599 resultados para gfp
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Abstract Background Down syndrome is the most frequent genetic disorder in humans. Rare cases involving partial trisomy of chromosome 21 allowed a small chromosomal region common to all carriers, called Down Syndrome Critical Region (DSCR), to be determined. The DSCR1 gene was identified in this region and is expressed preferentially in the brain, heart and skeletal muscle. Recent studies have shown that DSCR1 belongs to a family of proteins that binds and inhibits calcineurin, a serine-threonine phosphatase. The work reported on herein consisted of a study of the subcellular location of DSCR1 and DSCR1-mutated forms by fusion with a green fluorescent protein, using various cell lines, including human. Results The protein's location was preferentially nuclear, independently of the isoform, cell line and insertion in the GFP's N- or C-terminal. A segment in the C-terminal, which is important in the location of the protein, was identified by deletion. On the other hand, site-directed mutational analyses have indicated the involvement of some serine and threonine residues in this event. Conclusion In this paper, we discuss the identification of amino acids which can be important for subcellular location of DSCR1. The involvement of residues that are prone to phosphorylation suggests that the location and function of DSCR1 may be regulated by kinases and/or phosphatases.
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Hek-293 cell line presents good production platform for recombinant therapeutic proteins, however little is known about the components that contribute to the cellular control of recombinant protein production. In this study, we generated a Hek-293 producing recombinant factor VIII (FVIII) and we evaluated the immunoglobulin-binding protein (BiP) and phytanoil-CoA α-hydroxylase (PAHX) expression levels which are known for diminishing FVIII production. Our analyses showed that the recombinant cell population expresses 3.1 ± 1.4 fold of BIP mRNA (P = 0.0054) and 97.8 ± 0.5 fold of PAHX mRNA (P = 0.0016) compared to nontransduced cells. The amount of these proteins was inversely correlated to the secreted FVIII. In conclusion, BIP and PAHX expression are augmented in human cells producing FVIII and they antagonize the amount of therapeutic factor VIII in the cell culture.
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Abstract Background Despite recent advances in the understanding of lignocellulolytic enzyme regulation, less is known about how different carbon sources are sensed and the signaling cascades that result in the adaptation of cellular metabolism and hydrolase secretion. Therefore, the role played by non-essential protein kinases (NPK) and phosphatases (NPP) in the sensing of carbon and/or energetic status was investigated in the model filamentous fungus Aspergillus nidulans. Results Eleven NPKs and seven NPPs were identified as being involved in cellulase, and in some cases also hemicellulase, production in A. nidulans. The regulation of CreA-mediated carbon catabolite repression (CCR) in the parental strain was determined by fluorescence microscopy, utilising a CreA: GFP fusion protein. The sensing of phosphorylated glucose, via the RAS signalling pathway induced CreA repression, while carbon starvation resulted in derepression. Growth on cellulose represented carbon starvation and derepressing conditions. The involvement of the identified NPKs in the regulation of cellulose-induced responses and CreA derepression was assessed by genome-wide transcriptomics (GEO accession 47810). CreA:GFP localisation and the restoration of endocellulase activity via the introduction of the ∆creA mutation, was assessed in the NPK-deficient backgrounds. The absence of either the schA or snfA kinase dramatically reduced cellulose-induced transcriptional responses, including the expression of hydrolytic enzymes and transporters. The mechanism by which these two NPKs controlled gene transcription was identified, as the NPK-deficient mutants were not able to unlock CreA-mediated carbon catabolite repression under derepressing conditions, such as carbon starvation or growth on cellulose. Conclusions Collectively, this study identified multiple kinases and phosphatases involved in the sensing of carbon and/or energetic status, while demonstrating the overlapping, synergistic roles of schA and snfA in the regulation of CreA derepression and hydrolytic enzyme production in A. nidulans. The importance of a carbon starvation-induced signal for CreA derepression, permitting transcriptional activator binding, appeared paramount for hydrolase secretion.
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Intravital imaging techniques are the best approach to investigate in situ cellular behavior under physiological conditions. Many techniques have emerged during these last few years for this purpose. We recently described an intravital imaging technique that allows for the observation of placenta physiological responses at the labyrinth layer of this tissue. This technique will be very useful to study many placental opportunistic infections and in this article we reinforce its usefulness by analyzing placental physiological entrapment of beads and parasites. In particular, our results show that small beads (1.0 μm) or Plasmodium chabaudi-GFP-infected-Red Blood Cells (Pc-GFP-iRBCs) cannot get trapped inside small or large blood vessels of popliteal lymph nodes (PLNs). Inside the placenta, clusters of beads could only be found inside the maternal blood vessels. However, Pc-GFP-iRBCs were found inside and outside the maternal blood vessels. We observed that trophoblasts can ingest infected-Red Blood Cells (iRBCs) in vitro and immunofluorescence of placenta revealed Pc-GFP-iRBCs inside and outside the maternal blood vessels. Taken together, we conclude that fast deposition of particles inside blood vessels seems to be an intrinsic characteristic of placenta blood flow, but iRBCs could be internalized by trophoblast cells. Thus these results represent one of the many possible uses of our intravital imaging technique to address important questions inside the parasitological field.
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A microorganism was isolated which could grow on unusually high concentrations of the toxic pollutant 4-chlorophenol. Taxonomic studies showed that the microorganism constituted a novel species within the genus Arthrobacter and it was named Arthrobacter chlorophenolicus A6. A. chlorophenolicus A6 was chromosomally tagged with either the gfp gene, encoding the green fluorescent protein (GFP), or the luc gene, encoding firefly luciferase. When the tagged cells were inoculated into 4-chlorophenol contaminated soil they could completely remove 175 µg/g 4-chlorophenol within 10 days, whereas no loss of 4-chlorophenol was observed in the uninoculated control microcosms. During these experiments the gfp and luc marker genes allowed monitoring of cell number and metabolic status. When A. chlorophenolicus A6 was grown on mixtures of phenolic compounds, the strain exhibited a preference for 4-nitrophenol over 4-chlorophenol, which in turn was preferred over phenol. Analysis of growth and degradation data indicated that the same enzyme system was used for removal of 4-chlorophenol and 4-nitrophenol. However, degradation of unbstituted phenol appeared to be mediated by another or an additional enzyme system. The luc-tagged A. chlorophenolicus A6 gave valuable information about growth, substrate depletion and toxicity of the phenolic compounds in substrate mixtures. The 4-chlorophenol degradation pathway in A. chlorophenolicus A6 was elucidated. The metabolic intermediate subject to ring cleavage was found to be hydroxyquinol and two different pathway branches led from 4-chlorophenol to hydroxyquinol. A gene cluster involved in 4-chlorophenol degradation was cloned from A. chlorophenolicus A6. The cluster contained two functional hydroxyquinol 1,2-dioxygenase genes and a number of other open reading frames presumed to encode enzymes involved in 4-chlorophenol catabolism. Analysis of the DNA sequence suggested that the gene cluster had partly been assembled by horizontal gene transfer. In summary, 4-chlorophenol degradation by A. chlorophenolicus A6 was studied from a number of angles. This organism has several interesting and useful traits such as the ability to degrade high concentrations of 4-chlorophenol and other phenols alone and in mixtures, an unusual and effective 4-chlorophenol degradation pathway and demonstrated ability to remove 4-chlorophenol from contaminated soil.
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Transcription is controlled by promoter-selective transcriptional factors (TFs), which bind to cis-regulatory enhancers elements, termed hormone response elements (HREs), in a specific subset of genes. Regulation by these factors involves either the recruitment of coactivators or corepressors and direct interaction with the basal transcriptional machinery (1). Hormone-activated nuclear receptors (NRs) are well characterized transcriptional factors (2) that bind to the promoters of their target genes and recruit primary and secondary coactivator proteins which possess many enzymatic activities required for gene expression (1,3,4). In the present study, using single-cell high-resolution fluorescent microscopy and high throughput microscopy (HTM) coupled to computational imaging analysis, we investigated transcriptional regulation controlled by the estrogen receptor alpha (ERalpha), in terms of large scale chromatin remodeling and interaction with the associated coactivator SRC-3 (Steroid Receptor Coactivator-3), a member of p160 family (28) primary coactivators. ERalpha is a steroid-dependent transcriptional factor (16) that belongs to the NRs superfamily (2,3) and, in response to the hormone 17-ß estradiol (E2), regulates transcription of distinct target genes involved in development, puberty, and homeostasis (8,16). ERalpha spends most of its lifetime in the nucleus and undergoes a rapid (within minutes) intranuclear redistribution following the addition of either agonist or antagonist (17,18,19). We designed a HeLa cell line (PRL-HeLa), engineered with a chromosomeintegrated reporter gene array (PRL-array) containing multicopy hormone response-binding elements for ERalpha that are derived from the physiological enhancer/promoter region of the prolactin gene. Following GFP-ER transfection of PRL-HeLa cells, we were able to observe in situ ligand dependent (i) recruitment to the array of the receptor and associated coregulators, (ii) chromatin remodeling, and (iii) direct transcriptional readout of the reporter gene. Addition of E2 causes a visible opening (decondensation) of the PRL-array, colocalization of RNA Polymerase II, and transcriptional readout of the reporter gene, detected by mRNA FISH. On the contrary, when cells were treated with an ERalpha antagonist (Tamoxifen or ICI), a dramatic condensation of the PRL-array was observed, displacement of RNA Polymerase II, and complete decreasing in the transcriptional FISH signal. All p160 family coactivators (28) colocalize with ERalpha at the PRL-array. Steroid Receptor Coactivator-3 (SRC-3/AIB1/ACTR/pCIP/RAC3/TRAM1) is a p160 family member and a known oncogenic protein (4,34). SRC-3 is regulated by a variety of posttranslational modifications, including methylation, phosphorylation, acetylation, ubiquitination and sumoylation (4,35). These events have been shown to be important for its interaction with other coactivator proteins and NRs and for its oncogenic potential (37,39). A number of extracellular signaling molecules, like steroid hormones, growth factors and cytokines, induce SRC-3 phosphorylation (40). These actions are mediated by a wide range of kinases, including extracellular-regulated kinase 1 and 2 (ERK1-2), c-Jun N-terminal kinase, p38 MAPK, and IkB kinases (IKKs) (41,42,43). Here, we report SRC-3 to be a nucleocytoplasmic shuttling protein, whose cellular localization is regulated by phosphorylation and interaction with ERalpha. Using a combination of high throughput and fluorescence microscopy, we show that both chemical inhibition (with U0126) and siRNA downregulation of the MAP/ERK1/2 kinase (MEK1/2) pathway induce a cytoplasmic shift in SRC-3 localization, whereas stimulation by EGF signaling enhances its nuclear localization by inducing phosphorylation at T24, S857, and S860, known partecipants in the regulation of SRC-3 activity (39). Accordingly, the cytoplasmic localization of a non-phosphorylatable SRC-3 mutant further supports these results. In the presence of ERalpha, U0126 also dramatically reduces: hormone-dependent colocalization of ERalpha and SRC-3 in the nucleus; formation of ER-SRC-3 coimmunoprecipitation complex in cell lysates; localization of SRC-3 at the ER-targeted prolactin promoter array (PRL-array) and transcriptional activity. Finally, we show that SRC-3 can also function as a cotransporter, facilitating the nuclear-cytoplasmic shuttling of estrogen receptor. While a wealth of studies have revealed the molecular functions of NRs and coregulators, there is a paucity of data on how these functions are spatiotemporally organized in the cellular context. Technically and conceptually, our findings have a new impact upon evaluating gene transcriptional control and mechanisms of action of gene regulators.
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Beet soil-borne mosaic virus (BSBMV) and Beet necrotic yellow vein virus (BNYVV) are members of Benyvirus genus. BSBMV has been reported only in the United States while BNYVV has a worldwide distribution. Both viruses are vectored by Polymyxa betae, possess similar host ranges, particles number and morphology. Both viruses are not serologically related but have similar genomic organizations. Field isolates consist of four RNA species but some BNYVV isolates contain a fifth RNA. RNAs 1 and 2 are essential for infection and replication while RNAs 3 and 4 play important roles on plant and vector interactions, respectively. Nucleotide and amino acid analyses revealed BSBMV and BNYVV are different enough to be classified in two different species. Additionally in BNYVV/BSBMV mixed infections, a competition was previous described in sugar beet, where BNYVV infection reduces BSBMV accumulation in both susceptible and resistant cultivars. Considering all this observations we hypothesized that BNYVV and BSBMV crossed study, exploiting their similarities and divergences, can improve investigation of molecular interactions between sugar beets and Benyviruses. The main achievement of our research is the production of a cDNA biologically active clones collection of BNYVV and BSBMV RNAs, from which synthetic copies of both Benyviruses can be transcribed. Moreover, through recombination experiments we demonstrated, for the first time, the BNYVV RNA 1 and 2 capability to trans-replicate and encapsidate BSBMV RNA 3 and 4, either the BSBMV RNA 1 and 2 capability to replicate BNYVV RNA2 in planta. We also demonstrated that BSBMV RNA3 support long-distance movement of BNYVV RNA 1 and 2 in B. macrocarpa and that 85 foreign sequence as p29HA, GFP and RFP, are successfully expressed, in C. quinoa, by BSBMV RNA3 based replicon (RepIII) also produced by our research. These results confirm the close correlation among the two viruses. Interestingly, the symptoms induced by BSBMV RNA-3 on C. quinoa leaves are more similar to necrotic local lesions caused by BNYVV RNA-5 p26 than to strongly chlorotic local lesions or yellow spot induced by BNYVV RNA- 3 encoded p25. As previous reported BSBMV p29 share 23% of amino acid sequence identity with BNYVV p25 but identity increase to 43% when compared with sequence of BNYVV RNA-5 p26. Based on our results the essential sequence (Core region) for the longdistance movement of BSBMV and BNYVV in B. macrocarpa, is not only carried by RNA3s species but other regions, perhaps located on the RNA 1 and 2, could play a fundamental role in this matter. Finally a chimeric RNA, composed by the 5’ region of RNA4 and 3’ region of RNA3 of BSBMV, has been produced after 21 serial mechanically inoculation of wild type BSBMV on C. quinoa plants. Chimera seems unable to express any protein, but it is replicated and transcript in planta. It could represent an important tool to study the interactions between Benyvirus and plant host. In conclusion different tools, comprising a method to study synthetic viruses under natural conditions of inoculum through P. Betae, have been produced and new knowledge are been acquired that will allow to perform future investigation of the molecular interactions between sugar beets and Benyviruses.
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The aim of the present study is understanding the properties of a new group of redox proteins having in common a DOMON-type domain with characteristics of cytochromes b. The superfamily of proteins containing a DOMON of this type includes a few protein families. With the aim of better characterizing this new protein family, the present work addresses both a CyDOM protein (a cytochrome b561) and a protein only comprised of DOMON(AIR12), both of plant origin. Apoplastic ascorbate can be regenerated from monodehydroascorbate by a trans-plasma membrane redox system which uses cytosolic ascorbate as a reductant and comprises a high potential cytochrome b. We identified the major plasma membrane (PM) ascorbate-reducible b-type cytochrome of bean (Phaseolus vulgaris) and soybean (Glycine max) hypocotyls as orthologs of Arabidopsis auxin-responsive gene air12. The protein, which is glycosylated and glycosylphosphatidylinositol-anchored to the external side of the PM in vivo, was expressed in Pichia pastoris in a recombinant form, lacking the glycosylphosphatidylinositol-modification signal, and purified from the culture medium. Recombinant AIR12 is a soluble protein predicted to fold into a β-sandwich domain and belonging to the DOMON superfamily. It is shown to be a b-type cytochrome with a symmetrical α-band at 561 nm, to be fully reduced by ascorbate and fully oxidized by monodehydroascorbate. Redox potentiometry suggests that AIR12 binds two high-potential hemes (Em,7 +135 and +236 mV). Phylogenetic analyses reveal that the auxin-responsive genes AIR12 constitute a new family of plasma membrane b-type cytochromes specific to flowering plants. Although AIR12 is one of the few redox proteins of the PM characterized to date, the role of AIR12 in trans-PM electron transfer would imply interaction with other partners which are still to be identified. Another part of the present project was aimed at understanding of a soybean protein comprised of a DOMON fused with a well-defined b561 cytochrome domain (CyDOM). Various bioinformatic approaches show this protein to be composed of an N-terminal DOMON followed by b561 domain. The latter contains five transmembrane helices featuring highly conserved histidines, which might bind haem groups. The CyDOM has been cloned and expressed in the yeast Pichia pastoris, and spectroscopic analyses have been accomplished on solubilized yeast membranes. CyDOM clearly reveal the properties of b-type cytochrome. The results highlight the fact that CyDOM is clearly able to lead an electron flux through the plasmamembrane. Voltage clamp experiments demonstrate that Xenopus laevis oocytes transformed with CyDOM of soybean exhibit negative electrical currents in presence of an external electron acceptor. Analogous investigations were carried out with SDR2, a CyDOM of Drosophila melanogaster which shows an electron transport capacity even higher than plant CyDOM. As quoted above, these data reinforce those obtained in plant CyDOM on the one hand, and on the other hand allow to attribute to SDR2-like proteins the properties assigned to CyDOM. Was expressed in Regenerated tobacco roots, transiently transformed with infected a with chimeral construct GFP: CyDOM (by A. rhizogenes infection) reveals a plasmamembrane localization of CyDOM both in epidermal cells of the elongation zone of roots and in root hairs. In conclusion. Although the data presented here await to be expanded and in part clarified, it is safe to say they open a new perspective about the role of this group of proteins. The biological relevance of the functional and physiological implications of DOMON redox domains seems noteworthy, and it can but increase with future advances in research. Beyond the very finding, however interesting in itself, of DOMON domains as extracellular cytochromes, the present study testifies to the fact that cytochrome proteins containing DOMON domains of the type of “CyDOM” can transfer electrons through membranes and may represent the most important redox component of the plasmamembrane as yet discovered.
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Introduction Phospholipase Cb1 (PLC-β1) is a key player in the regulation of nuclear inositol lipid signaling and of a wide range of cellular functions, such as proliferation and differentiation (1,2,3). PLCb1 signaling depends on the cleavage of phosphatidylinositol 4,5-bisphosphate and the formation of the second messengers diacylglycerol and Inositol tris-phosphate which activate canonical protein kinase C (cPKC) isoforms. Here we describe a proteomic approach to find out a potential effector of nuclear PLC-b1 dependent signaling during insulin stimulated myogenic differentiation. Methods Nuclear lysates obtained from insulin induced C2C12 myoblasts were immunoprecipitated with anti-phospho-substrate cPKC antibody. Proteins, stained with Comassie blue, were excised, digested and subsequently analysed in LC-MS/MS. For peptide sequence searching, the mass spectra were processed and analyzed using the Mascot MS/MS ion search program with the NCBI database. Western blotting, GST-pull down and co-immunoprecipitation were performed to study the interaction between eEF1A2 and cPKCs. Site direct mutagenesis was performed to confirm the phosphorylated motif recognized by the antibody. Immunofluorescence analysis, GFP-tagged eEF1A2 vector and subcellular fractionation were performed to study nuclear localization and relative distribution of eEF1A2. Results We have previously shown that PLC-β1 is greatly increased at the nuclear level during insulin-induced myoblasts differentiation and that this nuclear localization is essential for induction of differentiation. Thus, nuclear proteins of insulin stimulated C2C12 myoblasts, were immunoprecipitated with an anti-phospho-substrate cPKC antibody. After Electrophoretic gel separation of proteins immunoprecipitated, several molecules were identified by LC-MS/MS. Among these most relevant and unexpected was eukaryotic elongation factor 1 alpha 2 (eEF1A2). We found that eEF1A2 is phosphorylated by PKCb1 and that these two molecules coimmunolocalized at the nucleolar level. eEF1A2 could be phosphorylated in many sites among which both threonine and serine residues. By site direct mutagenesis we demonstrated that it is the serine residue of the motif recognized by the antibody that is specifically phosphorylated by PKCb1. The silencing of PLCb1 gives rise to a reduction of expression and phosphorylation levels of eEF1A2 indicating this molecule as a target of nuclear PLCb1 regulatory network during myoblasts differentiation.
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ZusammenfassungNierenzellkarzinome (NZK) sind häufig gekennzeichnet durch den Funktionsverlust des von Hippel-Lindau Tumorsuppressorgens (VHL TSG). Man kennt heute eine Reihe potentieller Kandidatengene, die eventuell in Wechselwirkung mit dem VHL-Genprodukt stehen (VEGF, c-fos, c-myc). Zur Aufklärung der molekularen Vorgänge, die zur Pathogenese der gut vaskularisierten Nierenzellkarzinome beitragen, wurden NZK-Zellinien untersucht. Vektorkonstrukte wurden generiert, um das in vitro und in vivo Wachstumsverhalten vor und nach Transfektion zu beobachten. Mit Hilfe eines GFP-Fusionsproteins wurden zusätzlich Hinweise auf die intrazelluläre Lokalisation des VHL-Genproduktes (pVHL) geliefert. Nach Abschluß der vorliegenden Studien zeigte sich eine direkte Abhängigkeit der beiden Gene VHL und VEGF. Sowohl die in vitro als auch die in vivo Ansätze bewiesen eine Interaktion der beiden Gene. Die Frage nach einer Interaktion von pVHL mit den Genprodukten Fos und Myc läßt sich jedoch nicht eindeutig beantworten. Die Expressionsveränderungen dieser Gene erfolgten scheinbar willkürlich, eine Interaktion konnte nicht bestätigt werden.Die Lokalisation des VHL-Genproduktes ist von Fall zu Fall unterschiedlich, ein Zusammenhang mit den verschiedenen Funktionen des VHL-Gens ist demnach wahrscheinlich. Zusammenfassend läßt sich sagen, daß das VHL TSG eine Rolle bei der Kontrolle der Angiogenese spielt, eine Interaktion mit VEGF ist mehr als wahrscheinlich. Zukünftig sind bei der Aufklärung des Pathomechanismus von Nierenzellkarzinomen deshalb vor allem Studien nötig, die dem VHL TSG als Angiogeneseinhibitor eine zentrale Bedeutung bei der Heilung sporadischer Tumoren mit starker Vaskularisierung zukommen lassen.
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Im Rahmen dieser Arbeit wurden Pseudovirionen mit gfp als Reportergen generiert und zur Charakterisierung verschiedener Aspekte der HPV-Infektion verwendet. Es konnte gezeigt werden, daß Heparansulfatproteoglykane für die Infektion mit HPV16- und HPV33-Pseudovirionen essentiell sind, da: (i) Heparin, nicht aber Chondroitin- oder Dermatansulfat die Infektion inhibiert, (ii) Heparinase I oder chloratbehandelte Zellen vollständig bzw. teilweise resistent gegen eine Infektion sind, (iii) monoklonale Antikörper Pseudovirionen neutralisieren, indem sie die Bindung an Heparin verhindern. Ein intakter C-Terminus des L1-Proteins ist für die Heparinbindung nicht notwendig. Alpha-6 Integrin ist kein obligater HPV-Rezeptor. Die Neutralisation gebundener Pseudovirionen durch ein neutralisierendes Antiserum einerseits und durch Heparin andererseits demonstriert, daß die Aufnahme von Pseudovirionen sehr langsam verläuft und daß die Bindung von einem heparinsensitiven zu einem heparinresistenten Zustand übergeht, möglicherweise unter Beteiligung weiterer Rezeptoren. Die Wirkung von verschiedenen Inhibitoren auf die Pseudoinfektion lassen schließen, daß Pseudovirionen über eine mikrofilamentabhängige und energieabhängige Endozytose mit anschließender Penetration durch saure Vesikel aufgenommen werden. Caveolen sind an der Aufnahme nicht beteiligt. Untersuchungen zur Neutralisation von HPV16-, HPV18- und HPV33-Pseudovirionen durch Antiseren gegen HPV16, 18, 31, 33, 35, 39 und 45 zeigen eine Kreuzneutralisation zwischen HPV31 und HPV33 einerseits und zwischen HPV18 und HPV45 andererseits.
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Im Rahmen dieser Arbeit wurden transgene Mausmodelle hergestellt, die eine weitere Aufklärung der Rolle des Transkriptionsfaktors Pax6 bei der Wanderung von Nervenzellen ermöglichen, sowie ein Kultursystem zur Darstellung embryonaler Wanderungen außerhalb des Mutterleibs entwickelt.Bei der YAC-transgenen Mäuselinie PhPax6-taulacZ wird das Reportergen taulacZ unter der Kontrolle des Pax6-Promotors exprimiert. Dadurch ist dort, wo Pax6 im Zellkern vorliegt, der Rest der Zelle über seine gesamte Ausdehnung mit der vom taulacZ-Transgen kodierten tau-b-Galactosidase markiert. Das räumlich-zeitliche Expressionsmuster von Pax6 und dem Transgen taulacZ wurde detailliert untersucht. Dabei wurde eine hohe Übereinstimmung festgestellt. Basierend auf der Darstellung der Zellen in ihrer gesamten Ausdehnung, die durch das taulacZ-Transgen erstmals möglich ist, wurde eine Klassifizierung Pax6-positiver Zelltypen vorgenommen. Zunächst wird Pax6 in Neuroepithelzellen, später in radialen Gliazellen exprimiert.Mit der zweiten transgenen Mäuselinie, PhPax6-tTA, wurde ein Werkzeug hergestellt, das die gezielte und hoch spezifische Expression von beliebigen Transgenen in Pax6-exprimierenden Zellen ermöglicht. In Pax6-positive Zellen der Medulla wurde das Grün Fluoreszierende Protein (GFP) eingeführt und das Wanderungsverhalten in vitro über mehrere Tage dargestellt. Erstmals können mit dieser Linie beliebige Expressionskonstrukte gezielt, hocheffizient und schnell in wandernde Neurone eingebracht werden, ohne störende Hinter-grundexpression in anderen Zellen.
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Le moderne tecniche di imaging e i recenti sviluppi nel campo della visione computazionale consentono sempre più diffusamente l'utilizzo di metodi di image analysis, specialmente in ambito medico e biologico, permettendo un maggiore supporto sia alla diagnosi, sia alla ricerca. Il lavoro svolto in questa tesi si pone in un contesto di ricerca di carattere interdisciplinare, e riguarda il progetto e la realizzazione di un‘interfaccia grafica per l'analisi di colture batteriche geneticamente modificate, marcate con proteine fluorescenti (GFP), acquisite tramite un microscopio ad epifluorescenza. Nota la funzione di risposta del sistema di acquisizione delle immagini, l'analisi quantitativa delle colture batteriche è effettuata mediante la misurazione di proprietà legate all'intensità della risposta al marcatore fluorescente. L'interfaccia consente un'analisi sia globale dei batteri individuati nell'immagine, sia di singoli gruppi di batteri selezionati dall'utente, fornendo utili informazioni statistiche, sia in forma grafica che numerica. Per la realizzazione dell'interfaccia sono state adottate tecniche di ingegneria del software, con particolare enfasi alla interazione uomo-macchina e seguendo criteri di usability, al fine di consentire un corretto utilizzo dello strumento anche da parte di personale senza conoscenza in campo informatico.
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Die Kapsidproteine L1 und L2 von humanen Papillomviren (HPV) werden im Cytoplasma infizierter Keratinocyten synthetisiert und gelangen unabhängig voneinander in den Kern (Florin et al. 2002b). L2 lokalisiert in speziellen Kerndomänen, sog. ND10, und induziert die Reorganisation dieser Kernstrukturen: L2-abhängig akkumuliert der transkriptionelle Modulator Daxx verstärkt in ND10 und außerdem kommt es zum Ausschluss des transkriptionellen Aktivators Sp100 aus diesen Domänen (Florin et al. 2002a). Im Anschluss an diese Umorganisation im Kern induziert L2 die Lokalisation des Kapsidproteins L1 in ND10 (Florin et al. 2002b). Da auch die Replikation und Transkription von Papillomviren in oder in unmittelbarer Nähe von ND10 stattfinden, werden ND10 als Orte der Papillomvirus-Morphogenese diskutiert (Swindle et al. 1999). Innerhalb dieser Arbeit konnte gezeigt werden, dass L1 und L2 im Cytoplasma der Zellen mit Chaperonen interagieren, und dass der Kerntransport von L2 von der L2/Hsc70-Assoziation abhängig ist. Hsc70, das mit dem C-Terminus von L2 assoziiert ist, wird in virusähnliche Partikel (VLPs) eingebaut. Erst durch die Verpackung von DNA in die Kapside kommt es zum Ausschluss von Hsc70 aus dem Papillomvirus-Kapsid. Ergebnisse dieser Arbeit lassen zudem vermuten, dass L2 über seinen C-Terminus mit Mikrotubuli interagieren kann, falls diese Aminosäure-Region in L2 nicht durch das Chaperon maskiert wird. Mit Hilfe dieser Erkenntnisse wurde eine Modellvorstellung für die Rolle von L2 während der Infektion und der Morphogenese von HPV entwickelt. Die ND10-Lokalisationsdomäne (NDLD) in L2 konnte wie bei keinem Protein zuvor auf eine sehr kurze Sequenz von 22 Aminosäuren eingeengt werden. Welcher Mechanismus für die ND10-Lokalisation verantwortlich ist, muss dagegen noch geklärt werden. Alle L2-Mutanten, die ND10-Lokalisation zeigen, induzieren auch die Reorganisation dieser Domänen. Dies spricht dafür, dass L2 direkt in ND10 die Veränderungen hervorruft und wahrscheinlich keine zusätzlichen Domänen in L2 daran beteiligt sind. Es konnten zwei L1-Interaktionsdomänen in L2 kartiert werden. Diese beiden Regionen in L2 konnten nicht genauer lokalisiert werden und umfassen möglicherweise mehrere L1-Interaktionsdomänen. Der Einbau von L2 in die Kapside kann nur im Kern infizierter Zellen stattfinden. Hierfür ist die Lokalisation der Kapsidproteine in ND10 nicht notwendig. Weiterführende Versuche müssen jedoch noch klären, inwieweit ND10 trotzdem unerlässlich für eine produktive Morphogenese sind. Zudem wurde klar, dass die ersten 150 Aminosäuren im L2-Protein für das L1/L2-Verhältnis in Kapsiden verantwortlich sind. In Virionen beträgt dieses Verhältnis 30:1, d. h. zwölf L2-Moleküle werden in die Partikel aus 360 L1-Molekülen eingebaut. Bei der Verwendung der Deletionsmutante L2-150/467 beträgt dieses Verhältnis 5:1. Weitere Analysen, welche Regionen von L1 und L2 miteinander interagieren und wodurch die Beschränkung des L1/L2-Verhältnisses in Papillomviren zustande kommt, können genauere Einblicke in den Aufbau der Kapside und speziell die Lage von L2 im Kapsid liefern.
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Nicht-umhüllte humane Papillomviren binden an Heparansulfatproteoglykane (HSPG) der Zelloberfläche und werden durch Endocytose in Zielzellen aufgenommen. Um eine effiziente Infektion zu etablieren, muss die virale DNA in den Zellkern transportiert werden. Auf welche Art und Weise hierbei die Endosomenmembran überwunden wird, war bislang völlig unklar. Die Suche nach potentiellen membrandestabilisierenden Eigenschaften der Kapsidproteine L1 und L2 von HPV führte im Vorfeld der vorliegenden Dissertation zur Identifizierung eines carboxyterminalen Peptids des minoren L2-Proteins, welches als sehr mikrobizid und fungizid beschrieben werden konnte. Es ist gekennzeichnet durch einen Bereich basischer und einen Bereich hydrophober Aminosäuren. Da das minore L2-Protein für den Infektionsprozess von Papillomviren essentiell ist, wurde im Rahmen dieser Arbeit die Rolle des C-terminalen Peptids für den Transport des infektiösen Materials durch die zelluläre Membranbarriere genauer untersucht. Es konnte gezeigt werden, dass das carboxyterminale L2-Peptid von HPV33 nach externer Zugabe eine cytotoxische Wirkung auf höhere eukaryotische Zellen hat. Es lokalisiert an zellulären Membranen und induziert eine pH-abhängige Reduktion des ATP-Gehalts von Säugerzellen. Weiter wurde nachgewiesen, dass das Peptid die Cytoplasmamembran permeabilisieren und für kleine, hydrophile Substanzen wie Propidiumjodid durchlässig machen kann. Mutationen innerhalb des Peptids verdeutlichten die Notwendigkeit beider Bereiche, basischer und hydrophober Aminosäuren, für den membrandestabilisierenden Effekt. Im Folgenden wurde die intrazelluläre Aktivität des L2-Peptids mit Hilfe von GFP2-Peptid-Fusionen analysiert. Das Peptid ist in der Lage, eine Integration des globulären GFP-Dimers in Membranen zu vermitteln, was bei einem hohen Prozentsatz der exprimierenden Zellen zum Absterben führt. Auch wt 33L2 weist im Gegensatz zu C-terminalen Deletions- und Punktmutanten die Fähigkeit zur Membranassoziation auf. Abschließend wurde der Effekt von Mutationen innerhalb dieses L2-Peptids auf die Infektiösität von L1/L2-Pseudovirionen beschrieben. Die Mutationen haben keinen Einfluss auf den Einbau des L2-Proteins in die Pseudovirionen und auf die DNA-Verpackung. Die Virusmorphogenese ist somit nicht negativ beeinträchtigt. Die Infektiösität der HPV33- wie auch von HPV16-Pseudovirionen mit C-terminal mutiertem L2-Protein ist jedoch auf das Niveau von solchen reduziert, die nur aus dem majoren L1 bestehen und geht gegen Null. Zusammenfassend kann man festhalten, dass das minore Kapsidprotein L2 von HPV am Carboxyterminus eine membrandestabilisierende Aktivität besitzt, welche unter Papillomviren konserviert und für eine effektive Infektion essentiell ist.
