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Interfacial Characterization of Polyhedral Oligomeric Silsesquioxane (POSS) Amphiphiles and Polymer Blends: Thermodynamics, Morphology, and RheologyDeng, Jianjun 25 April 2005 (has links)
Over the past two decades one class of oligomers, polyhedral oligomeric silsesquioxanes (POSS), has attracted considerable attention because of their unique hybrid organic/inorganic molecular structures and nanoscopic sizes. While surface and interfacial properties may play a key role in many potential POSS applications, relatively little is actually known about the surface properties of POSS. This dissertation provides studies of the interfacial aspects of both POSS molecules and POSS/polymer blends at the air/water interface (A/W) through surface pressure-area per molecule (π-<i>A</i>) isotherm, Brewster angle microscopy (BAM), and interfacial stress rheometry (ISR) studies.
Results for POSS Langmuir thin films at A/W show that trisilanol-POSS derivatives are a new class of amphiphiles, that exhibit multiple phase transitions in going from traditional 2D Langmuir monolayers (1 POSS molecule thick) to various 3D multilayer films upon compression. With small length/diameter ratios and bulky shapes, the monolayer phase behavior and packing states of different POSS are simpler than the traditional rod-like lipids. Meanwhile trisilanol-POSS derivatives have very different collapse behavior and multilayer organization showing strong substituent effects even though they have similar molecular sizes. While trisilanolisobutyl-POSS (TiBuP) monolayers undergo collapse around π ≈ 18 mNm⁻¹ and form various ordered or disordered solid-like 3D aggregates at different compression rates, trisilanolcyclohexyl-POSS (TCyP) monolayers collapse into trilayers via instantaneous nucleation with hemispherical edge growth around π ≈ 3.7 mNm⁻¹. ISR results reveal three different non-Newtonian flow regimes that correlate with phase transitions in the Pi-A isotherms. Further symmetric compression after trilayer formation induces TCyP thin films to self-assemble into highly ordered crystalline-like hydrophobic multilayers (≈8 POSS molecule thick) with unique rod-like morphologies, which are dramatically different from –collapsed– morphologies seen in other systems.
By treating POSS derivatives as ideal nanofiller for studying confinement effects on filled polymer systems, amphiphilic poly(dimethylsiloxane) (PDMS) derivatives with different polar functional groups are studied as blends with TiBuP and octaisobutyl-POSS at A/W to resolve one of the key challenges for current nanocomposite applications: How to control nanofiller dispersion in polymer matrices? The results in this dissertation reveal that introducing polar groups into polymeric matrix polymers is a good way to control dispersion. / Ph. D.
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Synthesis of Novel Polyhydroxyl Surfactants. Influence of the Relative Stereochemistry on Surfactant Properties.Neimert-Andersson, Kristina January 2003 (has links)
<p>This thesis deals with the synthesis and characterization ofnovel polyhydroxyl surfactants. The first part describes thesynthesis of a number of stereoisomers of a polyhydroxylsurfactant, and the second part concerns surface chemicalcharacterization.</p><p>A stereodivergent route for preparation of the hydrophilichead group was developed, featuring consecutive stereoselectivedihydroxylations of a diene. This afforded in total fourdifferent polyhydroxyl head groups. These surfactant headgroups were natural and unnatural sugar analogues, and wereused for the coupling with two different hydrophobic tailgroups.</p><p>Three of these surfactants were used to investigate thechiral discrimination in Langmuir monolayers at an air-waterinterface. The isotherms showed a remarkable difference incompressibility between surfactants of diastereomericrelationship and also a pronounced chiral discriminationbetween racemic and enantiomerically pure surfactants favoringheterochiral discrimination.</p>
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Proteínas inativadoras de ribossomos: identificação de novas proteínas e estudos de interação da cadeia-A da pulchellina (PAC) com monocamada de Langmuir / Ribosome inactivating proteins: identification of new members and studies of the interaction of pulchellin A-chain (PAC) with Langmuir monolayersReyes, Luis Fernando 29 March 2011 (has links)
Proteínas Inativadoras de Ribossomos (RIPs) são rRNA N-glicosilases capazes de inibir a síntese protéica pela remoção de uma adenina específica do RNA ribossomal. São geralmente classificadas em tipo 1 e tipo 2, sendo as últimas divididas em altamente tóxicas e não tóxicas. A maior parte das RIPs tipo 2 identificadas pertence a espécies de dicotiledôneas, como é o caso da pulchellina. As cadeias tóxicas das RIPs possuem uma região C-terminal hidrofóbica conservada, a qual se atribui a capacidade de interação com a membrana do retículo endoplasmático (RE), durante o transporte retrógrado da toxina para o citosol. Neste trabalho duas abordagens diferentes foram aplicadas para o estudo das RIPs tipo 2: identificação e caracterização de novos integrantes desta família de proteínas, e investigação da interação da cadeia-A da pulchellina (PAC) com sistemas miméticos da membrana celular. Na primeira abordagem, uma busca in silico em bancos de dados genéticos públicos permitiu identificar quatro novas RIPs do tipo 2 de monocotiledôneas. A análise da estrutura primária das proteínas identificadas mostrou a ocorrência de mutações em alguns dos principais aminoácidos que formam o sítio ativo nas RIPs, indicando uma possível perda de função. O representante de Saccharum officinarum (cana-de-açúcar) foi então analisado em maior detalhe, sendo sua cadeia-A clonada (soRIPA), expressa em sistema heterólogo e caracterizada em termos de atividade e estrutura secundária. Os ensaios in vitro mostraram que a soRIPA não foi capaz de depurinar ribossomos eucariotos. Porém, os ensaios de inibição da síntese proteica mostraram uma possível atividade inibitória da soRIP, que precisa ainda ser confirmada. A presença dos transcritos no banco do SUCEST sugere que estes genes não sejam pseudogenes, embora não tenha sido possível purificar a proteína a partir de extratos de folhas. Isto indica que se a soRIP está sendo traduzida, deve sofrer um rápido turnover, tornando difícil a sua detecção e purificação ou, ainda, que a ausência de sítios de ligação à galactose funcionais na cadeia-B impediu sua purificação por cromatografia de afinidade à galactose. A outra abordagem no estudo das RIPs tipo 2 foi centrada na cadeia-A recombinante da pulchellina (rPAC), estudando sua interação com monocamadas de Langmuir. Foram construídos 3 mutantes da rPAC, cada um com diferentes deleções na região C-terminal visando determinar a região responsável pela interação com a membrana do RE. A cinética de adsorção e pressão superficial exercida pela rPAC sobre a monocamada, assim como o estudo com os mutantes demontraram que a proteína interage fortemente com a monocamada fosfolipídica e que esta interação in vitro é dependente da presença da região C-terminal. De forma geral, os resultados obtidos neste trabalho contribuíram com novas informações sobre esta família de proteínas, identificando e analisando novos integrantes e, ainda, adicionando detalhes do mecanismo funcional do tráfego das toxinas RIPs. / Ribosome Inactivating Proteins (RIPs) are rRNA N-glycosilases which are able to inhibit the protein synthesis by removing a specific adenine from the ribosomal RNA. They are usually classified as type 1 and type 2, being the latter divided into highly toxic and nontoxic. The majority of type 2 RIPs currently identified are found in species of dicotyledons, as the pulchellin. The toxic chain of RIPs has a conserved hydrophobic C-terminal region, which is believed to be responsible for the interaction with the lipid membrane of the endoplasmic reticulum ER during the retrograde transport of the toxin to the cytosol. In this work, two different approaches were applied in the study of type 2 RIPs: identification and characterization of new members of this protein family, and investigation of the interaction of the pulchellin\'s A-chain (PAC) with systems that mimic the cellular membrane. In the first approach, an in silico search in public genetic databases was performed and allowed us to identify four new type 2 RIPs in monocots. The primary structure analysis of the identified proteins showed the presence of mutations in key amino acids that form the active site of RIPs, indicating a possible interference on its catalytic activity. The representative of Saccharum officinarum (sugar cane) was then analyzed in greater detail. Its A-chain clone (soRIPA) was expressed in a heterologous system and characterized in terms of activity and secondary structure. In vitro experiments showed that soRIPA was not able to perform the depurination of eukaryotic ribosomes. However, the inhibition of protein synthesis assays presented a possible low inhibitory activity of the soRIP, which still needs to be further investigated. The presence of transcripts on the bank of SUCEST indicates that these genes are not pseudogenes, although it was not possible to purify the protein from leaf extracts. If the soRIP is being translated, this may indicate that it undergoes a quick turnover, preventing its detection and purification. It is also possible that the absence of functional galactose binding sites in the B-chain has prevented its purification by galactose affinity chromatography. Our second approach to the study of type 2 RIPs was focused on the recombinant pulchellin A-chain (rPAC), by investigating its interaction with Langmuir monolayers. We have constructed three mutants of rPAC, each one with different deletions at the C-terminal to determine the region responsible for interaction with the membrane of the ER. The adsorption kinetic and surface pressure applied by rPAC on the monolayer, as well as the study of the mutants, have demonstrated that the protein has a strong interaction with the phospholipid monolayer and that this interaction in vitro is dependent on the presence of the C-terminal. The results of this work have provided new information about the type 2 RIP protein family, identifying and analyzing new members, and also bringing new details about the functional mechanism of the RIP\'s toxin traffic.
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Filmes de Langmuir e Langmuir-Blodgett de Polianilinas / Langmuir and Langmuir-Blodgett films of polyaniline.Riul Júnior, Antonio 19 May 1998 (has links)
Explorou-se a caracterização de monocamadas e filmes LB de polianilina (PANi), e um oligômero de polianilina, chamado aqui de 16-mero, com estearato de cádmio (CdSt). A análise dos filmes de Langmuir indicou que possivelmente não há mistura em nível molecular da PANi e do 16-mero com CdSt, ainda que a quantidade adicionada em solução de polímero ou oligômero influencie a estabilidade das monocamadas. Utilizou-se UV-vis, FTIR, difração de raios-X, condutividade elétrica, elipsometria, microscopia óptica e potencial de superficie para caracterização dos filmes LB. Os resultados de UV-vis indicaram uma transferência uniforme e ainda que os filmes recém depositados encontram-se desdopados. A análise de FTIR confirma a presença de CdSt nos filmes LB, e o efeito de desdopagem em subfases neutras, corroborando os resultados de UV-vis. A difração de raios-X indica a presença de domínios separados de PANi (e 16-mero) com CdSt nos filmes LB. Resultados elipsométricos indicaram uma espessura por camada em tomo de 25 Å. A excelente uniformidade obtida nos filmes LB mistos foi comprovada pelos resultados de microscopia óptica e potencial de superficie. Esses filmes mistos apresentaram valores de condutividade elétrica em tomo de 10-4 a 10-5 S.cm-1 (van der Pauw), tanto para a PANi quanto para o 16-mero. Investigou-se também o efeito da exposição dos filmes mistos PANi/CdSt aos raios-X. Nota-se um deslocamento para a região do vermelho, na região do visível, nos espectros de UVvis, similar à observada pela dopagem através de ácidos inorgânicos. Verificou-se que os efeitos de umidade da atmosfera de medida são predominantes nesse processo de dopagem. É feita uma análise dos resultados de condutividade elétrica, comparando-os com os encontrados na literatura. / A study has been made of composite Langmuir and Langmuir-Blodgett (LB) films of polyaniline (PANi), and a polyaniline oligomer (l6-mer polyaniline), with cadmium stearate (CdSt). The monolayers studies pointed to a phase separated system containing the polymer (or the 16-mer) and CdSt, with no mixing at the molecular leveI, although the relative contents of PANi and 16-mer in the solution have a strong influence on the monolayer stability. UV-vis, FTIR, X-ray difIraction (XRD), electrical conductivity, ellipsometry, optical microscopy and surface potential measurements were used in the LB film characterization. UV-vis results have shown a uniform transfer, with the as deposited films in the undoped state. FTIR results confirmed the presence of CdSt and undoped polyaniline (and 16-mer) in the transferred LB films, corroborating the UV-vis results. XRD has shown separated domains of CdSt and PANi (l6-mer also) in the LB films. Ellipsometry data indicated a thickness of 25 Å per deposited layer. The high uniformity in these mixed LB films was confirmed by optical microscopy and surface potential measurements. The electrical conductivity was approximately 10-4 to 10-5 S.cm-1 for both PANi and 16-mer. Mixed PANi/CdSt films were also exposed to X-ray irradiation. After a given dose rate there is a red shift in the UV-vis spectra from the 600 nm region to the 800 nm region, similar to the usual acid doping process observed in polyaniline. Humidity effects have a strong influence on the doping process. A comparison is made of the conductivity measurements made here with those reported in the literature.
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Estudo da interação da peroxidase de raiz forte em interfaces nanoestruturadas / Study of horseradish peroxidase interaction in nanostructured interfacesSchmidt, Thaís Fernandes 01 August 2008 (has links)
Neste projeto estudou-se a interação da enzima peroxidase de raiz forte (HRP) em interfaces nanoestruturadas e sua possível aplicação em biossensores de peróxido de hidrogênio. Foram utilizadas as técnicas de Langmuir, Langmuir-Blodgett (LB) e automontagem por adsorção física para formar filmes nanoestruturados. A interação da enzima com espécies em interfaces foi investigada com materiais que serviram de matrizes de adsorção, ou seja, a quitosana (Ch) e o fosfolipídio 1,2-dipalmitoil-sn-glicero-3-[fosfatidil-rac-(1-glicerol)] (sal de sódio) (DPPG). Os filmes de Langmuir foram caracterizados com medidas de pressão e potencial de superfície, espectroscopia no infravermelho, e tensão superficial dinâmica. Para os filmes LB e automontados, empregaram-se espectroscopias de fluorescência, ultravioleta-visível e infravermelho e microgravimetria por cristal de quartzo. A peroxidase de raiz forte apresentou forte interação com DPPG, confirmada em filmes de Langmuir por medidas de pressão de superfície, elasticidade dinâmica e de espectroscopia de reflexão e absorção no infravermelho, com modulação por polarização (PM-IRRAS). A massa de peroxidase transferida em filmes Langmuir-Blodgett (LB) mistos com DPPG foi de aproximadamente 200 ng, de acordo com medidas com uma microbalança de cristal de quartzo. A atividade da HRP foi mantida no filme LB, inclusive com atividade catalítica maior do que em meio homogêneo e nos filmes automontados com quitosana. As medidas de atividade não afetaram a morfologia dos filmes LB, estudada com microscopia de força atômica (AFM), ao contrário dos filmes automontados. Conclui-se que a imobilização de HRP é mais eficiente num filme LB, com matriz fosfolipídica, apresentando boas perspectivas de emprego em biossensores de peróxido de hidrogênio. / A study has been performed on the interaction of the enzyme horseradish peroxidase (HRP) in nanostructured interfaces and their possible application in biosensors for hydrogen peroxide. The nanostructured films were obtained with the Langmuir, Langmuir-Blodgett (LB) and layer-by-layer (LbL) methods. The interaction between HRP and species at interfaces was investigated using materials that served as matrix for immobilization, viz. chitosan (Ch) and the phospholipid 1,2-dipalmytoil-sn-glycero-3-[phosphatidyl-rac-(1-glycerol)] (sodium salt) (DPPG). The Langmuir films were characterized with surface pressure, surface potential, elasticity measurements and polarization-modulation reflection and absorption infrared spectroscopy (PM-IRRAS). For LB and LbL films, use was made of fluorescence, absorption in the UV-vis. and infrared spectroscopy. HRP displayed strong interaction with DPPG, which was confirmed in Langmuir films with measurements of surface pressure, dynamic elasticity and PM-IRRAS. The mass of HRP transferred onto a solid support in a mixed LB film with DPPG was 200 ng, according to data from a quartz crystal microbalance. The HRP activity was preserved in the mixed LB film, with a catalytic activity that was even higher than in solution or in LbL films of HRP/Ch. The catalytic activity measurements did not affect the morphology of the LB films, studied with atomic force microscopy (AFM), in contrast to the LbL films. The main conclusion is that HRP immobilization is more efficient in an LB film with a phospholipid matrix, with good prospects for developing biosensors for hydrogen peroxide.
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Influência da âncora de glicosilfosfatidilinositol na imobilização da fosfatase alcalina de placa óssea imobilizada em sistemas miméticos de membranas celulares: monocamadas de Langmuir e filmes Langmuir-Blodgett de fosfolipídios / Influence of the glycosylphosphatidylinositol anchor in the immobilization of rat osseous plate alkaline phosphatase immobilized in biomimetic systems: phospholipid Langmuir monolayers and Langmuir-Blogett filmsCaseli, Luciano 13 April 2005 (has links)
Nesse trabalho, estudou-se a incorporação da fosfatase alcalina de placa óssea de ratos em dois tipos de sistemas modelo que mimetizassem uma membrana celular: as monocamadas de Langmuir e os filmes Langmuir-Blodgett (LB), ambos formados com fosfolipídios. No intuito de se investigar o papel da âncora de glicosilfosfatidilinositol (GFI), covalentemente ligada ao grupo carboxi-terminal da cadeia polipeptídica, duas formas da enzima foram estudadas: uma com a âncora GFI intacta, solubilizada por ação de um tensoativo não-iônico, e a outra sem a parte hidrofóbica dessa âncora, clivada por ação de uma fosfolipase específica. A primeira forma enzimática foi chamada de FAT (fosfatase alcalina solubilizada por tensoativo), e a segunda de FAC (fosfatase alcalina clivada). Diferenças marcantes na atividade superficial foram observadas entre as duas formas. Comparativamente, a forma FAT adsorve mais rapidamente à interface ar/água que a forma FAC, que mostra um tempo de indução significativo. A incorporação da forma FAT às monocamadas de ácido dimiristoilfosfatídico (DMPA) também ocorre mais rapidamente que a forma FAC. No entanto, o uso de alta força iônica acelerou a adsorção da forma FAC à interface ar/água (com ou sem DMPA). Uma pressão de superfície de exclusão de 20mN/m foi encontrado para a forma FAC, enquanto para a forma FAT, essa pressão representa uma mudança no perfil das curvas pressão x tempo. Isso revelou que, devido à presença da âncora GFI, essa forma enzimática é capaz de incorporar às monocamadas de DMPA, mesmo em altas pressões de superfície. Isotermas superficiais de monocamadas mistas de DMPA e fosfatase alcalina também mostraram diferentes perfis para duas formas enzimáticas estudadas. Enquanto a forma FAT provoca uma alteração na compressibilidade em pressões de até 20mN/m, a forma FAC desloca a curva pressão x área para áreas mais elevadas. Tal fato foi explicado pelo fato da forma FAT incorporar na monocamada preferencialmente com a âncora GFI posicionada entre as cadeias apolares do DMPA, enquanto a forma FAC deva incorporar a cadeia polipeptídica à interface lipídica . Microscopias de fluorescência e no ângulo de Brewster revelaram que a forma FAT provoca agregação espontânea do DMPA na interface ar/água, levando a uma microeterogeneidade, na qual três fases distintas podem ser observadas. A obtenção de espectros de infravermelho na interface ar/água, associada com medidas de atividade catalítica in situ, revelou que a atividade da fosfatase alcalina é modulada pela capacidade de empacotamento interfacial, medida pelo módulo de compressibilidade superficial. Em 20mN/m, há uma reorganização molecular na interface, o que vai restringir a flexibilização da cadeia polipeptídicia, que estará voltada para a interface ar/água. No entanto, ao menos até 30mN/m, nenhuma alteração conformacional foi detectada, como revelada pelos espectros de infravermelho. Filmes LB mistos de DMPA e as duas formas de fosfatase alcalina revelaram que o empacotamento máximo de proteína depende da presença da âncora GFI. Dados usando microgravimetria, atividade enzimática, infravermelho, elipsometria, e microscopia de força atômica mostraram que a adsorção da âncora na interface posiciona o eixo maior do elipsóide, formador da cadeia polipeptídica, paralelamente à matriz lipídica. Na ausência da âncora GFI, o posicionamento da cadeia polipeptídica na interface é aleatório, e para um alto grau de empacotamento, as interações entre os resíduos de aminoácidos intermoleculares favorecerão o posicionamento do eixo maior do elipsóide em uma posição mais perpendicular à interface lipídica / Não consta
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Efeitos da dimerização e modificações na porção N-terminal do peptídeo antimicrobiano Aureína 1.2 em sua interação com filmes de Langmuir e atividade biológica / Effects of dimerization and modifications in the N-terminal portion of the antimicrobial peptide Aurein 1.2 in its interaction with Langmuir monolayers and in its biological activityMontanha, Érica Azzolino 08 November 2016 (has links)
Filmes de Langmuir são usados como modelos simplificados de membranas celulares, cujas propriedades podem ser correlacionadas com efeitos fisiológicos de moléculas de interesse biológico, como os peptídeos antimicrobianos (PAMs). Nesta dissertação investigamos a interação do peptídeo Aureína 1.2, na forma de monômero (AU), dímero ((AU)2K) e com variações na porção N-terminal (KAU e DAU), com filmes de Langmuir obtidos do extrato lipídico da bactéria Escherichia coli. Todos os peptídeos injetados em concentrações de 20 a 200nM se incorporaram ao filme de Langmuir, causando expansão nas isotermas de pressão superficial, que foi significativamente maior para o dímero. O módulo de compressibilidade do filme de E. coli à pressão superficial correspondente à de uma membrana real praticamente dobrou, de cerca de 40mN/m para 80nM/m para o dímero, ao passo que para os outros peptídeos a alteração não foi significativa. Dos espectros de reflexão e absorção no infravermelho com modulação de polarização (PM-IRRAS), observou-se que todos os peptídeos interagiram tanto com as caudas quanto com as cabeças polares das moléculas do extrato de E. coli no filme de Langmuir. Diferentemente dos resultados de pressão e compressibilidade, não há tendência de um peptídeo ter interação mais relevante do que os outros. O maior efeito do dímero na expansão e compressibilidade do filme de Langmuir não se refletiu numa maior atividade bactericida contra E. coli, pois sabe-se da literatura que a atividade é maior para a Aureína 1.2 (AU). Provavelmente porque essa atividade deve depender da camada externa de lipopolissacarídeos de uma bactéria Gram-negativa. / Langmuir films are used as simplified cell membrane models whose properties can be correlated with physiological effects of molecules of biological interest, such as antimicrobial peptides (AMPs). In this dissertation we report on the interaction of Aurein 1.2 peptide as monomer (AU), dimer ((AU)2K) and modified peptide in the N-terminal portion (KAU and SAD), with Langmuir films obtained from a lipid extract of Escherichia coli. All peptides injected at concentrations from 20 to 200nM were incorporated into the Langmuir film, causing the surface pressure isotherm to expand, particularly for the dimer. The compressibility modulus of the E. coli Langmuir film at the surface pressure corresponding to an actual membrane nearly doubled, from about 40mN/m to 80nM/m for the dimer, whereas for the other peptides the change was not significant. From the polarization-modulated infrared reflection - absorption spectra (PM-IRRAS), we observed that all peptides interacted with both tails and polar heads of the molecules of E. coli extract in the Langmuir film. Unlike the results of pressure and compressibility, there was no tendency of a peptide having more relevant interaction than the others. The larger effect of the dimer in the expansion and compressibility of the Langmuir film was not reflected in a higher bactericidal activity against E. coli, since it is known from literature that the activity is higher for Aurein 1.2 (AU). Probably because this activity should depend on the outer layer of lipopolysaccharides of Gram-negative bacteria.
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The structure of langmuir monolayers probed with vibrational sum frequency spectroscopyGurau, Marc Cory 29 August 2005 (has links)
Langmuir monolayers can be employed as simple model systems to study interactions at surfaces. Such investigations are important to fields ranging from biology to materials science. Herein, several aspects of these films and their associated water structure have been examined with vibrational sum frequency spectroscopy (VSFS). This second order nonlinear optical spectroscopy is particularly well suited for simultaneous investigations of the monolayer and the associated water structure with unprecedented surface specificity. The structures of these systems were altered through the control of experimental parameters including monolayer pressure, subphase temperature, pH and ionic content. Thermodynamic information about structural changes in a fatty amine monolayer's hydrophobic region was obtained by observation of the pressure and temperature dependence of the monolayer's solid to liquid phase transition. Further studies used the coordination of divalent cations to acid monolayers to perturb the water layers nearest to the film which enabled a better understanding of the water related VSFS features from these hydrophilic interfaces. Information from both the monolayer and water structure was then combined in order to examine the role of water in mediating ion-biomaterial interactions, often expressed in terms of the Hofmeister series.
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Investigations of amino acid-based surfactants at liquid interfacesYang, Dengliang 01 November 2005 (has links)
Herein are presented collective studies of amino acid-based surfactants, also known as lipoamino acids, at liquid interfaces. Chapter III describes an investigation of domain morphology of N-Stearoylglutamic acid (N-SGA) Langmuir monolayers at the air/water interface by epifluorescence microscopy. Anisotropic feather-like domains were observed in L-enantiomeric monolayers while symmetric circular domains were found in racemic N-SGA monolayers. At a surface pressure of 30 mN/m the enantiomeric domains melted at 31 ??C while the racemic domains melted at 27 ??C. This result is exactly opposite to the behavior found in bulk crystals where the racemate melts at a higher temperature. These results were explained in terms of different molecular packing and hydrogen bonding between bulk crystals and two-dimensional thin films for enantiomeric and racemic compounds. Chapter IV summarizes the investigations of hydrogen bonding in N-acyl amino acid monolayers by vibrational sum-frequency spectroscopy (VSFS). The intermolecular hydrogen bonding interaction between the adjacent molecules through amide-amide groups in N-stearoylalanine (N-SA) is characterized by an NH stretch peak at 3311 cm-1. This is the first time that the amide NH stretching signals have been detected with the VSFS technique. A similar peak was detected at 3341 cm-1on N-SGA monolayer. The higher frequency indicates that the H-bond strength is weaker due to the larger size of the glutamic acid residue. The NH stretch mode can thus be used as a fingerprint of hydrogen bonding among amide-amide groups. A peak at 3050 cm-1 due to hydrogen bonding among carboxyl groups was also resolved from the VSFS spectra. Molecular models of intermolecular hydrogen bonding were proposed.
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Model membrane interactions with ions and peptides at the air/water interfaceMaltseva, Elena January 2005 (has links)
The interactions between peptides and lipids are of fundamental importance in the functioning of numerous membrane-mediated biochemical processes including antimicrobial peptide action, hormone-receptor interactions, drug bioavailability across the blood-brain barrier and viral fusion processes. Alteration of peptide structure could be a cause of many diseases.<br>
Biological membranes are complex systems, therefore simplified models may be introduced in order to understand processes occurring in nature. The lipid monolayers at the air/water interface are suitable model systems to mimic biological membranes since many parameters can be easily controlled. In the present work the lipid monolayers were used as a model membrane and their interactions with two different peptides B18 and Amyloid beta (1-40) peptide were investigated.<br>
B18 is a synthetic peptide that binds to lipid membranes that leads to the membrane fusion. It was demonstrated that it adopts different structures in the aqueous solutions and in the membrane interior. It is unstructured in solutions and forms alpha-helix at the air/water interface or in the membrane bound state. The peptide has affinity to the negatively charged lipids and even can fold into beta-sheet structure in the vicinity of charged membranes at high peptide to lipid ratio. It was elucidated that in the absence of electrostatic interactions B18 does not influence on the lipid structure, whereas it provides partial liquidization of the negatively charged lipids. The understanding of mechanism of the peptide action in model system may help to develop the new type of antimicrobial peptides as well as it can shed light on the general mechanisms of peptide/membrane binding.<br>
The other studied peptide - Amyloid beta (1-40) peptide, which is the major component of amyloid plaques found in the brain of patients with Alzheimer's disease. Normally the peptide is soluble and is not toxic. During aging or as a result of the disease it aggregates and shows a pronounced neurotoxicity. The peptide aggregation involves the conformational transition from a random coil or alpha-helix to beta-sheets. Recently it was demonstrated that the membrane can play a crucial role for the peptide aggregation and even more the peptide can cause the change in the cell membranes that leads to a neuron death. In the present studies the structure of the membrane bound Amyloid beta peptide was elucidated. It was found that the peptide adopts the beta-sheet structure at the air/water interface or being adsorbed on lipid monolayers, while it can form alpha-helical structure in the presence of the negatively charged vesicles. The difference between the monolayer system and the bulk system with vesicles is the peptide to lipid ratio. The peptide adopts the helical structure at low peptide to lipid ratio and folds into beta-sheet at high ratio. Apparently, Abeta peptide accumulation in the brain is concentration driven. Increasing concentration leads to a change in the lipid to peptide ratio that induces the beta-sheet formation. The negatively charged lipids can act as seeds in the plaque formation, the peptide accumulates on the membrane and when the peptide to lipid ratio increases it the peptide forms toxic beta-sheet containing aggregates. / Wechselwirkungen zwischen Peptiden und Lipiden sind von grundlegender Bedeutung für die Funktion vieler Membran-vermittelter biochemischer Prozesse wie der Wirkung von antimikrobiellen Peptiden, Hormon-Rezeptor Wechselwirkungen, Bioverfügbarkeit von Arzneistoffen durch die Blut-Hirn-Schranke und viraler Fusionsprozesse. Veränderungen in der Peptidstruktur können die Ursache für viele Erkrankungen sein.<br>
Biologische Membranen sind für grundlegende physikalisch-chemische Untersuchungen von Naturprozessen zu komplexe Systeme, so dass vereinfachte Modelle für solche Studien eingesetzt werden. Eine Lipidmonoschicht an der Wasser/Luft Grenzfläche ist ein geeignetes Modellsystem für eine Membranoberfläche. Viele physikalisch-chemischen Parameter können auf einfache Weise gezielt verändert werden. In der vorliegenden Arbeit wurden Lipidmonoschichten genutzt, um Wechselwirkungen mit zwei unterschiedlichen Peptiden (B18 and Amyloid Beta (1-40) Peptid) zu untersuchen.<br>
B18 ist ein oberflächenaktives synthetisches Peptid, das an Lipidmembranen bindet und zu Membranfusion führt. Es kann verschiedene Sekundärstrukturen ausbilden. So ist B18 in wässrigen Lösungen ungeordnet und bildet eine alpha-helikale Struktur an der Wasser/Luft Grenzfläche. Das Peptid hat eine große Affinität zu negativ geladenen Lipiden und kann in der Nähe von geladenen Membranoberflächen bei einem großen Peptid/Lipid Verhältnis eine Beta-Faltblatt Struktur ausbilden. Beim Fehlen elektrostatischer Wechselwirkungen hat B18 keinen Einfluss auf die Lipidstruktur. Es wirkt jedoch strukturabbauend auf anionische Lipide. Das Verständnis der Peptidwirkungen in Modellsystemen kann helfen, generelle Mechanismen von Peptide-Membran Wechselwirkungen zu verstehen und zur Entwicklung neuer antimikrobieller Peptide beizutragen.<br>
Amyloid Beta (1-40) Peptid ist die Hauptkomponente von Amyloid-Plaque, das im Gehirn von Alzheimer Patienten gefunden wird. Normalerweise ist das Peptid löslich und nicht toxisch. Hohe Neurotoxizität wird bei Peptidaggregation, die eine Strukturumwandlung von ungeordnet oder alpha-helikal zu Beta-Faltblatt nach sich zieht, beobachtet. In der vorliegenden Arbeit wurde die Struktur des Membran-gebundenen Amyloid Beta (1-40) Peptids untersucht. Es zeigte sich, dass das Peptid nach Adsorption an die Wasser/Luft Grenzfläche oder an Lipidmonoschichten eine Beta-Faltblatt Struktur ausbildet. Eine alpha-helikale Sekundärstruktur wird nur bei Anwesenheit negativ geladenen Lipidvesikel gefunden. Der entscheidende Unterschied zwischen den Monoschicht- und Vesikel-Systemen ist das Peptid/Lipid Verhältnis. Die alpha-helikale Struktur wird nur bei kleinem Peptid/Lipid Verhältnis beobachtet, während bei großem eine Beta-Faltblatt Struktur auftritt. Steigende Konzentration an Amyloid Beta (1-40) Peptid führt zum Anstieg des Peptid/Lipid Verhältnisses und damit zur Ausbildung der Beta-Faltblatt Struktur. Negativ geladene Lipide können somit als Keimpunkte für die Plaquebildung fungieren.
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