Molecular Strategies in the Analysis of the Porcine Genome / Molekulargenetische Strategien zur Analyse des Schweinegenoms

Chen, Kefei

05 February 2004

No description available.

Agricultural Sciences

Schwein

PGK2-Gen

Phosphoglycerat-Kinase

Männliche Fruchtbarkeit

Mikrosatellitenentwicklung

Phylogenetische Studien

630 Landwirtschaft

Veterinärmedizin

Porcine

PGK2 Gene

Phosphoglycerate Kinase

Male Fertility

Microsatellite Isolation

Phylogenetic Analysis

48.64

Interactions entre Spiroplasma citri et son insecte vecteur Circulifer haematoceps : la phosphoglycérate kinase de S. citri : une « actin-binding protein » impliquée dans la transmission du spiroplasme par la cicadelle / Interactions between Spiroplasma citri and its insect vector Circulifer haematoceps : s .citri phosphoglycerate kinase : an actin-binding protein involved in the spiroplasma transmission by leafhoppers.

Labroussaa, Fabien

20 December 2010

Spiroplasma citri est un mollicute phytopathogène transmis de plante à plante par des cicadelles du genre Circulifer selon un mode persistant circulant-multipliant. Les franchissements de l’épithélium intestinal et des glandes salivaires sont basés sur un mécanisme d’endocytose/exocytose. Ce processus d’invasion met en jeu, au sein de complexes protéiques, des protéines bactériennes spécifiques qui reconnaissent des motifs déterminés présents à la surface des cellules eucaryotes. La recherche de protéines de l’insecte vecteur interagissant avec S. citri a notamment conduit à l’identification de l’actine. Cette interaction a pu être confirmée à la fois in vitro et in vivo. L’interaction de l’actine avec son partenaire chez S. citri, qui s’est avéré être la phosphoglycérate kinase (PGK), est impliquée dans l’internalisation du spiroplasme dans les cellules de l’insecte. La région minimale de liaison à l’actine de la PGK a également été déterminée.La réalisation d’un mutant de S. citri dépourvu de PGK a été entreprise avec le plasmide navette pGOT mais n’a pas permis la sélection de spiroplasmes mutés dans ce gène essentiel. Néanmoins, la recherche de l’évènement de recombinaison chez les clones obtenus a permis de mettre en évidence la mutation de deux gènes chez ces derniers.L'ensemble des protéines impliquées dans la transmission du spiroplasme, identifiées au préalable chez ce dernier, n’étant pas essentielle au cours de ce processus, une étude préliminaire des complexes multi-protéiques contenant plusieurs de ces protéines a été réalisée. L’identification de complexes impliquant à la fois la PGK, la P32 et les ScARPs pourrait permettre de mieux comprendre les mécanismes régissant la vection de S. citri par son insecte. / Spiroplasma citri is a phytopathogenic mollicute transmitted from plant to plant by leafhoppers of the genus Circulifer in a persistent and propagative manner on condition to cross the intestinal and salivary glands barriers of the insect. These crossings are based on a endocytosis/exocytosis mechanism which involves bacterial protein complexes in order to recognize specific patterns on the surface of eukaryotic cells.Specific molecular interactions between S. citri proteins and those of C. haematoceps were investigated using far Western technology and had notably led to the identification of actin. This interaction has been confirmed both in vitro and in vivo. The interaction of actin with his partner in S. citri, which has been identified as the phosphoglycerate kinase (PGK), is involved in the internalization of spiroplasma into the insect cells. The minimal actin-binding region of PGK was also determined.The realization of a S. citri PGK mutant was carried out using the shuttle plasmid pGOT but the selection of spiroplasmas mutated in this essential gene failed. Nevertheless, findings in the localization of recombination events in S. citri chromosome, allowed us to identify mutations in two genes that could be tested in our experimental transmission system.The set of proteins involved in the spiroplasmal transmission, previously identified as non essential proteins in the invasion process, prompted us to study the role of multi-protein complexes containing several of these proteins. Identification of complexes involving both the PGK, the P32 and ScARPs should enable us to better understand mechanisms governing the transmission of S. citri by its insect.

Mollicute phytopathogène

Spiroplasma citri

Transmission

Insecte vecteur

Actine

Phosphoglycérate kinase

Interactions protéine-protéine

Phytopathogenic mollicute

Spiroplasma citri

Transmission

Insect vector

Actin

Phosphoglycerate kinase

Protein-protein interactions

Functional Characterization Of Rv0754(PE_PGRS11) : A Multifunctional PE_PGRS Protein From Mycobacterium Tuberculosis

Chaturvedi, Rashmi

07 1900

Mycobacterium tuberculosis, the causative agent of pulmonary tuberculosis, infects one-third of the world’s human population. Despite the multiplicity of antimicrobial mechanisms mounted by its host, M. tuberculosis shows a remarkable ability to survive either by evoking survival strategies or by interference with critical macrophage functions that are required to successfully respond to the infection. It has been postulated that the outcome of exposure to M. tuberculosis (in terms of disease symptoms) largely depends upon the selective gene expression of tuberculosis bacilli along with activation of specific signaling pathways in the infected host cells during different phases of infection. In this perspective, determination of the complete genome sequence of Mycobacterium tuberculosis has provided crucial information with respect to the physiology of this bacterium and the pathogenesis of tuberculosis. However, putative functional annotation to all hypothetical proteins coded by M. tuberculosis genome remains complex. One important outcome of the genome-sequencing project was the discovery of two new multigene families designated PE and PPE. About 10% of the M. tuberculosis coding capacity is devoted to the PE and PPE genes, named for the Pro-Glu (PE) and Pro-Pro-Glu (PPE) motifs near the N terminus of their gene products. In addition to these motifs, proteins of PE family share N-terminal domains of approximately 100 amino acids, whereas the PPE proteins possess an N-terminal domain of about 180 amino acids. Many PE and PPE proteins are composed only of these N-terminal homologous domains. However, other members possess an additional C-terminal segment of variable length, often composed of multiple copies of polymorphic GC rich sequences (PGRS). The uniqueness of the PE genes is further illustrated by the fact that these genes are restricted to mycobacteria. However, despite their abundance in mycobacteria, very little is known regarding the expression or the functions of PE family genes. Although the PE and PPE families of mycobacterial proteins are the focus of intense research, no precise function has so far been unraveled for any member of these families. In perspective of above-mentioned observations, we have chosen Rv0754 as a representative PE family gene. Rv0754 was shown to be upregulated in tubercle bacilli upon infection of bone marrow derived macrophages as well as in M. tuberculosis isolated from alveolar macrophages of infected mice. In the current investigation, we demonstrate that Rv0754 is hypoxia responsive gene based on promoter or transcript expression analysis. Further, extensive bioinformatics analysis predicated that Rv0754 posses possible Phosphoglycerate Mutase domain, an enzyme known for its significant role not only in the glycolytic pathway of the carbohydrate metabolism, but also for the crucial cell fate decision during conditions like oxidative stress as well as infection. Experimental data clearly suggests that hypoxic environment dependent expression of Rv0754 imparts resistance to macrophages from oxidative stress. These findings could be attributed to the presence of catalytically active Phosphoglycerate Mutase domain of Rv0754. More often, sophisticated regulation/modulation of key signaling events regulate the critical cell fate decisions during oxidative stress. In this context, TLR2 dependent triggering of PI3K-ERK1/2- NF-κB signaling axis by Rv0754 may be operative in imparting resistance to oxidative stress. Further, Rv0754 triggers COX-2 expression by activating PI3K-ERK1/2-NF-κB cascade in mouse macrophages. These observations are of relevance as Rv0754 is associated with cell wall and is exposed outside the surface of the bacterium suggesting the possible access to intracellular compartments of the infected macrophages. Additionally, Rv0754 elicited humoral antibody reactivities in a panel of human sera or in cerebrospinal fluid samples obtained from different clinical categories of tuberculosis patients. DNA immunizations experiments in mice clearly suggested that Rv0754 is an immunodominant antigen demonstrating significant T cell and humoral reactivity. These observations clearly advocate that Rv0754 protein is expressed in vivo during active infection with M. tuberculosis and that the Rv0754 is immunogenic. Taken together, our findings suggest that Rv0754 is a novel PE_PGRS protein with unique features which could generate conditions that favor survival of the mycobacteria.

PE-PGRS Protein

Mycobacterium Tuberculosis

Multifunctional Protein

Rv0754 Protein

Oxidative Stress

P13 Kinase

Mycobacteria

Rv1818c

Phosphoglycerate Mutase (PGM)

Microbiology