Global ETD Search

21	Proline Codon Translational Fidelity in Rhodopseudomonas palustris: Characterization of Novel Trans-editing Factor ProXp-abu Bacusmo, Jo Marie 18 September 2014 (has links) No description available. Biochemistry Chemistry Molecular Biology
22	Découverte et caractérisation d'une nouvelle forme de méthionyl-ARNt synthétase nucléaire chez la levure Saccharomyces cerevisiae / Discovery and characterization of a new methionyl-tRNA synthetase in Saccharomyces cerevisiae Laporte, Daphné 30 September 2016 (has links) La methionyl-ARNt synthétase (MetRS) de Saccharomyces cerevisiae aminoacyle les ARNt méthionine initiateur et élongateur (ARNtiMet et ARNteMet), mais possède également des fonctions atypiques. Nous avons montré que la MetRS rejoint le noyau durant la transition diauxique afin de réguler la transcription des gènes nucléaires des complexes III et V de la chaîne respiratoire mitochondriale. Pour ce faire, la MetRS possède au moins deux signaux de localisation nucléaire (NLS) dans sa séquence, l’un se situant dans les 55 premiers acides aminés (aa) et le second, au delà de la partie N-terminale lui permettant de recruter les sous-unités Rpb4 et Rpb7 de l’ARN pol II. Nous avons montré qu’en fermentation, la MetRS est clivée entre le 114ème et le 132ème aa et que cette forme clivée est essentielle à la viabilité des cellules, puisqu’un variant non clivé (MetRSK11A) ne permet pas la croissance. Nous avons surproduit et purifié un mutant de la MetRS clivée (MetRSΔ142) et montré que ce variant est plus efficace pour l’aminoacylation de l’ARNtiMet que la forme entière de MetRS. Ainsi, notre étude suggère que chez S. cerevisiae, la forme longue de MetRS cytoplasmique permet l’aminoacylation de l’ARNteMet, la forme longue de MetRS nucléaire régule la transcription, et la forme clivée de MetRS nucléaire et cytoplasmique permet l’aminoacylation de l’ARNtiMet / Methionyl-tRNA synthetase (MetRS) is the enzyme in charge of aminocylation of tRNA methionine initiator and elongator (tRNAiMet et tRNAeMet), but also displays atypical functions in Saccharomyces cerevisiae. In the present work, we showed that MetRS is imported to the nucleus during the diauxic shift in order to regulate transcription of genes coding for the complexes III and V subunits of the mitochondrial respiratory chain. To do so, MetRS harbors at least two nuclear localization signals (NLS), located within the 55 first aminoacids (NLS1) and beyond the N-terminal part (NLS2). The N- terminal part is responsible for the recruitment of RNA pol II subunits Rpb4 and Rpb7. We also showed that MetRS is cleaved through the 114th and the 132nd aminoacid during fermentation and that the proteolysed form is essential for the viability of the cell, since a mutant of MetRS which is not cleaved (MetRSK11A) did not allows the growth. We showed that an overproduced and purified a mutant representative of the cleaved form (MetRSΔ142) is more efficient for tRNAiMet aminoacylation than the full length MetRS. Thus, our study suggests that in S. cerevisiae, the cytoplasmic full length MetRS aminoacylates tRNAeMet, the nuclear full length MetRS regulates genes transcription, and the cytoplasmic and nuclear cleaved MetRS aminoacylates the tRNAiMet. Aminoacyl-ARNt synthétase ARNt Noyau Saccharomyces cerevisiae Transition diauxique Transcription Clivage Aminoacyl-tRNA synthetase TRNA Nucleus Saccharomyces cerevisiae Diauxic shift Transcription Cleavage 572.8
23	Le complexe multisysthématique AME de levure : dynamique de l'édifice et rôles non canoniques de ces composants / The multisynthetasic AME complex in yeast : dynamics of the complex and non canonical roles of its components Enkler, Ludovic 12 September 2014 (has links) Les complexes multisynthétasiques (MSC) sont des complexes multi-protéiques identifiés dans un grand nombre d’organismes pro- et eucaryotes. Ils impliquent des protéines d’assemblages et des aminoacyl-ARNt synthétases (aaRSs), responsables de l’aminoacylation de leurs ARNts homologues au cours de la traduction. La taille et la composition des MSC varient selon les organismes, et le rôle de ces complexes n’est pas encore totalement compris. Il semblerait néanmoins que chez les eucaryotes, l’accrétion en complexe soit une stratégie mise en oeuvre par les cellules pour empêcher les aaRSs d’assurer des fonctions additionnelles. Chez S.cerevisiae,nous montrons que la dynamique du complexe AME, composé de la méthionyl- et de la glutamyl-ARNt synthétase (MRS et ERS) ainsi que de la protéine d’ancrage Arc1p, est dépendante du métabolisme de la levure. En respiration la MRS joue le rôle de facteur de transcription et régule l’expression des gènes nucléaires du complexe III et V de la chaîne respiratoire, tandis que l’ERS active la traduction mitochondriale. Cette étude montre que la relocalisation synchrone est primordiale pour l’adaptation des cellules au métabolisme respiratoire. / Multisynthetase complexes (MSC) are complexes made of several proteins and were identified in a wide variety of organisms from pro- to eukaryotes. They are usually made of assembly factors and aminoacyl-tRNA synthetases (aaRSs), which are responsible for the aminoacylation of their corresponding tRNAs during translation. Depending on the organisms, size and composition of these complexes differ greatly and their role is not fully understood yet. Although it seems that in eukaryotes, accretions of aaRSs into MSC prevent aaRSs to perform their additional functions. In the yeast Saccharomyces cerevisiae, we show that the dynamic of the AME complex, made of the méthionyl- and glutamyl-tRNA synthetases (MRS and ERS) and the assembly protein Arc1p is linkedto yeast metabolism. In respiration, MRS is imported in the nucleus to act as a transcription factor and regulates the expression of nuclear genes belonging to complex III and V of the respiratory chain, while ERS is imported in mitochondria to activate translation. This study shows that synchronous relocation of both aaRSs is crucial for yeast cells to adapt to respiratory metabolism. Complexe multisynthétasique Aminoacyl-ARNt synthétase ARNt Saccharomyces cerevisiae Transition diauxique Mitochondrie Transcription Traduction Multisynthetase complex Aminoacyl-tRNA synthetase TRNA Saccharomyces cerevisiae Diauxic shift Mitochondria Transcription Translation 572.8
24	ARNt "manchots" : structure, fonctionnalité et évolution / Structure, function and evolution of armless mitochondrial tRNAs Jühling, Tina 14 December 2016 (has links) Les ARNt sont des molécules adaptatrices reliant l'information génétique de l’ARN messagers à la séquence d'acides aminés primaire des protéines. Les ARNt ont une structure typique, appelée "feuille de trèfle". Certains ARNt mitochondriaux montrent une forte dérivation de cette structure. Un cas extrême peut être observé dans les mitochondries du nématode R. culicivorax. Cette étude vise la caractérisation fonctionnelle de ces ARNt «bizarres» et de définir leurs propriétés structurales et leur fonctionnalité avec des protéines partenaires telles que les CCAses et les aminoacyl-ARNt synthetases. Ce travail révèle que les ARNt sans bras forment une structure secondaire en forme d'épingle à cheveux et que leurs structures 3D présentent une grande flexibilité intrinsèque. Les tests initiaux n’ont pas démontré l'activité d'aminoacylation. Cependant, les ARNt sans bras représentent des molécules fonctionnelles pour le CCAse, indiquant des adaptations de l’enzyme aux ARNt sans bras. / TRNAs are adapter molecules linking the genetic information of messenger RNAs with the primary amino acid sequence of proteins. tRNAs have a typical cloverleaf-like secondary structure. Some mitochondrial tRNAs show a high derivation from this canonical tRNA structure. An extreme case of structural truncations can be observed in mitochondria of the nematode R. culicivorax. This study aims the functional characterization of such “bizarre” tRNAs in defining their structural properties and their functionality with interacting partner proteins such as CCA-adding enzymes and aminoacyl-tRNA synthetases. This work reveals that armless tRNAs form a hairpin-shaped secondary structure. 3D structures exhibit a high intrinsic flexibility. Initial tests could not demonstrate aminoacylation activity. However, armless tRNAs represent functional molecules for CCA-incorporation, indicating adaptations of CCA-adding enzymes to armless tRNAs. ARN transfert Mitochondrie CCAse Aminoacyl-ARNt synthetase Romanomermis culicivorax Transfer RNA Mitochondria CCA-adding enzyme Aminoacyl-tRNA synthetase Romanomermis culicivorax 572.8
25	Maintaining Fidelity of Translation by Bacterial Trans-Editing Proteins:Caulobacter crescentus ProXp-ala and Rhodopseudomonas palustris ProXp-x Kuzmishin Nagy, Alexandra Burden 02 October 2019 (has links) No description available. Biochemistry Biology Chemistry Cellular Biology Experiments Microbiology Molecules aminoacyl-tRNA synthetase aaRS non-protein amino acid Ala Abu tRNA editing trans-editing Rhodopseudomonas palustris
26	STUDIES OF THE PYRROLYSYL-TRNA SYNTHETASE Jiang, Ruisheng 23 July 2013 (has links) No description available. Biochemistry Microbiology Archaeology pyrrolysine Amino Acid Aminoacyl tRNA Synthetase Archaea Bacteria RNA-binding Protein Transfer RNA (tRNA) 22nd Amino Acid Genetic Code Pyrrolysyl-tRNA Synthetase
27	Aminoacyl-tRNA Synthetase Production for Unnatural Amino Acid Incorporation and Preservation of Linear Expression Templates in Cell-Free Protein Synthesis Reactions Broadbent, Andrew 01 March 2016 (has links) (PDF) Proteins—polymers of amino acids—are a major class of biomolecules whose myriad functions facilitate many crucial biological processes. Accordingly, human control over these biological processes depends upon the ability to study, produce, and modify proteins. One innovative tool for accomplishing these aims is cell-free protein synthesis (CFPS). This technique, rather than using living cells to make protein, simply extracts the cells' natural protein-making machinery and then uses it to produce protein in vitro. Because living cells are no longer involved, scientists can freely adapt the protein production environment in ways not otherwise possible. However, improved versatility and yield of CFPS protein production is still the subject of considerable research. This work focuses on two ideas for furthering that research.The first idea is the adaptation of CFPS to make proteins containing unnatural amino acids. Unnatural amino acids are not found in natural biological proteins; they are synthesized artificially to possess useful properties which are then conferred upon any protein made with them. However, current methods for incorporating unnatural amino acids do not allow incorporation of more than one type of unnatural amino acid into a single protein. This work helps lay the groundwork for the incorporation of different unnatural amino acid types into proteins. It does this by using modified aminoacyl-tRNA synthetases (aaRSs), which are key components in CFPS, to be compatible with unnatural amino acids. The second idea is the preservation of DNA templates from enzyme degradation in CFPS. Among the advantages of CFPS is the option of using linear expression templates (LETs) in place of plasmids as the DNA template for protein production. Because LETs can be produced more quickly than plasmids can, using LETs greatly reduces the time required to obtain a DNA template for protein production. This renders CFPS a better candidate for high-throughput testing of proteins. However, LETs are more susceptible to enzyme-mediated degradation than plasmids are, which means that LET-based CFPS protein yields are lower than plasmid-based CFPS yields. This work explores the possibility of increasing the protein yield of LET-based CFPS by addition of sacrificial DNA, DNA which is not used as a protein-making template but which is degraded by the enzymes in place of the LETs. Andrew Broadbent cell-free protein synthesis (CFPS) unnatural amino acid incorporation aminoacyl-tRNA synthetase linear expression template (LET) aminoacylation assay sacrificial DNA Chemical Engineering
28	Aminoacyl-ARNt synthétases mitochondriales humaines : aspects fondamentaux et contribution à la compréhension de pathologies reliées / New properties of mitochondrial aminoacyl-tRNA synthetases and their connection to mitochondrial diseases Schwenzer, Hagen 21 October 2013 (has links) Les aminoacyl-ARNt synthetases (aaRS) sont impliquées dans le mécanismes de la traduction. Dans les cellules humaines, il existe deux jeux de gènes nucléaires codant pour les aaRS : un pour les aaRS cytosolique (cyt), le second pour les aaRS mitochondriales (mt). Les aaRS mt sont traduites dans le cytosole, adressées et importées dans la mitochondrie.Mutations dans 9 gènes d’aaRS mt ont été démontrées comme responsables de pathologies mitochondriales. Certaines des mutations n’affectent pas la propriété originelle d’aminoacylation. Il a été proposé que certaines de ces mutations puissent affecter des propriétés alternatives.Alors l’organisation des aaRS cyt est bien étudiée et que des implications dans des fonctions alternatives établies pour certaines d’entre elles, les connaissances quant aux aaRS mt restent parcimonieuses. L’objectif principal de ce manuscrit de thèse est: (i) révéler d’organisation sous-mt de l’AspRS mt; (ii) étendre l’analyse de l’organisation sous-mt à l’ensemble des aaRS mt; et (iii) contribuer à la compréhension de mécanismes moléculaires sous-jacents à certaines pathologies. Ces travaux ouvrent la porte vers d’autres investigations de l’organisation des aaRS à l’intérieur de la mitochondrie. Ces contributions seront utiles à la meilleure compréhension de mécanismes moléculaires sous-jacents à pathologies mitochondriales. / Aminoacyl-tRNA synthetases (aaRSs) are housekeeping enzymes involved in translation. In human cells, 2 different sets of nuclear genes code for aaRSs. One codes for cytosolic (cyt) aaRSs, and the second one codes for aaRSs of mitochondrial (mt) location. Mt-aaRSs are translated in the cytosol, targeted and imported into mitochondria.Mutations in 9 mt-aaRSs have been described. Some of the mutations do not display significant influence on the housekeeping aminoacylation activity. It has been proposed that those mutations affect alternative functions.Alternate functions have been described for cyt-aaRSs. While the organization of cyt-aaRSs is explored and their involvement into alternate functions established, the properties of the human mt-aaRSs remain unknown. On one site, this thesis integrate mt-AspRS into new functional networks (sub-mitochondrial localization and partnership). On the other site, it expand the view of the sub-mitochondrial organization to the full set of mt-aaRSs and should ultimately shed light into the molecular mechanisms underlying some of the pathologies. These results open the door for additional investigations to gain a complete view about the sub-mitochondrial organization of aaRSs. Those contributions will be of help for the understanding of molecular mechanisms underlying some mitochondrial disorders. Traduction mitochondriale Aminoacyl-ARNt synthétases Fonctions alternatives Organisation sous-mitochondriale Import Mutations reliées à des pathologies Évolution Mitochondrial translation machinery Aminoacyl-tRNA synthetase Non-translational functions Sub-mitochondrial organization Import Pathology-related mutations Evolution 572.8
29	Organisation sous-mitochondriale de l'aspartyl-ARNt synthétase humaine et implication dans le syndrome LBSL / Submitochondrial organization of human mitochondrial aspartyl-tRNA synthetase and its implication in LBSL disease Karim, Loukmane 04 October 2016 (has links) Les travaux présentés dans cette thèse ont eu pour objectif de contribuer à la compréhension du lien entre l’aspartyl-ARNt synthétase mitochondriale (AspRSmt) humaine et le syndrome LBSL, en étudiant les propriétés de cette enzyme au niveau cellulaire. Les objectifs étaient : 1) d’explorer l’organisation de l’AspRSmt dans la mitochondrie (Chapitre 1), 2) d’identifier la forme mature de l’AspRSmt après son import, ainsi que la localisation sous-mitochondriale de cette enzyme (Chapitre 2), 3) d’évaluer l’impact de quelques mutations, impliquées dans le syndrome LBSL, sur les propriétés de l’AspRSmt (Chapitre 3). Nous avons démontré que l’AspRSmt existe sous différentes formes de produits de maturation, et qu’elle est retrouvée, au moins, dans deux complexes, suggérant potentiellement différents partenaires et/ou fonctions pour cette enzyme. Nous avons établi la localisation sous-mitochondriale de l’AspRSmt, et démontré que cette dernière est doublement localisée avec une fraction soluble et une fraction périphérique interagissant avec la membrane. Nous avons également découvert que, sous certaines conditions de stress, l’AspRSmt est relarguée de la mitochondrie et pourrait avoir un lien avec le processus d’apoptose. En outre, nous avons évalué l’impact de quelques mutations, impliquées dans le syndrome LBSL, et trouvé qu’elles n’ont pas d’effet significatif sur les propriétés de l’AspRSmt. L’ensemble des résultats souligne, d’une part, les lacunes restant à combler concernant les propriétés de l’AspRSmt dans la compréhension du lien mutations/pathologie (LBSL), et d’autre part, suggère fortement l’existence d’une éventuelle fonction non canonique (alternative) de l’AspRSmt. / The aim of the PhD project was to contribute to the understanding of the link between mutations in the human mitochondrial aspartyl-tRNA synthetase (mt-AspRS) and LBSL disease, by studying the properties of this enzyme at the cellular level. Our objectives were: 1) to explore the organization of mt-AspRS in mitochondria (Chapter 1), 2) to identify the mature form of mt-AspRS after its import, and to characterize its submitochondrial localization (Chapter 2), 3) to assess, in cellulo, the impact of some LBSL-causing mutations on some properties of mt-AspRS (Chapter 3). We showed that mt-AspRS is processed into different mature forms, and that mt-AspRS belongs to two complexes likely suggesting different partners and/or functions. We demonstrated that mt-AspRS is dually localized with soluble and peripherally membrane-associated fractions. We also demonstrated that, under stress conditions, mt-AspRS is released outside mitochondria with a possible link to the apoptosis. Furthermore, we assessed the impact of some LBSL-causing mutation on some cellular properties of mt-AspRS, and showed that most mutations do not have a significant impact. This underscores the need for more studies about mt-AspRS properties, and strongly suggests a potential non-canonical (alternative) function of the enzyme. Traduction mitochondriale Aminoacyl-ARNt synthétase Fonction alternative Leukoencéphalopathie Organisation sous-mitochondriale Import/processing/maturation Mitochondrial translation Aminoacyl-tRNA synthetase Alternative function Leukoencephalopathy Submitochondrial localization Import/processing/maturation 572.8 616.83
30	Exploring Protein-Nucleic Acid Interactions Using Graph And Network Approaches Sathyapriya, R 03 1900 (has links) The flow of genetic information from genes to proteins is mediated through proteins which interact with the nucleic acids at several stages to successfully transmit the information from the nucleus to the cell cytoplasm. Unlike in the case of protein-protein interactions, the principles behind protein-nucleic acid interactions are still not very (Pabo and Nekludova, 2000) and efforts are still underway to arrive at the basic principles behind the specific recognition of nucleic acids by proteins (Prabakaran et al., 2006). This is mainly due to the innate complexity involved in recognition of nucleotides by proteins, where, even within a given family of DNA binding proteins, different modes of binding and recognition strategies are employed to suit their function (Luscomb et al., 2000). Such difficulties have also not made possible, a thorough classification of DNA/RNA binding proteins based on the mode of interaction as well as the specificity of recognition of the nucleotides. The availability of a large number of structures of protein-nucleic acids complexes (albeit lesser than the number of protein structures present in the PDB) in the past few decades has provided the knowledge-base for understanding the details behind their molecular mechanisms (Berman et al., 1992). Previously, studies have been carried out to characterize these interactions by analyzing specific non-covalent interactions such as hydrogen bonds, van der Walls, and hydrophobic interactions between a given amino acid and the nucleic acid (DNA, RNA) in a pair-wise manner, or through the analysis of interface areas of the protein-nucleic acid complexes (Nadassy et al., 1998; Jones et al., 1999). Though the studies have deciphered the common pairing preferences of a particular amino acid with a given nucleotide of DNA or RNA, there is little room for understanding these specificities in the context of spatial interactions at a global level from the protein-nucleic acid complexes. The representation of the amino acids and the nucleotides as components of graphs, and trying to explore the nature of the interactions at a level higher than exploring the individual pair-wise interactions, could provide greater details about the nature of these interactions and their specificity. This thesis reports the study of protein-nucleic interactions using graph and network based approaches. The evaluation of the parameters for characterizing protein-nucleic acid graphs have been carried out for the first time and these parameters have been successfully employed to capture biologically important non-covalent interactions as clusters of interacting amino acids and nucleotides from different protein-DNA and protein-RNA complexes. Graph and network based approaches are well established in the field of protein structure analysis for analyzing protein structure, stability and function (Kannan and Vishveshwara, 1999; Brinda and Vishveshwara, 2005). However, the use of graph and network principles for analyzing structures of protein-nucleic acid complexes is so far not accomplished and is being reported the first time in this thesis. The matter embodied in the thesis is presented as ten chapters. Chapter 1 lays the foundation for the study, surveying relevant literature from the field. Chapter 2 describes in detail the methods used in constructing graphs and networks from protein-nucleic acid complexes. Initially, only protein structure graphs and networks are constructed from proteins known to interact with specific DNA or RNA, and inferences with regard to nucleic acid binding and recognition were indirectly obtained . Subsequently, parameters were evaluated for representing both the interacting amino acids and the nucleotides as components of graphs and a direct evaluation of protein-DNA and Protein-RNA interactions as graphs has been carried out. Chapter 3 and 4 discuss the graph and network approaches applied to proteins from a dataset of DNA binding proteins complexed with DNA. In chapter 3, the protein structure graphs were constructed on the basis of the non-covalent interactions existing between the side chains of amino acids. Clusters of interacting side chains from the graphs were obtained using the graph spectral method. The clusters from the protein-DNA interface were analyzed in detail for the interaction geometry and biological importance (Sathyapriya and Vishveshwara, 2004). Chapter 4 also uses the same dataset of DNA binding proteins, but a network-based approach is presented. From the analysis of the protein structure networks from these DNA binding proteins, interesting observations relating the presence of highly connected nodes(or hubs) of the network to functionally important amino acids in the structure, emerged. Also, the comparison between the hubs identified from the protein-protein and the protein-DNA interfaces in terms of their amino acid composition and their connectivity are also presented (Sathyapriya and Vishveshwara, 2006) Chapter 5 and 6 deal with the graph and network applications to a specific system of protein-RNA complex (aminoacyl-tRNA synthetases) to gain insights into their interface biology based on amino acid connectivity. Chapter 5 deals with a dataset of aminoacyl-tRNA synthetase (aaRS) complexes obtained with various ligands like ATP, tRNA and L-amino acids. A graph based identification of side chain clusters from these ligand-bound aaRS structures has highlighted important features of ligand-binding at the catalytic sites of the two structurally different classes of aaRS (Class I and Class II). Side chain clusters from other regions of aaRS such as the anticodon binding region and the ligand-activation sites are discussed. A network approach is used in a specific system of aaRS(E.coli Glutaminyl-tRNA synthetase (GlnRS) complexed with its ligands, to specifically understand the effects of different ligand binding., in chapter 6. The structure networks of E.coli GlnRS in the ligand-free and different ligand-bound states are constructed. The ligand-free and the ligand-bound complexes are compared by analyzing their network properties and the presence of hubs to understand the effect of ligand-binding. These properties have elegantly captured the effects of ligand-binding to the GlnRS structure and have also provided an alternate method for comparing three dimensional structures of proteins in different ligand-bound states (Sathyapriya and Vishveshwara, 2007). In contrast to protein structure graphs (PSG), both the interacting amino acids and nucleotides (DNA/RNA) form the components of the protein-nucleic acid graphs (PNG) from protein-nucleic acid complexes. These graphs are constructed based on the non-covalent interactions existing between the side chains of the amino acids and nucleotides. After representing the interacting nucleotides and amino acids as graphs, clusters of the interacting components are identified. These clusters are the strongly interacting amino acids and nucleotides from the protein-nucleic acid complexes. These clusters can be generated at different strengths of interaction between the amino acid side chain and the nucleotide (measured in terms of its atomic connectivity) and can be used for detecting clusters of non-specific as well as specific interactions of amino acids and nucleotides. Though the methodology of graph construction and cluster identification are given in chapter 2, the details of the parameters evaluated for constructing PNG are given in chapter 7. Unlike in the previous chapters, the succeeding chapters deal exclusively with results that are obtained from the analyses of PNG. Two examples of obtaining clusters from a PNG are given, one each for a protein-DNA and a protein-RNA complex. In the first example, a nucleosome core particle is subjected to the graph based analysis and different clusters of amino acids with different regions of the DNA chain such as phosphate, deoxyribose sugar and the base are identified. Another example of aminoacyl-tRNA synthetase complexed with its cognate tRNA is used to illustrate the method with a protein-RNA complex. Further, the method of constructing and analyzing protein-nucleic acid graphs has been applied to the macromolecular machinery of the pre-translocation complex of the T. thermophilus 70S ribosome. Chapter 8 deals exclusively with the results identified from the analysis of this magnificent macromolecular ensemble. The availability of the method that can handle interactions between both amino acids and the nucleotides of the protein-nucleic acid complexes has given us the basis fro evaluating these interactions in a level higher than that of analyzing pair-wise interactions. A study on the evaluation of short hydrogen bonds(SHB) in proteins, which does not fall under the realm of the main objective of the thesis, is discussed in the Chapter 9. The short hydrogen bonds, defined by the geometrical distance and angle parameters, are identified from a non-redundant dataset of proteins. The insights into their occurrence, amino acid composition and secondary structural preferences are discussed. The SHB are present in distinct regions of protein three-dimensional structures, such that they mediate specific geometrical constraints that are necessary for stability of the structure (Sathyapriya and Vishveshwara, 2005). The significant conclusions of various studies carried out are summarized in the last chapter (Chapter 10). In conclusion, this thesis reports the analyses performed with protein-nucleic acid complexes using graph and network based methods. The parameters necessary for representing both amino acids and the nucleotides as components of a graph, are evaluated for the first time and can be used subsequently for other analyses. More importantly, the use of graph-based methods has resulted in considering the interaction between the amino acids and the nucleotides at a global level with respect to their topology of the protein-nucleic acid complexes. Such studies performed on a wide variety of protein-nucleic acid complexes could provide more insights into the details of protein-nucleic acid recognition mechanisms. The results of these studies can be used for rational design of experimental mutations that ascertain the structure-function relationships in proteins and protein-nucleic acid complexes. Protein-Nucleic Acid Interactions Protein-RNA Interactions Protein Structure Graphs Protein Nucleotide Graphs (PNG) Protein-DNA Complexes Protein-RNA Complexes Aminoacyl-tRNA Synthetase Glutaminyl-tRNA Synthetase (GlnRS) Proteins - Short Hydrogen Bonds Protein Structure Networks Protein-RNA Interaction Structure Graphs Protein-RNA Graphs 70S Ribosome Biochemical Genetics

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