L'implication de la Cycline B dans le processus de cytocinèse

Un dérèglement du cycle cellulaire peut causer le cancer. Lors de la cytocinèse un anneau contractile d’actine et de myosine se forme, se contracte, et donne un anneau du midbody qui mène à l’abscision. Le processus de cytocinèse est sous le contrôle de protéines telles que la GTPase Rho qui active la cytocinèse et les cyclines-Cdks qui l'inhibent. La Drosophile possède 3 cyclines mitotiques CycA/ CycB/ CycB3 qui sont successivement dégradées en fin de mitose et permettent l'initiation de la cytocinèse. La dernière étape d’abscission est un phénomène qui reste encore peu connu. Les protéines Vps4 et CHMP4C liées à ANCHR vont, sous la dépendance de la kinase Aurora B, promouvoir l’abscision mais, suite à quelques études récentes, il semble y avoir une implication de la cycline B. Ici, le but était de tester l’implication de cette cycline dans les processus de cytocinèse et d’abscision, elle a été menée par microscopie à haute résolution en temps réel avec des cellules S2 de l’organisme Drosophila melanogaster par le suivi de protéines recombinantes fluorescentes. L’étude a été divisée en deux axes : gain et perte de fonction par l’intermédiaire respectivement de la protéine Cycline B recombinante stable, non dégradable (CycBstable-GFP) et l’inhibition par l’utilisation d’ARN double brin (ARNdb) sur l’endogène. La CycBstable-GFP a perturbé la cytocinèse en induisant plusieurs anneaux contractiles et midbodies. En revanche la réduction de l’expression de CycB n'a pas eu d’effet observable, et elle ne semble pas avoir d’action sur l’abscission malgré le recrutement de CycB-GFP au midbody tardif. En revanche la protéine Cdk1 semble avoir un rôle dans l'abscision puisque sa réduction d’expression a induit un délai. Elle a donc une implication potentielle sur la cytocinèse.

Funktionelle Analyse der LC-FACS in Dictyostelium discoideum

"Funktionelle Analyse der LC-FACS in Dictyostelium discoideum" Das Dictyostelium discoideum Gen fcsA kodiert für ein 75 kDa großes Protein. Es kann durch Homologieanyalysen der Amino-säuresequenz zu den "long-chain fatty acyl-CoA"-Synthetasen ge-rechnet werden, die lang-kettige Fettsäuren durch die kovalente Bindung von Coenzym A akti-vie-ren und damit für diverse Reak-tionen in Stoffwechsel und Molekül-Synthese der Zelle verfügbar machen. Die hier untersuchte D. discoideum LC-FACS lokalisiert als peripher assoziiertes Protein an der cytosolischen Seite der Membran von Endo-somen und kleiner Vesikel. Bereits kurz nach der Bildung in der frühen sauren Phase kann die Lokalisation der LC-FACS auf Endosomen ge-zeigt werden. Sie dissoziiert im Laufe ihrer Neutra-li-sierung und kann auf späten Endosomen, die vor ihrer Exocytose stehen nicht mehr nach-gewiesen werden. Ein Teil der kleinen die in der gesamte Zelle verteilten kleinen Vesikel zeigt eine Kolokalisation mit lysosomalen Enzymen. Trotz des intrazellulären Verteilungs-mus-ters, das eine Beteiligung dieses Pro-teins an der Endocytose nahe-legt, konnte kein signifikanter Rückgang der Pino- und Phagocytose-Rate in LC-FACS Nullmutanten beobachtet werden. Der endo-cy-to-ti-sche Transit ist in diesen Zellen etwas verlängert, außerdem zeigen die Endosomen einen deutlich erhöhten pH-Wert, was zu einer weniger effektiven Prozessierung eines lysosomalen Enzyms führt (a-Mannosidase). Die Funktion der LC-FACS ist die Aufnahme von langkettigen Fettsäuren aus dem Lumen der Endosomen.

On the function of the Dictyostelium Argonaute A protein (AgnA) in epigenetic gene regulation

With molecular biology methods and bioinformatics, the Argonaute proteins in Dictyostelium discoideum were characterized, and the function of the AgnA protein in RNAi and DNA methylation was investigated, as well as cellular features. Also interaction partners of the PAZ-Piwi domain of AgnA (PAZ-PiwiAgnA) were discovered. The Dictyostelium genome encodes five Argonaute proteins, termed AgnA/B/C/D/E. The expression level of Argonaute proteins was AgnB/D/E > AgnA > AgnC. All these proteins contain the characteristic conserved of PAZ and Piwi domains. Fluorescence microscopy revealed that the overexpressed C-terminal GFP-fusion of PAZ-PiwiAgnA (PPWa-GFP) localized to the cytoplasm. Overexpression of PPWa-GFP leaded to an increased gene silencing efficiency mediated by RNAi but not by antisense RNA. This indicated that PAZ-PiwiAgnA is involved in the RNAi pathway, but not in the antisense pathway. An analysis of protein-protein interactions by a yeast-two-hybrid screen on a cDNA library from vegetatively grown Dictyostelium revealed that several proteins, such as EF2, EF1-I, IfdA, SahA, SamS, RANBP1, UAE1, CapA, and GpdA could interact with PAZ-PiwiAgnA. There was no interaction between PAZ-PiwiAgnA and HP1, HelF and DnmA detected by direct yeast-two-hybrid analysis. The fluorescence microscopy images showed that the overexpressed GFP-SahA or IfdA fusion proteins localized to both cytoplasm and nuclei, while the overexpressed GFP-SamS localized to the cytoplasm. The expression of SamS in AgnA knock down mutants was strongly down regulated on cDNA and mRNA level in, while the expression of SahA was only slightly down regulated. AgnA knock down mutants displayed defects in growth and phagocytosis, which suggested that AgnA affects also cell biological features. The inhibition of DNA methylation on DIRS-1 and Skipper retroelements, as well as the endogenous mvpB and telA gene, observed for the same strains, revealed that AgnA is involved in the DNA methylation pathway. Northern blot analysis showed that Skipper and DIRS-1 were rarely expressed in Ax2, but the expression of Skipper was upregulated in AgnA knock down mutants, while the expression of DIRS-1 was not changed. A knock out of the agnA gene failed even though the homologous recombination of the disruption construct occurred at the correct site, which indicated that there was a duplication of the agnA gene in the genome. The same phenomenon was also observed in ifdA knock out experiments.

Immunogenicity of the outer domain of a HIV-1 clade C gp120

Background: The possibility that a sub domain of a C clade HIV-1 gp120 could act as an effective immunogen was investigated. To do this, the outer domain ( OD) of gp120(CN54) was expressed and characterized in a construct marked by a re-introduced conformational epitope for MAb 2G12. The expressed sequence showed efficient epitope retention on the isolated ODCN54 suggesting authentic folding. To facilitate purification and subsequent immunogenicity ODCN54 was fused to the Fc domain of human IgGl. Mice were immunised with the resulting fusion proteins and also with gp120(CN54)-Fc and gp120 alone. Results: Fusion to Fc was found to stimulate antibody titre and Fc tagged ODCN54 was substantially more immunogenic than non-tagged gp120. Immunogenicity appeared the result of Fc facilitated antigen processing as immunisation with an Fc domain mutant that reduced binding to the FcR lead to a reduction in antibody titre when compared to the parental sequence. The breadth of the antibody response was assessed by serum reaction with five overlapping fragments of gp120(CN54) expressed as GST fusion proteins in bacteria. A predominant anti-inner domain and anti-V3C3 response was observed following immunisation with gp120(CN54)-Fc and an anti-V3C3 response to the ODCN54-Fc fusion. Conclusion: The outer domain of gp120(CN54) is correctly folded following expression as a C terminal fusion protein. Immunogenicity is substantial when targeted to antigen presenting cells but shows V3 dominance in the polyvalent response. The gp120 outer domain has potential as a candidate vaccine component.

Green fluorescent protein as a reporter of prion protein folding

Background: The amino terminal half of the cellular prion protein PrPc is implicated in both the binding of copper ions and the conformational changes that lead to disease but has no defined structure. However, as some structure is likely to exist we have investigated the use of an established protein refolding technology, fusion to green fluorescence protein (GFP), as a method to examine the refolding of the amino terminal domain of mouse prion protein. Results: Fusion proteins of PrPc and GFP were expressed at high level in E. coli and could be purified to near homogeneity as insoluble inclusion bodies. Following denaturation, proteins were diluted into a refolding buffer whereupon GFP fluorescence recovered with time. Using several truncations of PrPc the rate of refolding was shown to depend on the prion sequence expressed. In a variation of the format, direct observation in E. coli, mutations introduced randomly in the PrPc protein sequence that affected folding could be selected directly by recovery of GFP fluorescence. Conclusion: Use of GFP as a measure of refolding of PrPc fusion proteins in vitro and in vivo proved informative. Refolding in vitro suggested a local structure within the amino terminal domain while direct selection via fluorescence showed that as little as one amino acid change could significantly alter folding. These assay formats, not previously used to study PrP folding, may be generally useful for investigating PrPc structure and PrPc-ligand interaction.

Generation of anti-complement "prodrugs": cleavable reagents for specific delivery of complement regulators to disease sites

Expression of biologically active molecules as fusion proteins with antibody Fc can substantially extend the plasma half-life of the active agent but may also influence function. We have previously generated a number of fusion proteins comprising a complement regulator coupled to Fc and shown that the hybrid molecule has a long plasma half-life and retains biological activity. However, several of the fusion proteins generated had substantially reduced biological activity when compared with the native regulator or regulator released from the Fc following papain cleavage. We have taken advantage of this finding to engineer a prodrug with low complement regulatory activity that is cleaved at sites of inflammation to release active regulator. Two model prodrugs, comprising, respectively, the four short consensus repeats of human decay accelerating factor (CD55) linked to IgG4 Fc and the three NH2-terminal short consensus repeats of human decay accelerating factor linked to IgG2 Fc have been developed. In each, specific cleavage sites for matrix metalloproteinases and/or aggrecanases have been incorporated between the complement regulator and the Fc. These prodrugs have markedly decreased complement inhibitory activity when compared with the parent regulator in vitro. Exposure of the prodrugs to the relevant enzymes, either purified, or in supernatants of cytokine-stimulated chondrocytes or in synovial fluid, efficiently cleaved the prodrug, releasing active regulator. Such agents, having negligible systemic effects but active at sites of inflammation, represent a paradigm for the next generation of anti-C therapeutics.

Development of a rapid one-step immunochromatographic assay for HCV core antigen detection

Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)

Utilização do metabolismo protéico ( 15N-glicina) na detecção precoce de agravamento da atividade da doença em pacientes portadores de retocolite ulcerativa inespecífica

Disease activity was assessed in 10 (five males and five females) ulcerative colitis patients through the following parameters: clinical, laboratory, sigmoidoscopic and histological. Protein metabolism was also assessed with 15N-glycine and urinary ammonia as end product. Only one patient had exacerbation of the disease two months after the study started. This patient presented in the beginning of the study protein synthesis and breakdown of 4.51 and 3.47 g protein/kg/day, respectively, values higher than all other patients, showing an hypermetabolic state, suggesting an increase of the disease activity. However, this increase was not detected by others indicators and indexes utilised. These data allow to suggest the hypothesis that protein metabolism predicts precociously the exacerbation of disease activity in ulcerative colitis patients.

Avaliação dos polimorfismos nos genes enzima conversora de angiotensina e adenosina deaminase em pacientes com diabetes melito tipo 2

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES)

Desempenho produtivo e resposta inflamatória de Pacu (Piaractus mesopotamicus) alimentado com ração suplementada com cromo trivalente

Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)

Caracterização biofísica e produção de antissoro policlonal contra a capa proteica recombinante do Southem bean mosaic virus

Pós-graduação em Genética - IBILCE

Assessing the gain of biological data integration in gene networks inference

Background: A current challenge in gene annotation is to define the gene function in the context of the network of relationships instead of using single genes. The inference of gene networks (GNs) has emerged as an approach to better understand the biology of the system and to study how several components of this network interact with each other and keep their functions stable. However, in general there is no sufficient data to accurately recover the GNs from their expression levels leading to the curse of dimensionality, in which the number of variables is higher than samples. One way to mitigate this problem is to integrate biological data instead of using only the expression profiles in the inference process. Nowadays, the use of several biological information in inference methods had a significant increase in order to better recover the connections between genes and reduce the false positives. What makes this strategy so interesting is the possibility of confirming the known connections through the included biological data, and the possibility of discovering new relationships between genes when observed the expression data. Although several works in data integration have increased the performance of the network inference methods, the real contribution of adding each type of biological information in the obtained improvement is not clear. Methods: We propose a methodology to include biological information into an inference algorithm in order to assess its prediction gain by using biological information and expression profile together. We also evaluated and compared the gain of adding four types of biological information: (a) protein-protein interaction, (b) Rosetta stone fusion proteins, (c) KEGG and (d) KEGG+GO. Results and conclusions: This work presents a first comparison of the gain in the use of prior biological information in the inference of GNs by considering the eukaryote (P. falciparum) organism. Our results indicates that information based on direct interaction can produce a higher improvement in the gain than data about a less specific relationship as GO or KEGG. Also, as expected, the results show that the use of biological information is a very important approach for the improvement of the inference. We also compared the gain in the inference of the global network and only the hubs. The results indicates that the use of biological information can improve the identification of the most connected proteins.

Quantitative correlation between transcriptional levels of ER chaperone, peroximal protein and FVIII productivity in human Hek-293 cell line

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.

Caspase-mediated cleavage of the exosome subunit PM/Scl-75 during apoptosis

Recent studies have implicated the dying cell as a potential reservoir of modified autoantigens that might initiate and drive systemic autoimmunity in susceptible hosts. A number of subunits of the exosome, a complex of 3'→5' exoribonucleases that functions in a variety of cellular processes, are recognized by the so-called anti-PM/Scl autoantibodies, found predominantly in patients suffering from an overlap syndrome of myositis and scleroderma. Here we show that one of these subunits, PM/Scl-75, is cleaved during apoptosis. PM/Scl-75 cleavage is inhibited by several different caspase inhibitors. The analysis of PM/Scl-75 cleavage by recombinant caspase proteins shows that PM/Scl-75 is efficiently cleaved by caspase-1, to a smaller extent by caspase-8, and relatively inefficiently by caspase-3 and caspase-7. Cleavage of the PM/Scl-75 protein occurs in the C-terminal part of the protein at Asp369 (IILD369↓G), and at least a fraction of the resulting N-terminal fragments of PM/Scl-75 remains associated with the exosome. Finally, the implications of PM/Scl-75 cleavage for exosome function and the generation of anti-PM/Scl-75 autoantibodies are discussed.

Untersuchungen zur selektiven Deletion alloreaktiver Spender-T- Lymphozyten durch CD178-modifizierte dendritische Zellen im Rahmen der allogenen Blutstammzelltransplantation

Eine der häufigsten Komplikationen bei der allogenen Blutstammzelltransplantation stellt die Transplantat-gegen-Wirt-Erkrankung (Graft versus Host Disease, GvHD) dar. Sie wird durch allogene Spender-T-Lymphozyten verursacht, die Gewebe des Transplantatempfängers erkennen und inflammatorische Entzündungsprozesse auslösen. Neben dieser Alloreaktivität induzieren Spender-T-Lymphozyten jedoch auch immuntherapeutisch erwünschte Transplantat-gegen-Leukämie-Reaktionen (Graft versus Leukemia, GvL-Reaktion), bei denen residuelle Tumor- bzw. Leukämiezellen im Patienten durch Spender-T-Zellen spezifisch erkannt und eliminiert werden. Im Rahmen einer verbesserten Immmuntherapie wird daher versucht, GvHD-reaktive und GvL-reaktive Spender-T-Lymphozyten effizient voneinander zu separieren und so eine wirkungsvolle GvHD-Prophylaxe bzw. optimierte GvL-Induktion zu erreichen. In diesem Kontext war es Ziel dieser Arbeit, murine dendritische Zellen (DZ) so zu modifizieren, daß sie für die spezifische Deletion alloreaktiver T-Zellen in murinen GvHD/GvL-Tiermodellen eingesetzt werden können. Die Modifikation der DZ sollte dazu führen, daß über das CD95/CD178-System Aktivierungs-induzierter Zelltod (activation induced cell death, AICD) in alloreaktiven T-Zellen ausgelöst wird. Hierzu wurden für die Modifikation der DZ zwei verschiedene Mechanismen angewandt: a) die Transfektion der DZ mit CD178-mRNA sowie b) die zielgerichtete Immobilisierung von hCD178-X-Fusionsproteinen auf Oberflächenmolekülen von DZ bzw. T-Zellen. Als Positivkontrolle für die Induktion CD95-vermittelter Apoptose diente der agonistische anti-CD95-Antikörper Jo2. Bei der Transfektion muriner DZ mit mRNA zeigte sich anhand des Reportergens EGFP, daß aus dem Knochenmark generierte DZ mit hoher Effizienz mit EGFP-mRNA transfizierbar waren. Im Falle von hCD178-mRNA führte die Transfektion jedoch zu einer insuffizienten CD178-Expression, die mit den regulatorischen Eigenschaften der zytoplasmatischen CD178-Region in Verbindung gebracht werden konnte. So führte die Verwendung einer zytoplasmatisch trunkierten Form der CD178-mRNA (CD178Dzyt) zu einer durchflußzytometrisch nachweisbaren CD178-Expression in DZ. Mit diesen CD178Dzyt-exprimierenden DZ konnte in einem Proliferationstest die Proliferation alloreaktiver T-Zellen inhibiert werden. Die Beladung von DZ bzw. von T-Zellen mit hCD178-X-Fusionsproteinen führte in vitro ebenfalls zu einer deutlichen Reduktion von Alloreaktivität. Dabei konnte eine spezifische Deletion/Inhibition alloreaktiver T-Zellen nachgewiesen werden. Die Elimination alloreaktiver T-Zellen erfolgte in beiden Verfahren über AICD. Darüber hinaus wurde eine Bifunktionalität der Fusionsproteine festgestellt, da sie neben der Induktion CD95-vermittelter Apoptose auch in der Lage waren, die Kostimulation allogener T-Zellen effizient zu inhibieren. Mit Hilfe adoptiver T-Zell-Transferexperimente konnten abschließend die in vitro gewonnenen Ergebnisse in vivo in zwei verschiedenen GvHD-Mausmodellen bestätigt werden.