abstract

PrP(Sc), a misfolded and aggregated form of the cellular prion protein PrP(C), is the only defined constituent of the transmissible agent causing prion diseases. Expression of PrP(C) in the host organism is necessary for prion replication and for prion neurotoxicity. Understanding prion diseases necessitates detailed structural insights into PrP(C) and PrP(Sc). Towards this goal, we have developed a comprehensive collection of monoclonal antibodies denoted POM1 to POM19 and directed against many different epitopes of mouse PrP(C). Three epitopes are located within the N-terminal octarepeat region, one is situated within the central unstructured region, and four epitopes are discontinuous within the globular C-proximal domain of PrP(C). Some of these antibodies recognize epitopes that are resilient to protease digestion in PrP(Sc). Other antibodies immunoprecipitate PrP(C), but not PrP(Sc). A third group was found to immunoprecipitate both PrP isoforms. Some of the latter antibodies could be blocked with epitope-mimicking peptides, and incubation with an excess of these peptides allowed for immunochromatography of PrP(C) and PrP(Sc). Amino-proximal antibodies were found to react with repetitive PrP(C) epitopes, thereby vastly increasing their avidity. We have also created functional single-chain miniantibodies from selected POMs, which retained the binding characteristics despite their low molecular mass. The POM collection, thus, represents a unique set of reagents allowing for studies with a variety of techniques, including western blotting, ELISA, immunoprecipitation, conformation-dependent immunoassays, and plasmon surface plasmon resonance-based assays.

Published

2008

2. The complete genome sequence of a Crimean-Congo Hemorrhagic Fever virus isolated from an endemic region in Kosovo

Author

Dedushaj Iusuf, Petrovec Miroslav, Hafner-Bratkovič Iva, Saksida Ana, Khristova Marina L, Nichol Stuart T, Duh Darja, Ahmeti Salih, and Avšič-Županc Tatjana

Subjects

Infectious and parasitic diseases, RC109-216

Abstract

Abstract The Balkan region and Kosovo in particular, is a well-known Crimean-Congo hemorrhagic fever (CCHF) endemic region, with frequent epidemic outbreaks and sporadic cases occurring with a hospitalized case fatality of approximately 30%. Recent analysis of complete genome sequences of diverse CCHF virus strains showed that the genome plasticity of the virus is surprisingly high for an arthropod-borne virus. High levels of nucleotide and amino acid differences, frequent RNA segment reassortment and even RNA recombination have been recently described. This diversity illustrates the need to determine the complete genome sequence of CCHF virus representatives of all geographically distinct endemic areas, particularly in light of the high pathogenicity of the virus and its listing as a potential bioterrorism threat. Here we describe the first complete CCHF virus genome sequence of a virus (strain Kosova Hoti) isolated from a hemorrhagic fever case in the Balkans. This virus strain was isolated from a fatal CCHF case, and passaged only twice on Vero E6 cells prior to sequence analysis. The virus total genome was found to be 19.2 kb in length, consisting of a 1672 nucleotide (nt) S segment, a 5364 nt M segment and a 12150 nt L segment. Phylogenetic analysis of CCHF virus complete genomes placed the Kosova Hoti strain in the Europe/Turkey group, with highest similarity seen with Russian isolates. The virus M segments are the most diverse with up to 31 and 27% differences seen at the nt and amino acid levels, and even 1.9% amino acid difference found between the Kosova Hoti and another strain from Kosovo (9553-01). This suggests that distinct virus strains can coexist in highly endemic areas.

Published

2008

3. Globular domain of the prion protein needs to be unlocked by domain swapping to support prion protein conversion.

Author

Hafner-Bratkovic I, Bester R, Pristovsek P, Gaedtke L, Veranic P, Gaspersic J, Mancek-Keber M, Avbelj M, Polymenidou M, Julius C, Aguzzi A, Vorberg I, and Jerala R

Subjects

Animals, Cell Line, Circular Dichroism, Disulfides chemical synthesis, Disulfides metabolism, Enzyme-Linked Immunosorbent Assay, Flow Cytometry, Mice, Microscopy, Atomic Force, Microscopy, Electron, Transmission, Mutation, Prions genetics, Prions ultrastructure, Prions chemistry, Prions metabolism

Abstract

Prion diseases are fatal transmissible neurodegenerative diseases affecting many mammalian species. The normal prion protein (PrP) converts into a pathological aggregated form, PrPSc, which is enriched in the β-sheet structure. Although the high resolution structure of the normal PrP was determined, the structure of the converted form of PrP remains inaccessible to high resolution techniques. To map the PrP conversion process we introduced disulfide bridges into different positions within the globular domain of PrP, tethering selected secondary structure elements. The majority of tethered PrP mutants exhibited increased thermodynamic stability, nevertheless, they converted efficiently. Only the disulfides that tether subdomain B1-H1-B2 to subdomain H2-H3 prevented PrP conversion in vitro and in prion-infected cell cultures. Reduction of disulfides recovered the ability of these mutants to convert, demonstrating that the separation of subdomains is an essential step in conversion. Formation of disulfide-linked proteinase K-resistant dimers in fibrils composed of a pair of single cysteine mutants supports the model based on domain-swapped dimers as the building blocks of prion fibrils. In contrast to previously proposed structural models of PrPSc suggesting conversion of large secondary structural segments, we provide evidence for the conservation of secondary structural elements of the globular domain upon PrP conversion. Previous studies already showed that dimerization is the rate-limiting step in PrP conversion. We show that separation and swapping of subdomains of the globular domain is necessary for conversion. Therefore, we propose that the domain-swapped dimer of PrP precedes amyloid formation and represents a potential target for therapeutic intervention.

Published

2011

4. Tetracysteine-tagged prion protein allows discrimination between the native and converted forms.

Author

Gaspersic J, Hafner-Bratkovic I, Stephan M, Veranic P, Bencina M, Vorberg I, and Jerala R

Subjects

Animals, Cell Line, Mice, Microscopy, Electron, Transmission, Prions chemistry, Prions metabolism, Prions ultrastructure, Protein Folding, Protein Stability, Protein Structure, Secondary, Temperature, Tetracycline metabolism, Circular Dichroism methods, Prions analysis, Spectrometry, Fluorescence methods, Tetracycline chemistry

Abstract

The conformational conversion of prion protein (PrP) from a native conformation to the amyloid form is a hallmark of transmissible spongiform encephalopathies. Conversion is usually monitored by fluorescent dyes, which bind generic amyloids and are less suited for living cell imaging. We report a new method for the synthesis of membrane-permeable and membrane-impermeable biarsenical reagents, which are then used to monitor murine PrP (mPrP) misfolding. We introduced tetracysteine (TC) tags into three different positions of mPrP, which folded into a native-like structure. Whereas mPrPs with a TC tag inserted at the N-terminus or C-terminus supported fibril formation, insertion into the helix 2-helix 3 loop inhibited conversion. We devised a quantitative protease-free method to determine the fraction of converted PrP, based on the ability of the fluorescein arsenical helix binder reagent to differentiate between the monomeric and fibrilized form of TC-tagged PrP, and showed that TC-tagged mPrP could be detected on transfected cells, thereby expanding the potential use of this method for the detection and study of conformational diseases.

Published

2010

5. Expression, purification and structural studies of a short antimicrobial peptide.

Author

Zorko M, Japelj B, Hafner-Bratkovic I, and Jerala R

Subjects

Amino Acid Sequence, Animals, Anti-Bacterial Agents isolation & purification, Calorimetry, Cell Line, Chromatography, High Pressure Liquid, Escherichia coli genetics, Escherichia coli metabolism, Lipids chemistry, Mass Spectrometry, Mice, Micelles, Models, Molecular, Peptides genetics, Peptides isolation & purification, Protein Structure, Tertiary, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Spectrophotometry, Anti-Bacterial Agents chemistry, Anti-Bacterial Agents metabolism, Gene Expression, Peptides chemistry, Peptides metabolism

Abstract

We have produced a small antimicrobial peptide PFWRIRIRR in bacteria utilizing production in the form of insoluble fusion protein with ketosteroid isomerase. The recombinant peptide was rapidly and efficiently isolated by acidic cleavage of the fusion protein based on the acid labile Asp-Pro bond at the N-terminus of the peptide. The peptide has antibacterial activity and neutralizes macrophage activation by LPS. The selectivity of the peptide against bacteria correlates with preferential binding to acidic phospholipid vesicles. Solution structure of the peptide in SDS and DPC micelles was determined by NMR. The peptide adopts a well-defined structure, comprising a short helical segment. Cationic and hydrophobic clusters are segregated along the molecular axis of the short helix, which is positioned perpendicular to the membrane plane. The position of the helix is shifted in two micellar types and more nonpolar surface is exposed in anionic micelles. Overall structure explains the advantageous role of the N-terminal proline residue, which forms an integral part of the hydrophobic cluster.

Published

2009

6. Curcumin binds to the alpha-helical intermediate and to the amyloid form of prion protein - a new mechanism for the inhibition of PrP(Sc) accumulation.

Author

Hafner-Bratkovic I, Gaspersic J, Smid LM, Bresjanac M, and Jerala R

Subjects

Amyloid metabolism, Binding, Competitive, Cerebellum metabolism, Cerebellum pathology, Circular Dichroism, Creutzfeldt-Jakob Syndrome pathology, Curcumin chemistry, Curcumin metabolism, Drug Design, Humans, In Vitro Techniques, PrPSc Proteins chemistry, Protein Structure, Secondary, Stereoisomerism, Creutzfeldt-Jakob Syndrome drug therapy, Creutzfeldt-Jakob Syndrome metabolism, Curcumin pharmacology, PrPSc Proteins metabolism

Abstract

Conversion of the native, predominantly alpha-helical conformation of prion protein (PrP) into the beta-stranded conformation is characteristic for the transmissible spongiform encephalopathies such as Creutzfeld-Jakob disease. Curcumin, an extended planar molecule and a dietary polyphenol, inhibits in vitro conversion of PrP and formation of protease resistant PrP in neuroblastoma cell lines. Curcumin recognizes the converted beta-form of the PrP both as oligomers and fibrils but not the native form. Curcumin binds to the prion fibrils in the left-handed chiral arrangement as determined by circular dichroism. We show that curcumin labels the plaques of the brain sections of variant Creutzfeld-Jakob disease cases and stains the same structures as antibodies against the PrP. In contrast to thioflavin T, curcumin also binds to the alpha-helical intermediate of PrP present at acidic pH at stoichiometry of 1 : 1. Congo red competes with curcumin for binding to the alpha-intermediate as well as to the beta-form of PrP but is toxic and binds also to the native form of PrP. We therefore show that the partially unfolded structural intermediate of the PrP can be targeted by non-toxic compound of natural origin.

Published

2008

7. The complete genome sequence of a Crimean-Congo hemorrhagic fever virus isolated from an endemic region in Kosovo.

Author

Duh D, Nichol ST, Khristova ML, Saksida A, Hafner-Bratkovic I, Petrovec M, Dedushaj I, Ahmeti S, and Avsic-Zupanc T

Subjects

Animals, Chlorocebus aethiops, Europe, Female, Hemorrhagic Fever Virus, Crimean-Congo classification, Humans, Phylogeny, Recombination, Genetic, Sequence Homology, Serial Passage, Vero Cells, Yugoslavia epidemiology, Disease Outbreaks, Genome, Viral, Hemorrhagic Fever Virus, Crimean-Congo genetics, Hemorrhagic Fever, Crimean epidemiology, Hemorrhagic Fever, Crimean virology

Abstract

The Balkan region and Kosovo in particular, is a well-known Crimean-Congo hemorrhagic fever (CCHF) endemic region, with frequent epidemic outbreaks and sporadic cases occurring with a hospitalized case fatality of approximately 30%. Recent analysis of complete genome sequences of diverse CCHF virus strains showed that the genome plasticity of the virus is surprisingly high for an arthropod-borne virus. High levels of nucleotide and amino acid differences, frequent RNA segment reassortment and even RNA recombination have been recently described. This diversity illustrates the need to determine the complete genome sequence of CCHF virus representatives of all geographically distinct endemic areas, particularly in light of the high pathogenicity of the virus and its listing as a potential bioterrorism threat. Here we describe the first complete CCHF virus genome sequence of a virus (strain Kosova Hoti) isolated from a hemorrhagic fever case in the Balkans. This virus strain was isolated from a fatal CCHF case, and passaged only twice on Vero E6 cells prior to sequence analysis. The virus total genome was found to be 19.2 kb in length, consisting of a 1672 nucleotide (nt) S segment, a 5364 nt M segment and a 12150 nt L segment. Phylogenetic analysis of CCHF virus complete genomes placed the Kosova Hoti strain in the Europe/Turkey group, with highest similarity seen with Russian isolates. The virus M segments are the most diverse with up to 31 and 27% differences seen at the nt and amino acid levels, and even 1.9% amino acid difference found between the Kosova Hoti and another strain from Kosovo (9553-01). This suggests that distinct virus strains can coexist in highly endemic areas.

Published

2008

8. The POM monoclonals: a comprehensive set of antibodies to non-overlapping prion protein epitopes.

Author

Polymenidou M, Moos R, Scott M, Sigurdson C, Shi YZ, Yajima B, Hafner-Bratkovic I, Jerala R, Hornemann S, Wuthrich K, Bellon A, Vey M, Garen G, James MN, Kav N, and Aguzzi A

Subjects

Animals, Antibody Affinity, Blotting, Western, Cross Reactions, Epitope Mapping, Flow Cytometry, Humans, Immunoglobulin Isotypes immunology, Immunoglobulin Variable Region isolation & purification, Immunohistochemistry, Immunoprecipitation, Mice, Peptide Mapping, Surface Plasmon Resonance, Antibodies, Monoclonal biosynthesis, Epitopes immunology, Prions immunology

Abstract

PrP(Sc), a misfolded and aggregated form of the cellular prion protein PrP(C), is the only defined constituent of the transmissible agent causing prion diseases. Expression of PrP(C) in the host organism is necessary for prion replication and for prion neurotoxicity. Understanding prion diseases necessitates detailed structural insights into PrP(C) and PrP(Sc). Towards this goal, we have developed a comprehensive collection of monoclonal antibodies denoted POM1 to POM19 and directed against many different epitopes of mouse PrP(C). Three epitopes are located within the N-terminal octarepeat region, one is situated within the central unstructured region, and four epitopes are discontinuous within the globular C-proximal domain of PrP(C). Some of these antibodies recognize epitopes that are resilient to protease digestion in PrP(Sc). Other antibodies immunoprecipitate PrP(C), but not PrP(Sc). A third group was found to immunoprecipitate both PrP isoforms. Some of the latter antibodies could be blocked with epitope-mimicking peptides, and incubation with an excess of these peptides allowed for immunochromatography of PrP(C) and PrP(Sc). Amino-proximal antibodies were found to react with repetitive PrP(C) epitopes, thereby vastly increasing their avidity. We have also created functional single-chain miniantibodies from selected POMs, which retained the binding characteristics despite their low molecular mass. The POM collection, thus, represents a unique set of reagents allowing for studies with a variety of techniques, including western blotting, ELISA, immunoprecipitation, conformation-dependent immunoassays, and plasmon surface plasmon resonance-based assays.

Published

2008

9. Identification of an epitope on the recombinant bovine PrP that is able to elicit a prominent immune response in wild-type mice.

Author

Cernilec M, Vranac T, Hafner-Bratkovic I, Koren S, Venturini AC, Popović M, Juntes P, and Serbec VC

Subjects

Amino Acid Sequence, Animals, Cattle, Cells, Cultured, Cricetinae, Deer, Encephalopathy, Bovine Spongiform diagnosis, Encephalopathy, Bovine Spongiform immunology, Epitopes genetics, Humans, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Prions administration & dosage, Prions genetics, Rabbits, Rats, Recombinant Proteins administration & dosage, Recombinant Proteins genetics, Sheep, Swine, Epitopes immunology, Prions immunology, Recombinant Proteins immunology

Abstract

The main cause for the development of transmissible spongiform encephalopathies (TSE) is the conformational change of prion protein from the normal cellular isoform (PrP(C)) into the abnormal isoform, named prion (PrP(Sc)). The two isoforms have the same primary structure, and with PrP being highly conserved among different species, no immune response to PrP(Sc) has been observed in infected humans or other mammals so far. The problem of inducing immune response was encountered when producing monoclonal antibodies against PrP, therefore mice lacking a functional Prnp gene were predominantly used for the immunization. In the present paper we report that by immunizing wild-type BALB/c mice with chemically unmodified recombinant bovine PrP a potent humoral immune response was achieved. Furthermore, we were able to isolate the monoclonal antibody (mAb) E12/2 and few other mAbs, all reacting specifically with bovine and human PrP, but not with PrP from several other mammals. The epitope of mAb E12/2 is located at the C-terminal end of helix 1, with His155 being crucial for binding. It has been proven that mAb E12/2 is useful for human and bovine TSE research as well as for diagnostics. Our results show that there are sufficient structural differences between mouse and bovine PrP to provoke a prominent humoral immune response.

Published

2007