Caracterização do Gene NtCDKG;2 Expresso no Pistilo de Nicotiana tabacum L. / Characterization of the Gene NtCDKG;2 Expressed in Nicotiana tabacum L. Pistil

Greice Lubini

18 October 2012

A biologia da reprodução sexual de plantas é um campo de pesquisa de grande importância, já que a maioria dos alimentos consumidos pelo homem é composta de partes reprodutivas das plantas (frutos e sementes), oriundas do desenvolvimento de partes do pistilo fertilizado. Em Nicotiana tabacum, identificou-se um gene específico de estigma/estilete, SCI1 (Stigma/style Cell-cycle Inhibitor 1), que atua na inibição da proliferação celular (DePaoli et al., 2011). Através de ensaios de pull-down, verificou-se a interação da proteína SCI1 com uma proteína quinase dependente de ciclina (CDK) (Strini, dados não publicados). Este trabalho visou à caracterização dessa nova CDK, ortóloga da CDKG;2 de Arabidopsis. A sequência correspondente de N. tabacum (NtCDKG;2) foi amplificada por PCR, a partir de cDNAs de estigmas/estiletes, clonada e sequenciada, o que permitiu a confirmação de sua identidade. A expressão de NtCDKG;2 foi analisada nos diferentes órgãos vegetativos e reprodutivos, por qRT-PCR, o que evidenciou um perfil de expressão ubíqua. Ao estudar o perfil de expressão desse gene nos estigmas/estiletes dos doze estádios de desenvolvimento floral de N. tabacum, observa-se que NtCDKG;2 é mais expresso nos estádios tardios do desenvolvimento em direção à antese, indicando uma função importante de sua proteína ao final do desenvolvimento do pistilo. Análises de expressão de NtCDKG;2 em estigmas/estiletes, de plantas de N. tabacum com produção aumentada do hormônio auxina no pistilo, sugerem que NtCDKG;2 é regulado transcricionalmente por esse hormônio. A expressão transiente da proteína de fusão NtCDKG;2-GFP, em folhas de N. tabacum, evidenciou a localização nuclear da proteína em estudo. Também foram geradas plantas transgênicas estáveis com superexpressão e com silenciamento por RNAi de NtCDKG;2. Apesar dos altos níveis de transcritos de NtCDKG;2 nas plantas de superexpressão e dos baixos níveis nas plantas silenciadas, não foram observadas alterações fenotípicas macroscópicas nessas plantas. Adicionalmente, obteve-se a expressão da proteína NtCDKG;2, fusionada a uma tag de histidina em sua porção N-terminal, em células de Escherichia coliBL21(DE3)CodonPlusRP. Através dos estudos realizados neste trabalho e análises conjuntas da literatura, é possível propor que NtCDKG;2 codifique uma proteína que está envolvida no controle do ciclo celular nos estigmas/estiletes de N. tabacum. / The biology of plant sexual reproduction is a research field of great importance, since most of the food consumed by humans is composed of plant reproductive parts (fruits and seeds), originated by the development of fertilized pistil parts. In Nicotiana tabacum, it was identified a stigma/style-specific gene, SCI1 (Stigma/style Cell-cycle Inhibitor 1), which acts in the inhibition of cell proliferation (DePaoli et al., 2011). Through pull down assays, the interaction of the SCI1 protein with a cyclin-dependent protein kinase (CDK) was verified (Strini, unpublished). This work aimed the characterization of this new CDK, orthologous to the Arabidopsis CDKG;2. The N. tabacum corresponding sequence (NtCDKG;2) was PCR amplified, from stigmas/styles cDNAs, cloned and sequenced, which allowed the confirmation of its identity. The NtCDKG;2 expression was analyzed in the different vegetative and reproductive organs, by qRT-PCR, evidentiating an ubiquitous expression pattern. Studying the expression pattern of this gene in stigmas/styles of the twelve stages of N. tabacum flower development, it was observed that NtCDKG;2 is more expressed at the later developmental stages towards anthesis, indicating an important function of its protein in the end of pistil development. NtCDKG;2 expression analyses in stigmas/styles of N. tabacum plants with an enhanced auxin production in the pistil suggest that NtCDKG;2 is transcriptionally regulated by this hormone. The transient expression of the fusion protein NtCDKG;2-GFP, in N. tabacum leaves, evidentiated the nuclear localization of the studied protein. Stable transgenic plants overexpressing and silencing NtCDKG;2 by RNAi were also generated. Despite the high transcript levels in the plants overexpressing NtCDKG;2 and the low transcript levels in the silencing plants, macroscopic phenotypic alterations were not observed on these plants. Additionally, the expression of the NtCDKG;2 protein, with a histidine tag fused in its N-terminal, was obtained in Escherichia coli BL21(DE3)CodonPlusRP cells. Through studies performed on this work and literature analyses, it is possible to propose that NtCDKG;2 encodes a protein that is involved in the control of cell cycle at the N. tabacum stigmas/styles.

CDKs

Ciclo celular

Desenvolvimento do pistilo

Expressão heteróloga

Localização subcelular

Plantas transgênicas

CDKs

Cell cycle

Heterologous expression

Pistil development

Subcellular localization

Transgenic plants

Variabilité et déterminants de la bioaccumulation des métaux par les poissons marins : cas du Grand Ecosystème Marin du Courant des Canaries / Variability and determinants of metal bioaccumulation by marine fish : case study of the Canary current

Le Croizier, Gaël

13 June 2017

Le Grand Ecosystème Marin du Courant des Canaries est un des principaux systèmes mondiaux d’upwelling et assure une des plus importantes productions de pêche parmi les grands écosystèmes marins d’Afrique. Cet écosystème est soumis à des apports en éléments métalliques entraînant leur accumulation par les organismes marins et notamment les poissons. En termes de bioaccumulation, une forte variabilité est observée entre les espèces exploitées mais également entre individus d’une même espèce. Ce travail de thèse se propose de caractériser les paramètres majeurs qui déterminent l’accumulation des métaux par les poissons marins, en prenant pour cas d’étude l’écosystème du courant des Canaries. Deux approches ont été adoptées, l’une portant sur les particularités physiologiques et l’autre sur les mécanismes écologiques régissant la bioaccumulation. A un premier niveau d’intégration, les caractéristiques physiologiques spécifiques telles que l’efficacité d’assimilation, les concentrations en métallothionéines et le mode de séquestration des métaux agissent sur la bioaccumulation. Ensuite, à un second niveau, la nature des proies joue un rôle crucial sur l’exposition aux métaux du fait de la dominance de la voie de transfert trophique chez les poissons marins. A un dernier niveau d’intégration, l’habitat représente un paramètre déterminant, principalement en influant sur les niveaux de contamination des proies soumis au cycle des métaux dans l’environnement marin. Cette thèse a présenté une approche innovante, en proposant une étude intégrée de la cellule à l’écosystème en passant par l’individu, dédiée à la compréhension d’un mécanisme impliquant des répercutions tant sur la préservation des ressources marines que sur la santé des consommateurs. / The Canary Current Large Marine Ecosystem in West Africa is one of the most productive upwelling ecosystems. It is subjected to anthropogenic inputs leading to metal accumulation by marine fish species, which show a great variability in terms of metal concentrations. This PhD work aims to characterize the major parameters determining metal accumulation by marine fish, based on the case study of the Canary current. Two main approaches were developed concerning physiological and ecological features. At a first integration level, physiological characteristics such as assimilation efficiency, metallothionein concentrations and subcellular metal partitioning influence bioaccumulation. At a second level, prey composition plays a key role due to the dominance of metal accumulation through dietary intakes in marine fish. Finally, habitat drives metal exposure to fish due to the biogeochemical cycle of the metal elements.This study proposed an innovating approach, combining analyses from the cellular level to the ecosystem one, including the individual level, and aiming for a thorough comprehension of a mechanism implying consequences on marine resource conservation and human safety.

Eléments métalliques

Poissons marins

Répartition subcellulaire

Cinétiques d’accumulation

Ecologie trophique

Metal elements

Marine fish

Subcellular partitioning

Accumulation kinetics

Trophic ecology

577.7

The localisation and regulation of phosphatidylinositol-4-phosphate 5-Kinase gamma splice variants and the discovery of a new mammalian splice variant, PIP5KIγ_v6

Xia, Yang

January 2011

Type I PIP kinases (phosphatidylinositol 4-phosphate 5-kinases, PIP5Ks) catalyse the majority of cellular synthesis of PI(4,5)P2. To date, three mammalian isoforms (r1, r2, r3) have been found. PIP5KIr is subject to complex C-terminal splice variation, enhancing its transcriptional diversity through evolution and producing at least 5 known spliceoforms in the mammals. This study addresses several important questions. (1) Several remarkable differences have been discovered between the neuronal splice variant PIP5KIr_i3 and its close variant, Ir_i2, whose peptide lacks a 26-AA insert near its C-terminus. This study attempts to map these behavioural differences onto motifs within the peptide insert. Furthermore, a site of point mutation is identified near the activation loop, which amplifies the above differences. (2) This study documents properties of the more recently discovered PIP5KIr_i3, about which relatively little is known, for example, the regulation of its subcellular localisation, kinase activity and post-translational modifications. By site-directed mutagenesis and examining more closely several crucial motifs, insight is gained into the putative relationship between the enzyme’s phosphorylation state, cellular localisation, lipid kinase activity and autophosphorylation. (3) The discovery of a new PIP5KIr splice variant, Ir_v6, is described. First discovered in rodents, PIP5KIr_i6 encompasses the 26-AA insert of Ir_i3, but lacks the common C-terminus of Ir_i2 and Ir_i3 which contains peptide motifs that have several roles in vivo. A polyclonal antibody against the C-terminus of Ir_i6 was also developed. Preliminary characterisation of Ir_i6 demonstrates a similar subcellular localisation, but a wider expression profile than its close relative, Ir_i3, suggesting potentially differential functions across tissues and at various developmental stages. (4) The existence of Ir_v3 and Ir_v6 is also confirmed in humans. In light of recent findings of other novel human spliceoforms, this is shown to be a case of intra-exonic splicing producing “alternative 5’ splice site” exons in the human. Overall, this thesis should help to better understand the regulation and physiological roles of PIP5KIr and, specifically, its different splice variants.

615.1

Caractérisation de la protéine 140K impliquée dans l’adressage aux chloroplastes des complexes de réplication du virus de la mosaïque jaune du navet (TYMV) / Characterization of the 140K protein involved in targeting to the chloroplasts of the replication complexes of the Turnip Yellow mosaic virus (TYMV) replication complexes

Moriceau, Lucille

21 December 2015

Le virus de la mosaïque jaune du navet (TYMV) possède un génome monopartite constitué d’ARN de polarité positive codant pour trois protéines, dont seule la polyprotéine 206K est indispensable à la réplication virale.Elle subit une maturation protéolytique, générant les protéines 140K et 66K, localisées au niveau de l’enveloppe des chloroplastes, siège de la réplication virale.Adressée aux chloroplastes, la protéine 140K y recrute la 66K et se comporte comme une protéine intégrale membranaire.Le domaine d’adressage aux chloroplastes (DAC) de la protéine 140K a été défini grâce à la transfection et à des protoplastes d’Arabidopsis thaliana par différentes constructions codantpour des versions délétées de la protéine fusionnées à l’EGFP, et à leur observation en microscopie confocale. Le DAC comprend deux hélices alpha amphipathiques dont la présence a été attestée par dichroïsme circulaire. Leur nécessité pour la localisation aux chloroplastes, l’association aux membranes et la réplication virale, a été étudiée. Différents patterns de distribution subcellulaire de la protéine 140K ont été observés. Ils sont corrélés au taux d’expression de la protéine. Sa dimérisation a également été démontrée.L’implication d’autres résidus du DAC dans la localisation subcellulaire, la dimérisation et la réplication virale, a également été recherchée. / Turnip yellow mosaic virus (TYMV) is a positive single-stranded RNA virus. Among the three ORFs encoded by the TYMV genome, 206K is the only protein required for viral replication. It is cleaved into 140K and 66K, which are both present at the chloroplast envelope membrane, where viral replication takes place.The 140K protein is targeted to chloroplasts, where it recruits 66K, and behaves as an integral membrane protein. The chloroplast targeting domain (DAC) of the 140K protein was defined using Arabidopsis thaliana protoplasts transfected by various constructs encoding deleted versions of 140Kfused to EGFP and subsequent confocal microscopy. The DAC comprises two amphipathic alpha helices, as confirmed by circular dichroism. Their involvement in chloroplast localisation and membrane association has been assessed, as well as their contribution to viral replication.We observed different subcellular distribution patterns of 140K protein, which correlate with the expression level of the protein. Its capability to dimerize has also been demonstrated.The involvement of other DAC residues in subcellular localisation, dimerization and viral replication has been studied.

Virus à ARN de polarité positive

Complexe de réplication

Localisation subcellulaire

Hélice alpha amphipathique

Microscopie confocale

Positive strand RNA virus

Replication complex

Subcellular localization

Amphipathic alpha helix

Confocal microscopy

Abnormal Localization and Accumulation of FLT3-ITD, a Mutant Receptor Tyrosine Kinase Involved in Leukemogenesis

Koch, Sina, Jacobi, Angela, Ryser, Martin, Ehninger, Gerhard, Thiede, Christian

January 2008

Aberrant subcellular localization of mutant transmembrane receptors is increasingly acknowledged as a possible mechanism for an altered signaling quality leading to transformation. There is evidence that mutated receptor tyrosine kinases of subclass III, for example the platelet-derived growth factor receptor (PDGFR) and KIT-protein, are aberrantly localized in human cancers. In order to further analyze this phenomenon, we investigated the localization of FLT3, a subclass III receptor tyrosine kinase frequently mutated in leukemia. By immunofluorescence staining and confocal laser scanning microscopy we found that in retrovirally transduced COS7 cells, wild type FLT3 receptor protein is localized primarily at the cell surface. In contrast, a mutant FLT3 receptor protein with an internal tandem duplication (ITD) accumulates in a perinuclear region and is not detectable at the plasma membrane. Surprisingly, and in contrast to previously published data, intracellular FLT3-ITD accumulation could neither be detected in the endoplasmic reticulum (ER) nor in the Golgi apparatus. Furthermore, transient overexpression per se leads to accumulation of wild type FLT3 receptor protein in the ER in addition to surface localization, probably due to inefficient intracellular transport by the overloaded sorting machinery of the secretory pathway. Based on our data and the immature glycosylation pattern of FLT3-ITD, we speculate that the mutant protein resides most probably in an unidentified compartment of the secretory pathway between the ER and the Golgi apparatus. / Dieser Beitrag ist mit Zustimmung des Rechteinhabers aufgrund einer (DFG-geförderten) Allianz- bzw. Nationallizenz frei zugänglich.

info:eu-repo/classification/ddc/610

ddc:610

Buněčná lokalizace rezistentních proteinů Vga(A)LC a Msr(A) prostřednictvím fluorescenční mikroskopie / Subcellular localization of resistant proteins Vga(A)LC and Msr(A) using fluorescence microscopy

Nguyen Thi Ngoc, Bich

January 2018

Vga(A)LC and Msr(A) are clinically significant resistant proteins in staphylococci that confer resistance to translational inhibitors. They belong to ARE ABC-F protein subfamily, which is part of ABC transporters. Unlike typical ABC transporters, ABC-F proteins do not have transmembrane domains that are responsible for the transport of substances through the membrane. Therefore, they do not have characteristic transport function but regulatory or resistance function. Their mechanism of action on the ribosome has been described only recently, where these proteins displace the antibiotic from the ribosome. However, some aspects of their function are still unclear. For example, what is the function of the Vga(A) location on a membrane that has been detected in the membrane fraction but not in the ribosomal. In this work, using fluorescence microscopy, I observed subcellular localization of the Vga(A)LC-mEos2, Vga(A)LC-GFP and Msr(A)-eqFP650 resistant fusion proteins in live cells of S. aureus under different culture conditions . It has been shown that Vga(A)LC-GFP and Msr(A)-eqFP650 occur in a foci near the membrane. Depending on ATPase activity or the presence of an antibiotic, the localization of Msr(A)-eqFP650 in the cell changes from focal to diffuse, presumably on ribosomes, suggesting a...

Simultaneous Electrophysiological and Morphological Assessment of Impact Damage to Nerve Cell Networks

Rogers, Edmond A.

05 1900

A ballistic pendulum impulse generator was used to impact networks in primary culture growing on microelectrode arrays. This approach has the advantage of imparting pure tangential acceleration insults (50 to 300 g) with simultaneous morphological and electrophysiological multichannel monitoring for days before and after the impact. Action potential (AP) production, network activity patterns, and cell electrode coupling of individual units using AP waveshape templates were quantified. Network adhesion was maintained after tangential impacts up to 300g with minimal loss of pre-selected active units. Time lapse phase contrast microscopy revealed stable nuclei pre-impact, but post impact nuclear rotation in 95% of observations (n= 30). All recording experiments (n=31) showed a repeatable two-phase spike production response profile: recovery to near reference in 1-2 hrs, followed by a slow activity decay to a stable, level plateau approximately 30-40% below reference. Phase 1 consisted of a complex two-step recovery: rapid activity increase to an average 23.6% (range: 11-34%) below reference, forming a level plateau lasting from 5 to 20 min, followed by a climb to within 20% of reference where a second plateau was established for 1 to 2 hrs. Cross correlation profiles showed changes in firing hierarchy after impact, and in spontaneous network oscillatory activity. Native oscillations were found in the Delta band (2 to 3 Hz), and decreased by approximately 20% after impact. Under network disinhibition with bicuculline, oscillations were slower (0.8-1Hz) and decreased 40% after impact. These data link network performance deficits with microscopically observable subcellular changes.

impact trauma

network dynamics

electrophysiology

subcellular damage

nuclear rotation

functional damage

Biology, Neuroscience

Biophysics, Medical

Engineering, Biomedical

Neural circuitry.

Brain damage -- Animal models.

Electrophysiology.

Mechanisms Underlying the Regulation and Functions of HDAC7

Gao, Chengzhuo

22 July 2008

No description available.

Biochemistry

Cellular Biology

Molecular Biology

HDAC7

subcellular distribution

transcriptional activity

CRM1

14-3-3

CaMK

PML NBs

PML sumoylation

SUMO E3 ligase

PML NB formation

Myogenesis

THE FUNCTION OF CALCIUM/CALMODULIN DEPENDENT PROTEIN KINASE II IN CELL CYCLE REGULATION

BEAUMAN, SHIRELYN RAE

30 June 2003

No description available.

Cyclin B1

subcellular localization

cell cycle

Targeting Motifs

Subcellular and functional analyses of two small heat shock proteins and protein kinases from peroxisomes of Arabidopsis thaliana L. / Subzelluläre und funktionelle Analysen von zwei kleinen Hitzeschockproteinen und Proteinkinasen von Peroxisomen aus Arabidopsis thaliana L.

Ma, Changle

19 January 2006

No description available.

570 Biowissenschaften, Biologie

Mathematics and Computer Science

Chaperonen

Protein-Kinasen

GFP

Peroxisomen

oxidativem Stress

subzellulares zielendes Signal

Chaperones

protein kinase

green fluorescent protein

peroxisome

oxidative stress

subcellular targeting signal

42 Biologie

W Biologie