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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
21

Estudos termodinâmicos e estruturais da interação cabeça-cauda da , alpha-tropomiosina muscular / Thermodynamic and structural studies of the head-to-tail complex of the muscular alpha-Tropomyosin

Corrêa, Fernando 20 June 2008 (has links)
Tropomiosina (Tm) é uma das proteínas que compõe o filamento fino (actina, Tm, Troponina) do sistema muscular esquelético e desempenha um importante papel na regulação da contração muscular. Tm é um coiled-coil de 284 resíduos que forma longos homopolímeros lineares através da sobreposição de onze resíduos entre os terminais de Tms adjacentes (Interação cabeça-cauda) em condições de baixa força iônica. A presença de vários resíduos carregados (D2, K5, K6, K7, D275, H276 e D280) nas extremidades da Tm sugere que contatos intermoleculares eletrostáticos entre estes aminoácidos podem ter um importante papel na estabilidade dos polímeros. Entretanto, a estrutura do complexo cabeça-cauda demonstra que a maioria dos contatos intermoleculares na interface é de natureza hidrofóbica. A fim de analisarmos a contribuição dos grupos carregados para a estabilidade do complexo cabeça-cauda, construímos fragmentos recombinantes correspondentes à metade amino (ASTm1-142 ) e carboxi (Tm143-284(5OHW269)) terminais da proteína contendo mutações pontuais daqueles resíduos para alanina, e adicionalmente H276 para Glu. Medimos a afinidade entre todas as possíveis combinações destes fragmentos na ausência e presença de íons Mg2+, visto que este cátion está sempre presente em condições fisiológicas e é importante para estabilizar a interação entre Tm e actina. Os efeitos das mutações foram analisados por simulações de docking, desnaturações térmicas e ciclos de duplos mutantes. Os resultados demonstram que os aminoácidos K5, K7 e D280 presentes na interface formam contatos intermoleculares essenciais para a estabilidade do complexo. Enquanto, D2, K6, D275 e H276 não participam na formação de contatos intermoleculares, no entanto, contribuem para a estabilidade da interação cabeça- cauda através de suas interações intramoleculares que atuam na estabilidade das hélices individuais. Os aumentos na estabilidade da metade C-terminal da Tm (Tm143-284(5OHW)) induzidos por Mg2+ foram dependentes das mutações neste trecho da proteína sugerindo a presença de um sítio de ligação para este íon na extremidade carboxi terminal da molécula no trecho que forma a interação cabeça- cauda. Construímos um fragmento menor do C-terminal (Tm259-284(W269)) para acompanharmos mudanças no deslocamento químico induzidas pela ligação do íon usando ressonância magnética nuclear. Os resultados obtidos comprovaram nossa hipótese e nos permitiram definir pela primeira vez que a estrutura da Tm tem um ou mais sítios de ligação Mg2+ em uma região próxima ao resíduo H276 que está localizado entre vários resíduos carregados negativamente que participam da interação cabeça-cauda. Por último, estudamos os efeitos de solventes cosmótropicos (TFE e glicerol) nas estabilidades dos fragmentos da Tm, uma vez que a instabilidade (flexibilidade) da extremidade C-terminal é importante para a formação do complexo cabeça-cauda. Observamos que TFE, porém não glicerol, reduziu a afinidade entre os terminais. Ambos os co-solventes induziram aumentos na estabilidade dos fragmentos, no entanto, apenas TFE induziu um aumento no conteúdo de α-hélice e causou uma redução significativa na cooperatividade de desenovelamento das proteínas. Estes resultados indicam que estes compostos orgânicos estabilizam as estruturas dos fragmentos individuais da Tm de maneiras diferentes e que estas diferenças podem estar relacionadas aos diferentes efeitos observados na formação da interação cabeça-cauda. / Tropomyosin (Tm) is a protein component of the skeletal muscle thin filament (actin, Tm, Troponin) which has an important role in the regulation of muscle contraction. Tm is a dimeric coiled-coil (284 aminoacids) which forms long linear homopolymers through the overlap of eleven residues of adjacent Tm termini (Head- to-tail interaction) in low ionic strength conditions. The presence of several charged amino acids (D2, K5, K6, K7, D275, H276 e D280) in Tm extremities suggests that electrostatic contacts among those residues may have an important role in the stability of the polymers. Nevertheless, the solution structure of the head-to-tail complex demonstrated that most of the contacts in the interface are hydrophobic. In order to study the contribution of these charged residues to the stability of the head- to-tail complex, we built recombinant fragments corresponding to the amino (ASTm1-142) and carboxy (Tm143-284(5OHW269)) termini containing single mutations of those amino acids to alanine, and additionally a substitution of H276 for Glu. We measured the binding affinities among all possible combinations of wild-type and mutant fragments in the absence or presence of Mg2+ ions. This cation is always physiologically present in the muscle and it is known to strengthen the binding of Tm to actin. The effects of the mutations were analyzed by protein-protein docking, thermodynamic cycles and thermal denaturations. The results show that residues K5, K7 and D280 are essential to the stability of the complex. Though D2, K6, D275 and H276 are exposed to the solvent and do not participate in intermolecular contacts in the NMR structure, they may contribute to the complex stability by modulating the stability of the helices at the Tm termini. Mg2+-induced increases in stability of the C- terminal were sensitive to mutations in residues located in the head-to-tail overlap region, suggesting that Mg2+ ions may bind specifically to the carboxy extremity of the protein. We produced a small peptide (Tm259-284(W269)) to follow amide chemical shift perturbations upon Mg2+ binding by nuclear magnetic resonance measurements. The results obtained with this peptide allowed us to define for the first time that the Tm structure has one or more Mg2+ binding sites in a region centered in the vicinity of H276 in which are located several negatively charged residues that participate in the head-to-tail interaction. We also studied the effects of kosmotropic co-solvents (TFE and glycerol) in the stability of Tm fragments, as the instability (flexibility) of the C- terminal region has been pointed as important for the formation of the head-to-tail complex. We observed that TFE, but not glycerol, reduces the affinity between the termini. Both TFE and glycerol increased the stability of the isolated N- and C- terminal fragments; however, only TFE caused an increase in the helical content and a significant reduction in the cooperativity of unfolding of the proteins. Our results show that these two co-solvents stabilize the structures of individual Tm fragments in different manners and that these differences may be related to their different effects on head-to-tail complex formation.
22

Hydrodynamics in the Calibration of Optical Tweezers for Coiled-Coil Studies

Ehrlich, Christoph 13 November 2019 (has links)
Coiled-coil motifs are part of 5–10 % of the eukaryotic proteome and are involved in important cellular processes such as membrane trafficking, chromosome segregation or mechanosensing. Their canonical form is well understood and based on a heptad repeat with hydrophobic amino acids at positions 1 and 4. A sequence of these peptides folds into an α-helix and two, or more, of these helices bind together by winding around each other, covering up the hydrophobic residues and giving rise to the coiled-coil structure. Coiled-coil proteins appearing in nature do, however, deviate from this form by introducing discontinuities into the heptad repeat. The effect of these imperfections on the structure is only known for few cases and not generally understood or predictable. The additional impact of these discontinuities on the dynamic function of coiled-coil domains is unknown altogether. Here, in order to tackle these questions, the adhesive forces between the α-helices are studied in single-molecule experiments. To measure these small forces (∼ pN) with a high spatial and temporal resolution, a dual-trap optical tweezers setup was constructed. Special emphasis was put on realizing the required high resolution, a large degree of automation and versatility during the building process. The instrument’s performance was assessed by recording force-extension curves of DNA yielding results for the molecular parameters persistence length and stretch modulus in good agreement with those found in the literature. Additionally, the Allan deviation was computed for different configurations of beads and a high stability and resolution of the instrument was found with optimal performance on the time scale of 1–10 s. Optical tweezers require calibration to accurately measure forces. To this end, generally a scheme is used that leverages the Brownian motion of a trapped object in the harmonic potential, created by the laser focus, to determine the parameters required to convert the analog voltage signal to distances and forces. However, this approach requires prior knowledge of the bead’s drag coefficient. A method was suggested previously that allows to measure this parameter by exciting the trapped bead through an external fluid flow and observing its response. Yet, this scheme was proposed for single-trap devices only. The precision and versatility of the new instrument was increased by extending this technique to work with two traps and implementing it in the apparatus. To this aim, the underlying equations of a trapped bead’s motion were modified to include hydrodynamic interactions between the objects resulting from the external fluid flow. It was found that a single multiplicative factor is sufficient to correct the calibration results for the hydrodynamic effects and ensure precise calibration. The drag coefficient of several beads yielded the same result for a single and two traps within the measurement error thus confirming the validity of the method. The newly built instrument was then used to study the coiled-coil protein early endosome antigen 1 (EEA1). This 200 nm long homodimer was shown to undergo an entropic collapse upon binding a small GTPase at the N-terminus. For further investigations of this effect and the adhesives forces at play, an experiment was designed here to unzip the two α-helices of the protein. To this end, DNA handles were attached to each of the two helices using a sortase A based ligation reaction as force moderators and first optical tweezers experiments were performed with the protein-DNA chimera. Thus, the necessary tools for unzipping assays of EEA1 are now at hand to further research the entropic collapse process. To summarize, a dual-trap optical tweezers setup was built, the calibration routine extended and realized in a more precise way and the instrument was used to investigate binding energies of EEA1 α-helices. / Coiled-Coil Strukturmotive sind in 5–10 % aller Proteine von Eukaryoten vertreten und wichtiger Teil zellulärer Prozesse wie Membrantransport, Segregation von Chromosomen oder Mechanoperzeption. Ihre grundlegende Struktur besteht aus dem sogenannten Heptadenmuster, einer Sequenz aus sieben Aminosäuren mit hydrophoben Molekülen an Position eins und vier. Eine Reihe dieser Muster kann sich zu einer α-Helix falten und zwei, oder mehr, solcher Helices sich umeinander winden, um die hydrophoben Moleküle abzuschirmen. Das Ergebnis ist eine Coiled-Coil- oder Doppelwendelstruktur. Natürlich vorkommende Coiled-Coil Proteine weichen jedoch durch Fehlstellen im Heptadenmuster von dieser kanonischen Form ab. Die Auswirkung dieser Störstellen auf die Struktur des gesamten Moleküls ist bisher nur für einige wenige Fälle untersucht und nicht allgemein vorstanden oder vorhersagbar. Der zusätzliche Einfluss dieser Fehlstellen auf die Funktion und dynamischen Prozesse solcher Proteine ist gänzlich unbekannt. Um diesen Fragen nachzugehen werden hier die Bindungskräfte zwischen den α-Helices in Einzelmolekülstudien untersucht. Um diese winzigen Kräfte (∼ pN) mit hoher räumlicher und zeitlicher Auflösung untersuchen zu können, wurde im Rahmen der vorliegenden Arbeit eine optische Doppelfalle konstruiert. Besonderes Augenmerk lag dabei auf dem Erreichen der erforderlichen Auflösung, einem hohen Grad an Automatisierung und der vielfälting Einsatzfähigkeit des Instruments. Die Leistungsfähigkeit dieses Kraftmikroskops wurde besonders durch zwei Experimente überprüft und sichergestellt. Zum einen wurden DNA Moleküle gedehnt und die Polymerparameter Persistenzlänge und Zugmodul gemessen, welche sehr gut mit veröffentlichten Referenzwerten übereinstimmten. Zum anderen wurde die Allan Schwankung für verschiedene experimentelle Konfigurationen von mikroskopischen Kugeln ermittelt, was eine hohe Stabilität und Auflösung des Gerätes, mit optimaler Leistung bei Mittelung auf Zeitskalen von 1–10 s, bestätigte. Optische Fallen müssen kalibriert werden, um Kräfte exakt messen zu können. Im Allgemeinen kommt dafür ein Verfahren zum Einsatz, welches die brownsche Bewegung eines gefangenen Objektes im harmonischen Potential des Laserfokus ausnutzt. Aus diesen Fluktuationen werden die benötigten Parameter ermittelt, um das gemessene analoge Spannungssignal in Abstände und Kräfte umzuwandeln. Dieser Ansatz erfordert jedoch die Kenntnis des Reibungskoeffizienten des gehaltenen Objektes, meist einer mikroskopischen Kugel. Daher wurde eine Methode vorgeschlagen, die durch ein oszillierendes Flussfeld eine zusätzliche Bewegung der Kugel anregt aus welcher der Reibungskoeffizient bestimmt werden kann. Dieses Vorgehen reduziert die im vornherein benötigten Informationen, wurde jedoch nur für eine einzelne optische Falle entwickelt. Der Ansatz wurde in dieser Arbeit erweitert, indem die zu zugrundeliegenden Bewegungsgleichungen einer gefangenen Kugel um hydrodynamische Wechselwirkungen zwischen mehreren Objekten ergänzt und die Kalibrationparameter basierend darauf hergeleitet wurden. Im Ergebnis konnte gezeigt werden, dass ein einzelner multiplikativer Faktor ausreicht, um die Hydrodynamik zu berücksichtigen und die exakte Kalibration des Instruments sicherzustellen. Dieses Vorgehen wurde überprüft, indem der Reibungskoeffizient einer einzelnen oder mehrerer mikroskopischer Kugeln gleichzeitig durch Anlegen eines externen Flussfeldes gemessen wurde. Die Ergebnisse stimmen im Rahmen der Messgenauigkeit überein und bestätigen damit den gewählten Ansatz. Das neu implementierte Kraftmikroskop wurde im Folgenden eingesetzt, um das Coiled-Coil Protein Early Endosome Antigen 1 (EEA1) zu erforschen. Dieser 200 nm lange Homodimer kollabiert aufgrund entropischer Kräfte sobald eine kleine GTPase an seinen N-Terminus bindet. Um diesen Effekt und die wirkenden Bindungskräfte besser zu verstehen, wurde hier ein Experiment entwickelt bei dem die beiden α-Helicen auseinandergezogen werden. Dazu wurde mittels einer Sortase A basierten Ligationsreaktion an jede Helix ein DNA-Stück gebunden, über welches Kräfte auf das Molekül übertragen werden können. Erste Experimente wurden mit der optischen Doppelfalle und dieser Protein-DNA Chimäre durchgeführt. Somit sind alle benötigten Werkzeuge zum weiteren Studium des entropischen Kollapses von EEA1 verfügbar, indem die Bindungskräfte der α-Helicen untersucht werden. Zusammenfassend wurde eine hoch auflösende Doppelfalle konstruiert, die Kalibrationsmethode weiterentwickelt und verfeinert und das Kraftmikroskop zur Erforschung der Bindungskräfte der α-Helicen von EEA1 eingesetzt.
23

Analyse fonctionnelle de la polycystine-1 et de son domaine intracellulaire dans le développement de la polykystose rénale autosomique dominante

Côté, Olivier 04 1900 (has links)
La polykystose rénale autosomique dominante (PKRAD) est la maladie génétique rénale la plus commune touchant 1/500 personnes. Elle se caractérise principalement par la formation de kystes rénaux dans tous les segments du néphron, entraînant l’insuffisance rénale, et par des manifestations extrarénales kystiques (foie, pancréas, rate) et non-kystiques (anomalies cardiaques, vasculaires et cérébrales). Deux gènes, PKD1 et PKD2, sont responsables de 85 et 15% des cas respectivement. Ces gènes encodent les polycystine-1 (PC-1) et -2 (PC-2) qui forment un complexe à la membrane plasmique et ciliaire des cellules épithéliales rénales. PC-1 est une protéine transmembranaire de 4302 acides aminés possédant un court domaine intracellulaire incluant un motif coiled-coil impliqué dans l’interaction entre PC-1 et PC-2 in-vitro. L’importance du coiled-coil est démontrée par des mutations affectant spécifiquement ce motif chez des patients PKRAD. Le mécanisme pathogénétique responsable de la PKRAD est indéterminé. Chez la souris, la PKRAD se développe suite à l’ablation (Pkd1-/-) ou lors de la surexpression (SBPkd1TAG) de Pkd1, ce qui suggère un effet de dosage. Des anomalies ciliaires sont aussi souvent associées à PKRAD. Mon objectif était de déterminer in-vivo le mécanisme pathogénétique de la polycystine-1 dans le développement des symptômes PKRAD rénaux et extrarénaux et plus spécifiquement, le rôle du motif coiled-coil dans le mécanisme de kystogenèse. Pour ce faire, nous avons généré deux constructions, Pkd1 sauvage (Pkd1TAG) et Pkd1 tronquée de son motif coiled-coil (Pkd1ΔCoiled-coil), par recombinaison homologue à partir du BAC-Pkd1 sauvage comprenant la séquence murine entière de Pkd1. Trois lignées de souris Pkd1TAG générées par microinjection démontrent un niveau d’expression de Pkd1 qui corrèle avec le nombre de copie du transgène (2, 5 et 15 copies). Les souris Pkd1TAG reproduisent la PKRAD en développant des kystes rénaux dans toutes les parties du néphron et des cils primaires plus longs que les contrôles non transgéniques. Les analyses physiologiques supportent que les souris Pkd1TAG développent une insuffisance rénale et démontrent une augmentation du volume urinaire de même qu’une diminution de l’osmolalité, de la créatinine et des protéines urinaires. De plus, les souris Pkd1TAG développent des kystes hépatiques, des anomalies cardiaques associées à des dépôts de calcium et des anévrismes cérébraux. La sévérité du phénotype augmente avec l’expression de Pkd1 appuyant l’hypothèse d’un mécanisme de dosage. Nous avons aussi déterminé que l’expression du transgène Pkd1TAG complémente le phénotype létal-embryonnaire des souris Pkd1-/-. D’autre part, nous avons générés 4 lignées de souris Pkd1ΔCoiled-coil (2 et 15 copies du transgène) dont le nombre de copies corrèle avec le niveau d’expression du transgène. Ces souris Pkd1ΔCoiled-coil, contrairement aux Pkd1TAG de même âge, ne développent pas de kystes et possèdent des cils primaires de longueur normale. Afin d’évaluer le rôle du motif coiled-coil en absence de polycystine-1 endogène, nous avons croisé les souris Pkd1ΔCoiled-coil avec les souris Pkd1-/-. Contrairement aux souris Pkd1-/- qui meurent in-utéro, les souris Pkd1ΔCoiled-coil; Pkd1-/- survivent ~10 à 14 jours après la naissance. Elles démontrent des kystes rénaux et pancréatiques sévères, un retard de croissance et des anomalies pulmonaires. Tous les segments du néphron sont affectés. Mon projet démontre que la surexpression de Pkd1 est un mécanisme pathogénique de la PKRAD tant au niveau rénal qu’extrarénal. De plus, il démontre que le motif coiled-coil est un élément déterminant dans la kystogenèse/PKRAD in-vivo. / Autosomal dominant polycystic kidney disease (ADPKD) is a common genetic disorder affecting 1:500 people worldwide, independently from sex and origin. ADPKD is characterized by formation of large bilateral kidney cysts affecting all segments of the nephron and increasing progressively in size and number leading to end stage renal failure by mid-fifty. Moreover, this systemic disease includes several extrarenal symptoms such as intracranial aneurysms, valvular defects and cysts formation in the liver and the pancreas. PKD1 and PKD2 genes mutations are involved in 85 and 15 % of the clinical cases. PKD genes encode polycystin-1 (PC-1) and -2 (PC-2), which both form a complex at the cell and ciliary membrane of renal epithelial cells. PC-1 is a large transmembrane protein with a small intracellular tail including a coiled-coil motif implicated in PC-1/PC-2 interaction in-vitro. Interestingly, specific mutations affecting the coiled-coil motif cause ADPKD in humans. The pathogenetic mechanism of ADPKD is unknown. In mice, both ablation (Pkd1-/-) or overexpression (SBPkd1TAG) of Pkd1 cause ADPKD, suggesting a dosage model. Ciliary anomalies are also linked to polycystic kidney disease. Herein, we evaluated in-vivo the role of Pkd1 in the development of renal and extrarenal manifestations of ADPKD and more specifically, the role of the coiled-coil motif in cystogenesis. We generated two constructions, wildtype Pkd1 (Pkd1TAG) and coiled-coil deleted Pkd1 (Pkd1ΔCoiled-coil), by homologous recombination from the wildtype Pkd1-BAC comprising the whole Pkd1 murine sequence. Three Pkd1TAG mice lines have been generated by microinjection and show expression patterns correlating with the copy number of the transgene (2, 5 and 15 copy). All Pkd1TAG mice develop renal cysts affecting all nephron segments as in ADPKD and longer primary cilia compared to wildtype mice. Physiologic analysis supports renal failure by increased urinary output and decreased of urinary proteins, osmolality and creatinin levels. Pkd1TAG mice also show cysts in the liver, cardiac and valvular anomalies associated with calcium deposition and cerebral aneurysms. The severity of the phenotype increased with Pkd1 expression suggesting a dosage model. Importantly, the Pkd1TAG transgene rescue embryonic lethality of Pkd1-/- mice. Furthermore, we generated 4 lines of Pkd1ΔCoiled-coil mice of 2 and 15 copies of the transgene correlating also to the level of expression. Compared to age-matched Pkd1TAG, Pkd1ΔCoiled-coil mice develop no cysts and show normal cilia length. To gain more insights on the role of coiled-coil motif in absence of endogenous Pc-1, we mated Pkd1ΔCoiled-coil with Pkd1-/- mice. Compared to the lethal embryonic Pkd1-/- mice, Pkd1ΔCoiled-coil; Pkd1-/- live ~ 10 to 14 days. They show severe renal and pancreatic cysts as well as growth retardation and pulmonary defects. My study demonstrates that Pkd1 overexpression is a pathogenic mechanism to induce ADPKD renal and extrarenal phenotype. Moreover, this work shows that the coiled-coil motif of polycystin-1 is a critical determinant in ADPKD cystogenesis.
24

YopD translocator function in Yersinia pseudotuberculosis type III secretion

Costa, Tiago R. D. January 2012 (has links)
Type III secretion systems (T3SS) are a common feature of Gram-negative bacteria, allowing them to inject anti-host effectors into the interior of infected eukaryotic cells. By this mechanism, these virulence factors help the bacteria to modulate eukaryotic cell function in its favor and subvert host innate immunity. This promotes a less hostile environment in which infecting bacteria can colonize and cause disease. In pathogenic Yersinia, a crucial protein in this process is YopD. YopD is a T3S substrate that, together with YopB, forms a translocon pore in the host cell membrane through which the Yop effectors may gain access to the target-cell cytosol. The assembly of the translocator pore in plasma membranes is considered a fundamental feature of all T3SSs. How the pore is formed, what determines the correct size and ultimately the stoichiometry between YopD YopB, is still unknown. Portions of YopD are also observed inside HeLa cells. Moreover, YopD functions together with its T3S chaperone, LcrH, to control Yops synthesis in the bacterial cytoplasm. The multifunctional YopD may influence all these processes by compartmentalizing activities into discrete modular domains along the protein length. Therefore, understanding how particular domains and/or residues within these regions coordinate multiple functions of the protein will provide a platform to improve our knowledge of the molecular mechanisms behind translocation through T3SSs. Comprehensive site-directed mutagenesis of the YopD C-terminal amphipathic α-helix domain, pinpointed hydrophobic residues as important for YopD function. Some YopD variants were defective in self-assembly and in the ability to interact with the needle tip protein, LcrV, which were required to facilitate bacterial T3S activity. A similar mutagenesis approach was used to understand the role of the two predicted coiled-coils located at the N-terminal and C-terminal region of YopD. The predicted N-terminal element that occurs solely in the Yersinia YopD translocator family is essential for optimal T3SS and full disease progression. The predicted YopD C-terminal coiled-coil shapes a functional translocon inserted into host cell membranes. This translocon was seen to be a dynamic structure facilitating at least two roles during effectors delivery into cells; one to guarantee translocon pore insertion into target cell membranes and the other to promote targeted activity of internalized effector toxins. In Yersinia expression of yop genes and secretion of the corresponding polypeptides is tightly regulated at a transcriptional and post-transcriptional level. If T3S chaperones of the translocator class are known to influence transcriptional output of T3SS genes in other bacteria, we show that in Yersinia the class II T3S chaperone LcrH has no such effect on the LcrF transcriptional activator activity. We also demonstrate that there are possibly additional yop-regulatory roles for the LcrH chaperone besides forming a stable complex with YopD to impose post-transcriptional silencing on Yops synthesis. This mechanism that relies upon an active T3SS, might act independently of both YopD and the regulatory element LcrQ. In conclusion, this work has sought to delineate the encrypted functions of the YopD translocator that contribute to Yersinia T3SS-dependent pathogenesis. Contributions of the YopD cognate chaperone LcrH in yop regulatory control are also presented.
25

Multivalent Interactions Based on Supramolecular Self-Assembly and Peptide-Labeled Quantum Dots for Imaging GPCRs

Zhou, Min January 2006 (has links)
Multivalent interactions are common in nature, such as influenza virus infecting epithelial cells, clearance of pathogens by antibody-mediated attachment to macrophages, etc. To mimic nature, we utilized a bottom-up approach to develop various multivalent self-assembling systems based on leucine-zipper peptides. We tethered several pairs of leucine-zipper peptides to PAMAM dendrimers to form leucine-zipper dendrimers (LZDs). We conjugated Fos/Jun to the dendrimer to make D0Fos4 and D0Jun4, and studied the interactions between these LZDs and their cognate peptide target, either Jun or Fos. Our experiments showed that the D0Fos4 can non-covalently assemble four copies of Jun, and this approach can be further used for the rapid non-covalently assembling of multimeric ligands. We also pursued the multivalent target of GPCRs with a Fos/Jun assembly, and found the complex can potentially be used as a molecular switch to target GPCRs with controlled ligand activity. In a related project for bio-material design based on self-assembly of LZDs, we synthesized a different pair of LZDs, D-Ez4 and D-Kz4, and established that they can assemble at neutral pH to form helical fibrils which display higher order self-organized structures, providing a new methodology for bio-material design. In another effort for studying multivalent interactions, we conjugated three copies of the F23, mini-protein that binds the HIV-1 capsid protein, to a trimesic acid and obtained a trivalent inhibitor, Tri-F23. Tri-F23 showed enhanced binding in ELISA against gp120, but was not significantly more effective preventing HIV entry. This methodology provides a new strategy for developing multivalent inhibitors for preventing HIV-1 infection at the entry level. In a related area, we are developing imaging agents based on quantum dots that can detect GPCRs on whole cells and at the single molecule level. To this end, a new method was developed for biocompatible amphphilic polymers to coat quantum dots. This amphiphilic polymer facilitates rapid quantum dot conjugation to any ligand with a free thiol or engineered cysteine. Several GPCR targeted peptides have been utilized for imaging receptors on whole cells and as single molecules. These efforts will guide the rational design of multivalent ligands for targeting GPCRs and other cell surface proteins.
26

Analyse fonctionnelle de la polycystine-1 et de son domaine intracellulaire dans le développement de la polykystose rénale autosomique dominante

Cote, Olivier 04 1900 (has links)
La polykystose rénale autosomique dominante (PKRAD) est la maladie génétique rénale la plus commune touchant 1/500 personnes. Elle se caractérise principalement par la formation de kystes rénaux dans tous les segments du néphron, entraînant l’insuffisance rénale, et par des manifestations extrarénales kystiques (foie, pancréas, rate) et non-kystiques (anomalies cardiaques, vasculaires et cérébrales). Deux gènes, PKD1 et PKD2, sont responsables de 85 et 15% des cas respectivement. Ces gènes encodent les polycystine-1 (PC-1) et -2 (PC-2) qui forment un complexe à la membrane plasmique et ciliaire des cellules épithéliales rénales. PC-1 est une protéine transmembranaire de 4302 acides aminés possédant un court domaine intracellulaire incluant un motif coiled-coil impliqué dans l’interaction entre PC-1 et PC-2 in-vitro. L’importance du coiled-coil est démontrée par des mutations affectant spécifiquement ce motif chez des patients PKRAD. Le mécanisme pathogénétique responsable de la PKRAD est indéterminé. Chez la souris, la PKRAD se développe suite à l’ablation (Pkd1-/-) ou lors de la surexpression (SBPkd1TAG) de Pkd1, ce qui suggère un effet de dosage. Des anomalies ciliaires sont aussi souvent associées à PKRAD. Mon objectif était de déterminer in-vivo le mécanisme pathogénétique de la polycystine-1 dans le développement des symptômes PKRAD rénaux et extrarénaux et plus spécifiquement, le rôle du motif coiled-coil dans le mécanisme de kystogenèse. Pour ce faire, nous avons généré deux constructions, Pkd1 sauvage (Pkd1TAG) et Pkd1 tronquée de son motif coiled-coil (Pkd1ΔCoiled-coil), par recombinaison homologue à partir du BAC-Pkd1 sauvage comprenant la séquence murine entière de Pkd1. Trois lignées de souris Pkd1TAG générées par microinjection démontrent un niveau d’expression de Pkd1 qui corrèle avec le nombre de copie du transgène (2, 5 et 15 copies). Les souris Pkd1TAG reproduisent la PKRAD en développant des kystes rénaux dans toutes les parties du néphron et des cils primaires plus longs que les contrôles non transgéniques. Les analyses physiologiques supportent que les souris Pkd1TAG développent une insuffisance rénale et démontrent une augmentation du volume urinaire de même qu’une diminution de l’osmolalité, de la créatinine et des protéines urinaires. De plus, les souris Pkd1TAG développent des kystes hépatiques, des anomalies cardiaques associées à des dépôts de calcium et des anévrismes cérébraux. La sévérité du phénotype augmente avec l’expression de Pkd1 appuyant l’hypothèse d’un mécanisme de dosage. Nous avons aussi déterminé que l’expression du transgène Pkd1TAG complémente le phénotype létal-embryonnaire des souris Pkd1-/-. D’autre part, nous avons générés 4 lignées de souris Pkd1ΔCoiled-coil (2 et 15 copies du transgène) dont le nombre de copies corrèle avec le niveau d’expression du transgène. Ces souris Pkd1ΔCoiled-coil, contrairement aux Pkd1TAG de même âge, ne développent pas de kystes et possèdent des cils primaires de longueur normale. Afin d’évaluer le rôle du motif coiled-coil en absence de polycystine-1 endogène, nous avons croisé les souris Pkd1ΔCoiled-coil avec les souris Pkd1-/-. Contrairement aux souris Pkd1-/- qui meurent in-utéro, les souris Pkd1ΔCoiled-coil; Pkd1-/- survivent ~10 à 14 jours après la naissance. Elles démontrent des kystes rénaux et pancréatiques sévères, un retard de croissance et des anomalies pulmonaires. Tous les segments du néphron sont affectés. Mon projet démontre que la surexpression de Pkd1 est un mécanisme pathogénique de la PKRAD tant au niveau rénal qu’extrarénal. De plus, il démontre que le motif coiled-coil est un élément déterminant dans la kystogenèse/PKRAD in-vivo. / Autosomal dominant polycystic kidney disease (ADPKD) is a common genetic disorder affecting 1:500 people worldwide, independently from sex and origin. ADPKD is characterized by formation of large bilateral kidney cysts affecting all segments of the nephron and increasing progressively in size and number leading to end stage renal failure by mid-fifty. Moreover, this systemic disease includes several extrarenal symptoms such as intracranial aneurysms, valvular defects and cysts formation in the liver and the pancreas. PKD1 and PKD2 genes mutations are involved in 85 and 15 % of the clinical cases. PKD genes encode polycystin-1 (PC-1) and -2 (PC-2), which both form a complex at the cell and ciliary membrane of renal epithelial cells. PC-1 is a large transmembrane protein with a small intracellular tail including a coiled-coil motif implicated in PC-1/PC-2 interaction in-vitro. Interestingly, specific mutations affecting the coiled-coil motif cause ADPKD in humans. The pathogenetic mechanism of ADPKD is unknown. In mice, both ablation (Pkd1-/-) or overexpression (SBPkd1TAG) of Pkd1 cause ADPKD, suggesting a dosage model. Ciliary anomalies are also linked to polycystic kidney disease. Herein, we evaluated in-vivo the role of Pkd1 in the development of renal and extrarenal manifestations of ADPKD and more specifically, the role of the coiled-coil motif in cystogenesis. We generated two constructions, wildtype Pkd1 (Pkd1TAG) and coiled-coil deleted Pkd1 (Pkd1ΔCoiled-coil), by homologous recombination from the wildtype Pkd1-BAC comprising the whole Pkd1 murine sequence. Three Pkd1TAG mice lines have been generated by microinjection and show expression patterns correlating with the copy number of the transgene (2, 5 and 15 copy). All Pkd1TAG mice develop renal cysts affecting all nephron segments as in ADPKD and longer primary cilia compared to wildtype mice. Physiologic analysis supports renal failure by increased urinary output and decreased of urinary proteins, osmolality and creatinin levels. Pkd1TAG mice also show cysts in the liver, cardiac and valvular anomalies associated with calcium deposition and cerebral aneurysms. The severity of the phenotype increased with Pkd1 expression suggesting a dosage model. Importantly, the Pkd1TAG transgene rescue embryonic lethality of Pkd1-/- mice. Furthermore, we generated 4 lines of Pkd1ΔCoiled-coil mice of 2 and 15 copies of the transgene correlating also to the level of expression. Compared to age-matched Pkd1TAG, Pkd1ΔCoiled-coil mice develop no cysts and show normal cilia length. To gain more insights on the role of coiled-coil motif in absence of endogenous Pc-1, we mated Pkd1ΔCoiled-coil with Pkd1-/- mice. Compared to the lethal embryonic Pkd1-/- mice, Pkd1ΔCoiled-coil; Pkd1-/- live ~ 10 to 14 days. They show severe renal and pancreatic cysts as well as growth retardation and pulmonary defects. My study demonstrates that Pkd1 overexpression is a pathogenic mechanism to induce ADPKD renal and extrarenal phenotype. Moreover, this work shows that the coiled-coil motif of polycystin-1 is a critical determinant in ADPKD cystogenesis.
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Coiled coil Cytoskeleton in Bacterial Cell Architecture : Studies of Growth and Development in Streptomyces

Bagchi, Sonchita January 2011 (has links)
Bacterial cytoskeleton is an exciting and relatively new field of research. Recent findings have proven that microbes are well-organized and neatly structured organisms. In this study we have shown that intermediate filament-like proteins with a characteristic rod domain architecture of coiled coil segments separated by non-coiled coil linkers, are widely spread among bacteria. We identified and characterized an intermediate filament-like protein (named FilP after filamentous protein) in Streptomyces coelicolor. It shares the characteristic biochemical property of eukaryotic intermediate filaments of formation of spontaneous filaments in vitro without requiring any energy or co-factor. We have provided here a preliminary model of its assembly in vitro. FilP also forms in vivo filaments in S. coelicolor hyphae, which are strongest at the sub-apical location of growing vegetative hyphae. We have proposed that FilP cytoskeletal network provides rigidity to the hyphae, especially at the growing tips, by interacting with an essential coiled coil protein DivIVA and possibly other partner elements, yet to be found. S. coelicolor is a well-studied model organism with a complicated life cycle. It germinates from a spore and spreads by forming branched vegetative hyphae. Lack of nutrients in the environment initiates formation of aerial hyphae in the air, perpendicular to the vegetative ones. The aerial hyphae differentiate into spore chains and eventually grey-pigmented dispersed individual spores are released. The signals involved in sporulation including cell division and chromosome segregation are not clear yet. We characterized here a novel locus consisting of two genes: a small putative membrane protein with no defined function, named SmeA and a member of the SpoIIIE/FtsK family, called SffA. The expression of this locus appears to be dependent on whiA and whiG-whiH-whiI pathways. This finding is intriguing as it can provide insight to the relationship between two apparently unrelated pathways, both leading to the same function of septation and maturation during sporulation.
28

Towards a mucosal vaccine against group A streptococcus based on a live bacterial delivery system

Melina Mary Georgousakis Unknown Date (has links)
No description available.
29

Synthetic Peptides Model Instability of Cardiac Myosin Subfragment-2

Taei, Nasrin 08 1900 (has links)
Hypertrophic cardiomyopathy (HCM), a heart-related abnormality, is the most prevalent cause of sudden death in young athletes at sporting events. A cluster of cardiomyopathy mutations are localized in β-cardiac myosin at the N-terminal region of subfragment-2. Using resonance energy transfer probes, a synthetic peptide model system was developed to study stability of the coiled coil (S2 fragment) structure by determining monomer-dimer equilibrium of the peptide. Fluorescence resonance energy transfer and MacroModel software suite were used to obtain distance measurements along with measurement of coiled coil formation. The model peptide was used to characterize the effects of disease-causing-mutations and examine potential candidate drugs (polyamines) to counteract effects of mutations causing HCM. Distance measurements between donor and acceptor probes obtained by computational simulation and fluorescence resonance energy transfer (FRET) were consistent. Measurements also agreed with simulations of unlabeled wildtype, indicating coiled coil structural stability of the peptide. Interaction of the site-specific antibody with the peptide strongly inhibited dimerization and destabilized coiled coil structure of the peptide. Presence of negatively charged glutamate residues in the region of subfragment-2 strongly suggested a potential interaction site for positively charged polyamines. Binding of certain polyamines, such as poly-L-Lysine 11 residues and poly-D-Lysine 17 residues, demonstrated the ability to enhance dimerization and improve stability of the coiled coil structure, while some other polyamines were shown to have insignificant impact on the structure. In an attempt to characterize the effect of HCM-causing-mutations, peptides containing E924K mutation and lethal mutation E930 deletion were synthesized. Fluorescence resonance probes were conjugated to the mutant peptides to determine coiled coil formation. Results obtained from both dynamic simulations and resonance energy transfer experiments indicated that these mutations strongly inhibit dimerization, and thus, destabilize coiled coil structure of the peptide. Further experiments were conducted using heterodimers containing a chain of wildtype and a chain of mutant peptide. Both E924K & Edel930 mutations destabilized coiled coil formation and prevented dimerization. This peptide model system would provide a promising tool for drug development targeting HCM-causing-mutations along the S2 region of myosin.
30

Measuring the Interaction and Cooperativity Between Ionic, Aromatic, and Nonpolar Amino Acids in Protein Structure

Smith, Mason Scott 01 July 2018 (has links)
Protein folding studies have provided important insights about the key role of non-covalent interactions in protein structure and conformational stability. Some of these interactions include salt bridges, cation-π, and anion-Ï€ interactions. Understanding these interactions is crucial to developing methods for predicting protein secondary, tertiary, quaternary structure from primary sequence and understanding protein-protein interactions and protein-ligand interactions. Several studies have described how the interaction between two amino acid side chains have a substantial effect on protein structure and conformational stability. This is under the assumption that the interaction between the two amino acids is independent of surrounding interactions. We are interested in understanding how salt bridges, cation-π, and anion-π interactions affect each other when they are in close proximity. Chapter 1 is a brief introduction on noncovalent interactions and noncovalent interaction cooperativity. Chapter 2 describes the progress we have made measuring the cooperativity between noncovalent interactions involving cations, anions and aromatic amino acids in a coiled-coil alpha helix model protein. Chapter 3 describes cooperativity between cation, anion, and nonaromatic hydrophobic amino acids in the context of a coiled-coil alpha helix. In chapter 4 we describe a strong anion-π interaction in a reverse turn that stabilizes a beta sheet model protein. In chapter 5 we measure the interaction between a cysteine linked maleimide and two lysines in a helix and show that it is a general strategy to stabilize helical structure.

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