Global ETD Search

101	Characterizing the Role of Ribosomal Protein L7Ae in Archaeal RNase P Catalysis and Exploring the Use of Archaeal RNase P as a Functional Genomics Tool Cho, I-Ming 16 December 2010 (has links) No description available. Biochemistry RNase P ribonucleoprotein tRNA kink turn (K turn) L7Ae external guide sequence
102	Biochemical Analysis of Thermotoga maritima Ribonuclease III and its Ribosomal RNA Substrates Nathania, Lilian January 2011 (has links) The site-specific cleavage of double-stranded (ds) RNA is a conserved early step in bacterial ribosomal RNA (rRNA) maturation that is carried out by ribonuclease III. Studies on the RNase III mechanism of dsRNA cleavage have focused mainly on the enzymes from mesophiles such as Escherichia coli. In contrast, little is known of the RNA processing pathways and the functions of associated ribonucleases in the hyperthermophiles. Therefore, structural and biochemical studies of proteins from hyperthermophilic bacteria are providing essential insight on the sources of biomolecular thermostability, and how enzymes function at high temperatures. The biochemical behavior of RNase III of the hyperthermophilic bacterium Thermotoga maritima is analyzed using purified recombinant enzyme and the cognate pre-ribosomal RNAs as substrates. The T. maritima genome encodes a ~5,000 nucleotide (nt) transcript, expressed from the single ribosomal RNA (rRNA) operon. RNase III processing sites are expected to form through base-pairing of complementary sequences that flank the 16S and 23S rRNAs. The Thermotoga pre-16S and pre-23S processing stems are synthesized in the form of small hairpins, and are efficiently and site-specifically cleaved by Tm-RNase III at sites consistent with an in vivo role of the enzyme in producing the immediate precursors to the mature rRNAs. T. maritima (Tm)-RNase III activity is dependent upon divalent metal ion, with Mg^2+ as the preferred species, at concentrations >= 1 mM. Mn^2+, Co^2+ and Ni^2+ also support activity, but with reduced efficiency. The enzyme activity is also supported by salt (Na^+, K^+, or NH4^+) in the 50-80 mM range, with an optimal pH of ~8. Catalytic activity exhibits a broad temperature maximum of ~40-70 deg C, with significant activity retained at 95 deg C. Comparison of the Charged-versus-Polar (C-vP) bias of the protein side chains indicates that Tm-RNase III thermostability is due to large C-vP bias. Analysis of pre-23S substrate variants reveals a dependence of reactivity on the base-pair (bp) sequence in the proximal box (pb), a site of protein contact that functions as a positive determinant of recognition of E. coli (Ec)-RNase III substrates. The pb sequence dependence of reactivity is similar to that observed with the Ec-RNase III pb. Moreover, Tm-RNase III cleaves an Ec-RNase III substrate with identical specificity, and is inhibited by pb antideterminants that also inhibit Ec-Rnase III. These studies reveal the conservation acrosss a broad phylogenetic distance of substrate reactivity epitopes, both the positive and negative determinants, among bacterial RNase III substrates. / Chemistry Biochemistry Dsrna Processing Hyperthermophilic Enzyme Ribonuclease Iii Rna Rnase Iii Thermotoga Maritima
103	A MUTATIONAL-FUNCTIONAL ANALYSIS OF THE ESCHERICHIA COLI MACRODOMAIN PROTEIN, YMDB Smith, Alexandra Kimberly January 2018 (has links) Gene expression pathways exhibit many “twists and turns,” with theoretically numerous ways in which the pathways can be regulated by both negative and positive feedback mechanisms. A key step in gene expression is RNA maturation (RNA processing), which in the bacterial cell can be accomplished through RNA binding and enzymatic cleavages. The well-characterized bacterial protein Ribonuclease III (RNase III), is a conserved, double-stranded(ds)-specific ribonuclease. In the gram-negative bacterium Escherichia coli, RNase III catalytic activity is subject to both positive and negative regulation. A recent study has indicated that an E. coli protein, YmdB, may negatively regulate RNase III catalytic activity. It has been proposed that YmdB inhibition of RNase III may be part of an adaptive, post-transcriptional physiological response to cellular stress. In E. coli, the model organism in this study, YmdB protein is encoded by the single ymdB gene, and has a predicted molecular mass of ~18.8 kDa. YmdB has been classified as a macrodomain protein, as it exhibits a characteristic fold that specifically provides an ADP-ribose (ADPR) binding site. While YmdB can bind ADPR with good affinity, there may be additional ligands for the binding site. Thus, YmdB protein may interact with other components in the cell, which in turn could modulate the interaction of YmdB with RNase III. In previous research conducted within the Nicholson laboratory at Temple University, affinity-purified Escherchia coli(Ec) YmdB and Aquifex aeolicus (Aa) YmdB were found to exhibit ribonucleolytic activity. This observation initiated the long-term goal of learning how YmdB regulates RNase III, and how the ribonucleolytic activity of YmdB may be involved in this process. The specific goal of this thesis project was to further characterize the ribonucleolytic activity of Ec-YmdB through site-specific mutational analysis. Mutations were introduced into a proposed adenine-binding pocket previously identified by crystallography and by molecular modeling. The adenine-binding pocket is a region within the macrodomain fold where ADP-ribose could bind. The mutations were examined for their effect on Ec-YmdB cleavage of a model RNA, R1.1. The results of this study will contribute to the development of a model describing how the ribonucleolytic activity of YmdB is regulated. / Biology Biology Biology, Molecular Biochemistry Adenine-binding Adpr Escherichia Coli Macrodomain Rnase Iii Ymdb
104	Designing Cell-Free Protein Synthesis Systems for Improved Biocatalysis and On-Demand, Cost-Effective Biosensors Soltani Najafabadi, Mehran 06 August 2021 (has links) The open nature of Cell-Free Protein Synthesis (CFPS) systems has enabled flexible design, easy manipulation, and novel applications of protein engineering in therapeutic production, biocatalysis, and biosensors. This dissertation reports on three advances in the application of CFPS systems for 1) improving biocatalysis performance in industrial applications by site-specific covalent enzyme immobilization, 2) expressing and optimizing a difficult to express a mammalian protein in bacterial-based CFPS systems and its application for cost-effective, on-demand biosensors compatible with human body fluids, and 3) streamlining the procedure of an E. coli extract with built-in compatibility with human body fluid biosensors. Site-specific covalent immobilization stabilizes enzymes and facilitates recovery and reuse of enzymes which improves the net profit margin of industrial enzymes. Yet, the suitability of a given site on the enzyme for immobilization remains a trial-and-error procedure. This dissertation reports the reliability of several design heuristics and a coarse-grain molecular simulation in predicting the optimum sites for covalent immobilization of a target enzyme, TEM-1 ?-lactamase. This work demonstrates that the design heuristics can successfully identify a subset of favorable locations for experimental validation. This approach highlights the advantages of combining coarse-grain simulation and high-throughput experimentation using CFPS to efficiently identify optimal enzyme immobilization sites. Additionally, this dissertation reports high-yield soluble expression of a difficult-to-express protein (murine RNase Inhibitor or m-RI) in E. coli-lysate-based CFPS. Several factors including reaction temperature, reaction time, redox potential, and presence of folding chaperones in CFPS reactions were altered to find suitable conditions for m-RI expression. m-RI with the highest activity and stability was used to develop a lyophilized CFPS biosensor in human body fluids which reduced the cost of biosensor test by ~90%. Moreover, an E. coli extract with RNase inhibition activity was developed and tested which further streamlines the production of CFPS biosensors compatible with human body fluids. Mehran Soltani cell-free protein synthesis cell-free CFPS in vitro TEM-1 ?-lactamase antibiotics unnatural amino acid protein engineering site-specific covalent immobilization site-directed mutagenesis design heuristics coarse-grain simulation biosensor cell-free biosensor RNase inhibitor murine RNase inhibitor m-RI RNase inhibitor RNase A human body fluids saliva serum urine glutamine lyophilized point of care GroEL/ES folding chaperones E. coli extract Extract with RNase inhibition activity Engineering
105	Unraveling sugarcane-Diatraea saccharalis-opportunistic fungi interaction in sugarcane / Desvendando a interação cana-de-açúcar-Diatraea saccharalis-fungos oportunistas em cana-de-açúcar Franco, Flávia Pereira 10 March 2017 (has links) Plants respond to insect and pathogen attack by inducing and accumulating a large set of defense proteins. Colonization of sugarcane stalk by opportunistic fungi, such as Fusarium verticillioides and Colletotrichum falcatum, usually occurs after Diatraea saccharalis (Lepidoptera: Cambridae) caterpillars attack increasing the damage caused by the borer. Two homologous of BARWIN protein were identified in sugarcane, SUGARWIN1 and SUGARWIN2. Their gene expression is induced in response to wound and Diatraea saccharalis damage. However, the recombinant SUGARWIN protein does not affect insect development; but promotes significant morphological and physiological changes in Fusarium verticillioides and Colletotrichum falcatum, which lead to fungal cell death via apoptosis, indicating that SUGARWINs may work as a first layer of defense against the fungi infection. In this study, we deepen our understanding of the role of SUGARWINs in plant defense and the molecular mechanisms by which these proteins affect fungi by elucidating their molecular targets. Our results show that SUGARWINs play an important role in plant defense against opportunistic pathogens. We demonstrated that SUGARWINs are induced by C. falcatum, and the induction of SUGARWINs can vary among sugarcane varieties. The sugarcane variety exhibiting the highest level of SUGARWIN induction exhibited a considerable reduction in C. falcatum infection. Furthermore, SUGARWIN1 exhibited ribonuclease and chitinase activity, whereas SUGARWIN2 exhibited only chitinase activity. This variable enzymatic specificity seems to be the result of divergent amino acid composition within the substrate-binding site. Additionally, plants attacked by insects and pathogens display profound physiological, morphological and chemical changes or adaptations, which may result in organism attraction or avoidance. In this study, we also aimed to understand the insect-fungi association in sugarcane and the role of fungal volatile compounds in this association. Our results have shown that D. saccharalis positively influences C. falcatum infection on sugarcane, inducing a fast growing when compared to C. falcatum treatment without D. saccharalis attack. In addition, both fungi, C. falcatum and F. verticillioides, have been shown a double effect on D. saccharalis caterpillar, they promoted a strong attraction for insects due volatile organic compound emission and positively influenced D. saccharalis feeding and weight gain in diets supplemented with fungi. Fungal volatile organic compounds from C. falcatum and F. verticillioides were identified and quantified; acoradiene and acorenol were specifically induced by the fungi. These data suggest a synergistic interaction, mediated by organic volatile compounds, between D. saccharalis and the fungi C. falcatum and F. verticillioides in sugarcane. / As plantas respondem ao ataque de insetos e patógenos induzindo e acumulando um grande conjunto de proteínas de defesa. A colonização do caule de cana por fungos oportunistas, como Fusarium verticillioides e Colletotrichum falcatum, geralmente ocorre após o ataque de lagartas de Diatraea saccharalis (Lepidoptera: Cambridae), resultando no aumento do dano causado pelo inseto. Dois homólogos da proteína BARWIN foram identificados em cana-de-açúcar, SUGARWIN1 e SUGARWIN2. A expressão desses genes é induzida em resposta ao ferimento mecânico e ao ataque de Diatraea saccharalis, entretanto, a proteína não afeta o desenvolvimento do inseto, mas promove alterações morfológicas e fisiológicas significativas em Fusarium verticillioides e Colletotrichum falcatum, causando a morte destes fungos por apoptose. Esses dados indicam que as SUGARWINs podem funcionar como uma defesa inicial contra a infecção fúngica. Neste estudo, aprofundamos nosso entendimento do papel das SUGARWINs na defesa de plantas e os mecanismos moleculares pelos quais essas proteínas afetam os fungos, elucidando seus alvos moleculares. Nossos resultados mostraram que as SUGARWINs desempenham um papel importante na defesa da planta contra patógenos oportunistas. Foi demonstrado que essas proteínas também são induzidas por C. falcatum em cana-de-açúcar, e sua indução pode variar entre as variedades de cana-de-açúcar. A variedade de cana-de-açúcar que apresentou o maior nível de indução de SUGARWINs apresentou uma redução considerável na infecção por C. falcatum. Além disso, SUGARWIN1 exibiu atividade de ribonuclease e quitinase, enquanto que SUGARWIN2 exibiu apenas atividade de quitinase. Esta especificidade enzimática parece ser o resultado da composição divergente de aminoácidos no sítio de ligação do substrato. Além disso, as plantas atacadas por insetos e patógenos exibem profundas alterações fisiológicas, morfológicas e químicas ou adaptações, que podem resultar em atração ou repelência do organismo, dessa forma, estudamos também a associação inseto-fungos na cana-de-açúcar, e o papel dos compostos voláteis fúngicos nessa associação. Nossos resultados mostraram que D. saccharalis influencia positivamente a infecção por C. falcatum em cana-de-açúcar, induzindo crescimento rápido do fungo quando comparado ao tratamento com C. falcatum sem ataque de D. saccharalis. Além disso, ambos os fungos, C. falcatum e F. verticillioides, mostraram um efeito duplo sobre lagartas de D. saccharalis, promovendo uma forte atração desses insetos devido à emissão de compostos orgânicos voláteis e influenciando positivamente a alimentação de D. saccharalis e ganho de peso em dietas suplementadas com fungos. Os compostos orgânicos voláteis fúngicos de C. falcatum e F. verticillioides foram identificados e quantificados; acoradieno e acorenol foram especificamente induzidos pelos fungos. Estes dados sugerem uma interação sinergistica, mediada por compostos orgânicos voláteis, entre D. saccharalis e os fungos C. falcatum e F. verticillioides em cana-de-açúcar. Colletotrichum falcatum Colletotrichum falcatum Fusarium verticillioides Fusarium verticillioides BARWIN BARWIN Broca da cana Cana-de-açúcar Chitinase Interação planta-inseto-fungo Plant-insect-fungus interaction Quitinase RNase RNase Sugarcane Sugarcane borer SUGARWIN SUGARWIN
106	Translocation des colicines de type ribonuclease à travers la membrane interne bacterienne / Translocation of nuclease colicins D and E3 through the inner membrane of E. coli Chauleau, Mathieu 23 September 2011 (has links) Les colicines sont des toxines antibactériennes d’Escherichia coli qui sont relâchées par les cellules productrices (colicinogènes) dans le milieu extracellulaire en réponse à des conditions de stress environnementaux. Les colicines D et E3 sont des RNases qui clivent respectivement les tRNAArg et le 16S RNA ribosomique. Les deux colicines parvenues au cytoplasme de la cellule cible provoquent ainsi la mort par inactivation de la machinerie de biosynthèse des protéines. L’import de ces deux colicines nécessite d’abord le détournement de deux systèmes cellulaires différents (FepA/TonB ou BtuB/Tol) de leur fonction physiologique, permettant leur translocation à travers la membrane externe. L’idée que par la suite la translocation à travers la membrane interne nécessite au préalable une étape de processing des colicines nucléases est ancienne, mais elle n’a jamais été démontrée formellement. Nos travaux ont permis de montrer qu’une coupure endoprotéolytique des deux colicines constitue une étape de « processing » essentielle de leur action toxique. Nous avons détecté la présence du domaine C-terminal catalytique des deux colicines dans le cytoplasme des cellules cibles préalablement exposées à la toxine. Les mêmes fragments processés (PF) ont été identifiés dans les cellules sensibles et dans les cellules immunes contre ces colicines, qui sont protégées par une protéine d’immunité spécifique, formant un complexe neutre avec le domaine catalytique. Nous avons démontré que la protéase essentielle de la membrane interne, FtsH, est nécessaire au processing des deux colicines pendant leur import. Nous avons montré aussi que la signal-peptidase LepB, une autre enzyme essentielle de la membrane interne, interagit directement avec le domaine central de la colicine D in vitro et ainsi elle est un facteur protéique spécifiquement nécessaire au processing de la colicine D. Cependant ce n’est pas l’activité catalytique de LepB qui est impliquée dans la toxicité de la colicine D, mais elle jouerait un rôle structural. LepB ainsi faciliterait probablement l’association de la colicine D avec la membrane interne en vue de la reconnaissance de la toxine par FtsH. Nous avons aussi montré que la protéase OmpT de la membrane externe est responsable d’une coupure endoprotéolytique alternative, qui refléte probablement son rôle bien connu dans le système de défense des bactéries contre les peptides anti-microbiens. Même si cette coupure in vitro permet de libérer le domaine catalytique des colicines D et E3, il est établit maintenant que la protéase OmpT n’est pas impliquée dans le processing des colicines durant leur import dans le cytoplasme. / Colicins are antibacterial toxins of Escherichia coli that are released into the extracellular medium in response to environmental stress conditions. Colicin D is an RNase that cleaves the anticodon loop of all four isoaccepting tRNAArg. Colicin E3 cleaves 16 S ribosomal RNA. Both colicins provoke cell death by inactivating the protein biosynthetic machinery. Colicin producer cells are protected against both endogenous and exogenous toxin molecules by the constitutive expression of a cognate immunity protein, which forms a tight heterodimer complex with the nuclease domain of the colicin. The import of both colicins first requires the “hijack” of some distinct functions of the target cell (namely the BtuB/Tol and FepA/TonB systems, respectively), this allowing their translocation across the outer membrane. It has long been suggested that the import of nuclease colicins requires protein processing during the translocation across the inner membrane; however it had never been formally demonstrated. Our work shows that the two different RNase colicins E3 and D undergo a processing step inside the cell that is essential to their killing action. We have detected the presence of the C-terminal catalytic domains of these colicins in the cytoplasm of target bacteria. The same processed forms (PF) were identified in both colicin-sensitive cells and in cells immune to colicins, because of the expression of the cognate immunity protein. We demonstrate that the inner membrane protease FtsH is necessary for the processing of colicins D and E3 during their import. We also show that the signal peptidase LepB interacts directly with the central domain of colicin D in vitro and that it is a specific but not a catalytic requirement for in vivo processing of colicin D. The interaction of colicin D with LepB may ensure a stable association with the inner membrane that in turn allows the colicin recognition by FtsH. We have also shown that the outer membrane protease OmpT is responsible for alternative and distinct endoproteolytic cleavages of colicins D and E3 in vitro, presumably reflecting its known role in the bacterial defense against antimicrobial peptides. Even though the OmpT-catalyzed in vitro cleavage also liberates the catalytic domain from colicins D and E3, it is not involved in the processing of nuclease colicins during their import into the cytoplasm Toxines bactériennes Nucléases anti-microbiennes Import de colicines Translocation membranaire Processing protéolytique Signal-peptidase LepB Membrane protéase FtsH RNase colicine Bacterial toxines Antibacterial nucleases Colicin import Membrane translocation Proteolytic processing Signal-peptidase LepB Membrane-protease FtsH RNase colicin
107	An mRNA degradation complex in Bacillus subtilis / mRNA Abbau in Bacillus subtilis Lehnik-Habrink, Martin 26 October 2011 (has links) No description available. 570 Biowissenschaften, Biologie WF 200 Biology (incl. Psychology) Bacillus subtilis RNA Abbau RNase mRNA RNA Helikase Degradosom Proteinkomplex DEAD-box Bacillus subtilis RNA degradation RNase mRNA RNA helicase degradosome proteincomplex DEAD-box 42 Biologie
108	Les R-loops et leurs conséquences sur l'expression génique chez Escherichia coli. Baaklini, Imad 02 1900 (has links) Des variations importantes du surenroulement de l’ADN peuvent être générées durant la phase d’élongation de la transcription selon le modèle du « twin supercoiled domain ». Selon ce modèle, le déplacement du complexe de transcription génère du surenroulement positif à l’avant, et du surenroulement négatif à l’arrière de l’ARN polymérase. Le rôle essentiel de la topoisomérase I chez Escherichia coli est de prévenir l’accumulation de ce surenroulement négatif générée durant la transcription. En absence de topoisomérase I, l’accumulation de ce surenroulement négatif favorise la formation de R-loops qui ont pour conséquence d’inhiber la croissance bactérienne. Les R-loops sont des hybrides ARN-ADN qui se forment entre l’ARN nouvellement synthétisé et le simple brin d’ADN complémentaire. Dans les cellules déficientes en topoisomérase I, des mutations compensatoires s’accumulent dans les gènes qui codent pour la gyrase, réduisant le niveau de surenroulement négatif du chromosome et favorisant la croissance. Une des ces mutations est une gyrase thermosensible qui s’exprime à 37 °C. La RNase HI, une enzyme qui dégrade la partie ARN d’un R-loop, peut aussi restaurer la croissance en absence de topoisomérase I lorsqu’elle est produite en très grande quantité par rapport à sa concentration physiologique. En présence de topoisomérase I, des R-loops peuvent aussi se former lorsque la RNase HI est inactive. Dans ces souches mutantes, les R-loops induisent la réponse SOS et la réplication constitutive de l’ADN (cSDR). Dans notre étude, nous montrons comment les R-loops formés en absence de topoisomérase I ou RNase HI peuvent affecter négativement la croissance des cellules. Lorsque la topoisomérase I est inactivée, l’accumulation d’hypersurenroulement négatif conduit à la formation de nombreux R-loops, ce qui déclenche la dégradation de l’ARN synthétisé. Issus de la dégradation de l’ARNm de pleine longueur, des ARNm incomplets et traductibles s’accumulent et causent l’inhibition de la synthèse protéique et de la croissance. Le processus par lequel l’ARN est dégradé n’est pas encore complètement élucidé, mais nos résultats soutiennent fortement que la RNase HI présente en concentration physiologique est responsable de ce phénotype. Chose importante, la RNase E qui est l’endoribonuclease majeure de la cellule n’est pas impliquée dans ce processus, et la dégradation de l’ARN survient avant son action. Nous montrons aussi qu’une corrélation parfaite existe entre la concentration de RNase HI, l’accumulation d’hypersurenroulement négatif et l’inhibition de la croissance bactérienne. Lorsque la RNase HI est en excès, l’accumulation de surenroulement négatif est inhibée et la croissance n’est pas affectée. L’inverse se produit Lorsque la RNase HI est en concentration physiologique. En limitant l’accumulation d’hypersurenroulement négatif, la surproduction de la RNase HI prévient alors la dégradation de l’ARN et permet la croissance. Quand la RNase HI est inactivée en présence de topoisomérase I, les R-loops réduisent le niveau d’expression de nombreux gènes, incluant des gènes de résistance aux stress comme rpoH et grpE. Cette inhibition de l’expression génique n’est pas accompagnée de la dégradation de l’ARN contrairement à ce qui se produit en absence de topoisomérase I. Dans le mutant déficient en RNase HI, la diminution de l’expression génique réduit la concentration cellulaire de différentes protéines, ce qui altère négativement le taux de croissance et affecte dramatiquement la survie des cellules exposées aux stress de hautes températures et oxydatifs. Une inactivation de RecA, le facteur essentiel qui déclenche la réponse SOS et le cSDR, ne restaure pas l’expression génique. Ceci démontre que la réponse SOS et le cSDR ne sont pas impliqués dans l’inhibition de l’expression génique en absence de RNase HI. La croissance bactérienne qui est inhibée en absence de topoisomérase I, reprend lorsque l’excès de surenroulement négatif est éliminé. En absence de RNase HI et de topoisomérase I, le surenroulement négatif est très relaxé. Il semble que la réponse cellulaire suite à la formation de R-loops, soit la relaxation du surenroulement négatif. Selon le même principe, des mutations compensatoires dans la gyrase apparaissent en absence de topoisomérase I et réduisent l’accumulation de surenroulement négatif. Ceci supporte fortement l’idée que le surenroulement négatif joue un rôle primordial dans la formation de R-loop. La régulation du surenroulement négatif de l’ADN est donc une tâche essentielle pour la cellule. Elle favorise notamment l’expression génique optimale durant la croissance et l’exposition aux stress, en limitant la formation de R-loops. La topoisomérase I et la RNase HI jouent un rôle important et complémentaire dans ce processus. / Important fluctuations of DNA supercoiling occur during transcription in the frame of the “twin supercoiled domain” model. In this model, transcription elongation generates negative and positive supercoiling respectively, upstream and downstream of the moving RNA polymerase. The major role of bacterial topoisomerase I is to prevent the accumulation of transcription-induced negative supercoiling. In its absence, the accumulation of negative supercoiling triggers R-loop formation which inhibits bacterial growth. R-loops are DNA/RNA hybrids formed during transcription when the nascent RNA hybridizes with the template strand thus, leaving the non-template strand single stranded. In cells lacking DNA topoisomerase I, a constant and selective pressure for the acquisition of compensatory mutations in gyrase genes reduces the negative supercoiling level of the chromosome and allows growth. One of these mutations is a thermosensitive gyrase expressed at 37 °C. The overexpression of RNase HI, an enzyme that degrades the RNA moiety of an R-loop, is also able to correct growth inhibition in absence of topoisomerase I. In the presence of topoisomerase I, R-loops can also form when RNase HI is lacking. In these mutants, R-loop formation induces SOS and constitutive stable DNA replication (cSDR). In our study, we show how R-loops formed in cells lacking topoisomerase I or RNase HI can affect bacterial growth. When topoisomerase I is inactivated, the accumulation of hypernegative supercoiling inhibits growth by causing extensive R-loop formation which, in turn, can lead to RNA degradation. As a result of RNA degradation, the accumulation of truncated and functional mRNA instead of full length ones, is responsible for protein synthesis inhibition that alters bacterial growth. The mechanism by which RNA is degraded is not completely clear but our results strongly suggest that RNase HI is involved in this process. More importantly, the major endoribonuclease, RNase E, is not involved in RNA degradation because RNA is degraded before its action. We show also that there is a perfect correlation between RNase HI concentration, the accumulation of hypernegative supercoiling and bacterial growth inhibition. When RNase HI is in excess, no accumulation of hypernegative supercoiling and growth inhibition are observed. The opposite is true when RNase HI is at its wild type level. By preventing the accumulation of hypernegative supercoiling, the overproduction of RNase HI inhibits extensive R-loop formation and RNA degradation, thus, allowing growth. In absence of RNase HI (rnhA) and in presence of topoisomerase I, R-loops are also responsible for an inhibition in gene expression, including stress genes such as rpoH and grpE. The inhibition of gene expression is not related to RNA degradation as seen in absence of topoisomerase I but it is rather related to a reduction in gene expression. In absence of RNase HI, the diminution of genes expression is responsible for a reduction in the cellular level of proteins, which negatively affects bacterial growth and bacterial survival to heat shock and oxydative stress. Additional mutations in RecA, the protein that activates SOS and cSDR after R-loop formation in rnhA, do not correct this phenotype in rnhA. Thus, SOS and cSDR are not directly involved in the inhibition of gene expression in the absence of RNase HI. In absence of topoisomerase I, growth inhibition resumes when hypernegative supercoiling is reduced. When compared to wild type strains, DNA is very relaxed in absence of RNase HI and topoisomerase I. It seems that R-loop formation induces the relaxation of negatively supercoiled DNA. All this strongly supports the idea that negative supercoiling plays an important role in R-loop formation. Finally, our work shows how essential negative supercoiling regulation is for cell physiology. By preventing R-loop formation, regulation of negative supercoiling allows optimal gene expression, which is crucial for cellular growth and for stress survival. Both topoisomerase I and RNase HI play an important and complementary role in this process. Surenroulement de l'ADN DNA supercoiling Hypersurenroulement négatif Hypernegative supercoiling Topoisomérase I bactérienne Bacterial topoisomerase I Transcription Transcription R-loop R-loop RNase HI RNase HI Expression génique Gene expression
109	Les R-loops et leurs conséquences sur l'expression génique chez Escherichia coli Baaklini, Imad 02 1900 (has links) No description available. Surenroulement de l'ADN DNA supercoiling Hypersurenroulement négatif Hypernegative supercoiling Topoisomérase I bactérienne Bacterial topoisomerase I Transcription Transcription R-loop R-loop RNase HI RNase HI Expression génique Gene expression
110	Molecular analysis of the S-RNase in self-incompatible Solanum chacoense Qin, Xike January 2006 (has links) Thèse numérisée par la Direction des bibliothèques de l'Université de Montréal. Solanum chacoense Auto-incompatibilité gamétophytique S-RNase Région conservée C4 Mutagenèse dirigée un site Pollen diploïde hétéroallelique Glycoprotein et valeur seuil

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