Oxidação direta do etileno glicol sobre catalisadores eletroquímicos binários à base de Pt, Pd, e Sn suportados em carbono para aplicação em células alcalinas / Direct oxidation of ethylene glycol by binary electrochemical catalysts based on Pt, Pd and Sn supported on carbon substrate for application in alkaline fuel cells

Leticia Lopes de Souza

15 June 2016

Os catalisadores eletroquímicos binários de PtSn/C, PdSn/C e PtPd/C foram sintetizados em diferentes proporções pelo método da redução via borohidreto, posteriormente estes foram caracterizados por microscopia eletrônica de transmissão, difração de raios X, espectroscopia no infravermelho por transformada de Fourier (PtSn/C e PdSn/C) e energia dispersiva de raios X. As atividades eletroquímicas dos diferentes materiais preparados foram avaliadas por intermédio de voltametria cíclica, cronoamperometria e curvas de polarização em célula a combustível alimentada diretamente por etileno glicol em eletrólito alcalino. As curvas de densidade de potência indicaram que os catalisadores eletroquímicos contendo Sn e Pd são mais ativos para a reação de oxidação do etileno glicol, especialmente a composição 70%:30% - relação molar entre os metais suportados em carbono - dos catalisadores PtSn/C, PdSn/C e PtPd/C todos superando as medidas de potência do Pt/C. Este resultado indica que a adição de Sn e Pd favorece a oxidação do etileno glicol em meio alcalino. O melhor desempenho observado para os catalisadores eletroquímicos PtSn/C, PdSn/C e PtPd/C (70%:30%) poderia estar associado à sua maior seletividade quanto a formação de oxalato, ou seja , a formação deste produto resulta em um maior número de elétrons, por consequência em maiores valores de corrente. / Binary electrochemical catalysts PtSn/C, PdSn/C and PtPd/C were synthesized in different proportions by the method of reduction via borohydride. These were characterized by transmission electron microscopy, X-ray diffraction, Fourier transform infrared spectroscopy (PtSn/C and PdSn/C) and energy dispersive X-ray. The electrochemical activities of the different materials prepared were evaluated by cyclic voltammetry, chronoamperometry and polarization curves for fuel cell powered directly by ethylene glycol in an alkaline electrolyte. Power density curves indicated that the electrochemical catalysts Sn-containing or Pd-containing are more active for ethylene glycol oxidation reaction, particularly the (70%:30%) composition of PtSn/C, PdSn/C and PtPd/C, all of them exceeding power measurements of Pt/C. These results indicate that the addition of Sn and Pd promotes the oxidation of ethylene glycol in an alkaline medium and this improved performance may be associated with a higher selectivity for the formation of oxalate that results in a larger number of electrons, consequently enhancing the current values.

célula alcalina

etileno glicol

infravermelho

alkaline

ethylene glycol

fourier transform infrared spectroscopy

A eletrooxidação de etileno glicol: estudo dos caminhos reacionais em superfícies de PtRu em meio alcalino / The electrooxidation of ethylene glycol: study of the reaction paths in PtRu surfaces in alkaline medium

Nascimento, Diego Rogério Pinto do

27 July 2016

Submitted by Rosivalda Pereira (mrs.pereira@ufma.br) on 2017-06-02T19:15:27Z No. of bitstreams: 1 DiegoNascimento.pdf: 1137977 bytes, checksum: 18e235c8d743ce1d2f6c7baa61ad30c3 (MD5) / Made available in DSpace on 2017-06-02T19:15:27Z (GMT). No. of bitstreams: 1 DiegoNascimento.pdf: 1137977 bytes, checksum: 18e235c8d743ce1d2f6c7baa61ad30c3 (MD5) Previous issue date: 2016-07-27 / Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPQ) / Short chain alcohols have been studied for possible use in fuel cells. The ethylene glycol oxidation electrode Pt and PtRu, in alkaline medium, showed great efficiency and increasing the current density was evidenced by a gradual rise in temperature, which confirms that the temperature is a significant factor for the electrooxidation glycol favoring the formation of oxygenated species and facilitating the oxidation adsorbates. The ethylene glycol oxidation products on the surfaces of Pt and PtRu were identified by high-performance liquid chromatography and the presence of glycolaldehyde was confirmed as alcohol oxidation product of Pt and glycolaldehyde and glicoato on surfaces of PtRu. Bimetallic PtRu electrodes were prepared by electrodeposition in five different proportions: 94:06; 90:10; 88:12; 83:17 and 77:23. The percentage of both metals was determined by EDX technique. significant currents were obtained from these electrodes, since they were used as working electrodes. The best results are related to glycol oxidation on PtRu electrode (77:23), because it made possible the oxidation of alcohol to study less anodic potential, which was verified by glycol oxidation beginning around 0.25 V, as well have caused a significant decrease in the region characteristic of hydrogen. Thus, the PtRu alloy catalyst is considered to be good catalyst for CO oxidation and ethylene glycol in the alkaline medium. The number of moles to glycol oxidation products were determined at temperatures of 25 to 55 ° C for both a flat eterodo Pt as to eletrodeposito PtRu (77:23) and its activation energy was determined for each electrode the current data from the apalicação equaçãi Arrhenius, meeting 24.29 and 32.02 kJ.mol-1 to the flat electrode of Pt and PtRu eletrodepositdos respectively. / Álcoois de cadeias pequenas têm sido estudados para possível uso em células de combustível. A oxidação de etileno glicol em eletrodos de Pt e PtRu, em meio alcalino, mostrou grande eficiência e o aumento da densidade de corrente foi evidenciado por uma elevação gradual da temperatura, o que confirma que a temperatura é um fator significativo para a eletrooxidação do glicol, favorecendo a formação de espécies oxigenadas e facilitando a oxidação de adsorbatos. Os produtos de oxidação de etileno glicol em superfícies de Pt e PtRu foram identificados por cromatografia líquida de alta eficiência e a presença de glicolaldeido foi confirmada como produto de oxidação do álcool sobre Pt e glicolaldeido e glicoato sobre superfícies de PtRu. Os eletrodos bimetálicos de PtRu, foram preparados por eletrodeposição em cinco proporções diferentes: 94:06; 90:10; 88:12; 83:17 e 77:23. A porcentagem de ambos os metais foi determinado pela técnica de EDX. Foram obtidas correntes significativas a partir destes eletrodos, uma vez que os mesmos foram utilizados como eletrodos de trabalho. Os melhores resultados estão relacionados à oxidação do glicol em eletrodo PtRu (77:23), pois possibilitou a oxidação do álcool em estudo a potenciais menos anódicos, o que foi verificado pelo inicio de oxidação do glicol por volta de 0,25 V, além de ter ocasionado uma significativa diminuição na região característica do hidrogênio. Assim, o catalisador de liga de PtRu é considerado como bom catalisador para oxidação de CO e de etileno glicol no meio alcalino. O número de mol para os produtos de oxidação do glicol foram determinados às temperaturas de 25 e 55°C tanto para um eterodo liso de Pt quanto para o eletrodeposito de PtRu (77:23) e as respectivas energias de ativação para cada eletrodo foi determinada pelos dados de corrente obtidos a partir da apalicação da equaçãi de Arrhenius, encontrando-se 24,29 e 32,02 KJ.mol-1 para o eletrodo liso de Pt e PtRu letrodepositdos, respectivamente.

Eletrooxidação

Etileno glicol

Produtos

Temperatura

Electrooxidation

Ethylene glycol

Products

Temperature

Química Analítica

Vitrificação de embriões Mus domesticus domesticus contidos em volumes diferentes de 9,0 m de etileno glicol. / Vitrification of mus domesticus domesticus embryos exposed to differents volumes of 9.0 m ethylene glycol solution

Assaf, Sabrina Silveira

January 2003

Os experimentos tiveram como objetivo determinar a taxa de eclosão dos embriões vitrificados em volumes diferentes de 9,0 M de etileno glicol. Simultaneamente, testou-se dois procedimentos de estocagem dos fios de teflon, denominados caixa de aço inoxidável e globete/raque. No experimento I, os 881 embriões coletados foram distribuídos em 4 tratamentos: tratamento 1 (T1= controle): 307 embriões foram cultivados in vitro em meio PBSm, acrescido de 0,4% de BSA; tratamento 2 (T2): 292 embriões foram expostos à solução de glicerol 10% acrescida de 0,4% de BSA, envasados em palhetas de 0,25 mL e submetidos ao congelamento pelo método rápido em Biocool; tratamento 3 (T3): 138 embriões foram expostos durante 2 minutos à solução de desidratação (10% de EG + 6% BSA em PBSm) e então transferidos para a solução de vitrificação (50% de EG + 6% de BSA em PBSm), onde permaneceram por 30 segundos e foram colocados em volume de 1 μL no interior de um fio de teflon, medindo 0,4 mm de diâmetro, 2,0 cm de comprimento e 0,05 mm de espessura. Os fios foram acondicionados em uma caixa de aço inoxidável para serem armazenados em nitrogênio líquido; tratamento 4 (T4): 144 embriões foram expostos à solução de desidratação (10% de EG + 6% BSA em PBSm) e após 2 minutos, foram transferidos para a solução de vitrificação (50% de EG + 6% BSA em PBSm), onde permaneceram por 30 segundos, sendo após transferidos para um volume de 1 μL no interior do fio de teflon. Os fios de teflon foram estocados em globetes unidos às raques e mantidos em nitrogênio líquido. Após o aquecimento, os embriões foram cultivados em PBSm suplementado com 0,4% de BSA. As taxas de eclosão embrionária observadas foram: T1=76,29% (245/307); T2=41,05% (117/292); T3=37,98% (54/138) e T4=26,78% (37/144). No segundo experimento, 747 embriões foram distribuídos em 3 tratamentos: tratamento 1 (T1= controle): 80 embriões foram cultivados in vitro em meio KSOM acrescido de 0,4% de BSA; tratamento 2 (T2): 334 embriões expostos em solução de glicerol 10% acrescida de 0,4% de BSA, foram envasados em palhetas de 0,25 mL e submetidos ao congelamento pelo método rápido em Biocool; tratamento 3 (T3): 333 blastocistos foram expostos durante 2 minutos à solução de desidratação (10% de EG + 0,4% BSA em PBSm) e então transferidos para tubos eppendorf de 2,0 mL em contato com a solução de vitrificação (50% de EG + 0,4% BSA em PBSm). Após o cultivo in vitro, as taxas de eclosão embrionária observadas nos 3 tratamentos foram respectivamente: 88,75% (71/80), 40,44% (141/334) e 19,70% (66/333). Baseado nesses resultados conclui-se que embriões Mus domesticus domesticus submetidos à técnica de vitrificação após exposição à solução de 9,0 M de etileno glicol e envase em fios de teflon assegurou índices satisfatórios de sobrevivência embrionária. As taxas de sobrevivência dos embriões Mus domesticus domesticus foi independente do procedimento de estocagem em botijão de nitrogênio líquido. A vitrificação em solução de 9,0 M de etileno glicol com envase em tubos eppendorf não foi eficiente para promover altas taxas de sobrevivência embrionária, mas proporcionou segurança biológica aos embriões, durante o armazenamento. / This work was performed with Mus domesticus domesticus embryos to verify the in vitro viability of vitrified embryos using differents volumes of ethylene glycol–based solution. The experiment I consisted of four treatments. The 881 collected embryos were arranged as follows: treatment 1(control): 307 fresh embryos were cultured in vitro in PBSm + 0.4% BSA without being exposed to either dehydration or cryoprotectants agents; treatment 2: 292 embryos were loaded into 0.25 mL french straws containing 10% glycerol + 0.4% BSA in PBSm and after 10 minutes the straws were submitted to the rapid-freezing procedure (Biocool®, controlled freezer); treatment 3:138 embryos were exposed during 2 minutes to a dehydration solution (10% ethylene glycol + 6% BSA in PBSm) and then transferred to the vitrification solution (50% ethylene glycol + 6% BSA in PBSm) in teflon wire with 0.4 mm diameter, 2 cm length and 0.05 mm thickness containing the drop of 1μL volume, and placed into stainless steel box for the storage in LN2; treatment 4:144 embryos were exposed to a dehydration solution (10% ethylene glycol + 6% BSA in PBSm) and after 2 minutes were transferred to the teflon wire, that was previousily loaded with 1μL of the vitrification solution (50% ethylene glycol + 6% BSA in PBSm). Finally, the teflon wires were placed into plastic globets attached to aluminum canes and maintained in LN2. After thawing, the embryos were serially washed in PBSm, and then cultured in PBSm supplemented with 0.4% BSA. The hatched blastocyst rates observed in the treatments were: T1=76.29% (245/307); T2=41.05% (117/292); T3=37.98% (54/138) and T4=26.78% (37/144). In the second experiment, 747 embryos were arranged as follows: treatment 1(control): consisted of 80 fresh embryos cultured in vitro in KSOM medium + 0.4% BSA without being exposed to either dehydration or cryoprotectants agents; treatment 2: 334 embryos were loaded into 0.25 mL french straws containing 10% glycerol + 0.4% BSA in PBSm and after 10 minutes the straws were submitted to the rapid-freezing procedure (Biocool®, controlled freezer); treatment 3: 333 embryos were exposed during 2 minutes to a dehydration solution (10% ethylene glycol + 0.4% BSA in PBSm) and then transferred to the eppendorf tubes loaded with the vitrification solution (50% ethylene glycol + 0.4% BSA in PBSm). After in vitro culture, the hatched blastocysts rates observed were: T1=88.75% (71/80); T2=40.44% (141/334) and T3=19.70% (66/333). Based on these results it is concluded that the embryos of Mus domesticus domesticus submitted to vitrification procedure after being exposed to 9.0 M of ethylene glycol – based solution and loaded in teflon wires were efficient to promote satisfactory embryo survival rates. The survival rate of Mus domesticus domesticus embryos was independent of the LN2 storage procedure. The vitrification procedure after being exposed to 9.0 M of ethylene glycol – based solution and loaded in eppendorf tubes were not efficient to promote high embryo survival rate, but to warrant the embryo’s biologically security during storage in liquid nitrogen.

Reproducao animal : Camundongos

Etileno Glicol

Vitrification

Mouse

Embryos

Load

Ethylene glycol

Effects of Electronic Cigarette Liquid Solvents Propylene Glycol and Vegetable Glycerin on User Nicotine Delivery, Heart Rate, Subjective Effects, and Puff Topography

Spindle, Tory

01 January 2018

Electronic cigarettes (ECIGs) are a class of tobacco products that use a heating element to aerosolize a liquid, typically containing nicotine, allowing for user inhalation. Despite their rapid growth in popularity, little is known about ECIGs including how certain device and liquid factors influence nicotine delivery, user physiological and subjective responses, and puffing behavior (puff topography). Limited pre-clinical research has demonstrated that the ratio of two solvents commonly found in ECIG liquids, propylene glycol (PG) and vegetable glycerin (VG), may have an influence on the nicotine content of ECIG aerosols. However, the extent to which PG:VG ratio in ECIG liquids influences acute effects experienced by ECIG users is unknown. The primary purpose of this clinical laboratory study was to examine the influence of PG:VG ratio on plasma nicotine concentration, heart rate (HR), subjective effects, and puff topography in experienced ECIG users. Thirty ECIG-experienced individuals participated in four independent laboratory conditions that differed only by the PG:VG ratio in the ECIG liquid (100:0, 55:45, 20:80, and 2:98). In each condition, participants used a 3.3 volt “eGo” ECIG battery attached to a 1.5 Ohm dual coil “cartomizer” loaded with 1 ml of ECIG liquid (nicotine concentration: 18 mg/ml). Participants completed two ECIG use bouts (10 puffs with 30 sec inter-puff-interval) in each study condition. ECIG PG:VG ratio had a direct influence on nicotine delivery, subjective effects, and puff topography. Nicotine delivery and overall nicotine intake were highest following the use of the liquids containing mostly PG, despite participants taking significantly shorter and smaller puffs in these conditions, suggesting PG may be a more efficient nicotine-delivery vehicle than VG. Abstinence symptoms were suppressed similarly across all PG:VG ratios, and HR also increased in a similar fashion in all conditions following ECIG use. Participants reported significantly lower scores on items assessing sensory ECIG effects following use of the 100PG:0VG liquid, indicating a lower overall satisfaction with this liquid. Further evaluating the influence of PG and VG and other ECIG device and liquid characteristics on ECIG acute effects using clinical laboratory methodologies could inform regulations of these products.

electronic cigarettes

nicotine delivery

propylene glycol

vegetable glycerin

Health Psychology

Pharmacology

Effect of Polyethylene glycol 4000 supplementation on the performance of the indigenous Pedi goats fed different levels of Acacia nilotica leaf meal and Ad libitum buffalo grass hay.

Motubatse, Moakgosweng Robby

January 2006

Thesis (M.Sc. (Agriculture)) --University of Limpopo, 2006 / Two experiments were carried out to determine the effect of the level of Acacia nilotica leaf meal supplementation plus 23 g polyethylene glycol 4000 on diet intake, digestibility, and growth rate of indigenous Pedi goats fed ad libitum Buffalo grass, Buchloe dactyloides, hay. The first experiment lasted for 37 days, with the first 30 days being for adaptation and the last 7 days being for collection. Twenty yearling male Pedi goats weighing 22 ± 0.5 kg live weight were allocated to 4 treatments in a 2 x 2 Factorial arrangement in a Completely Randomised Design. Acacia nilotica leaf meal contained 120 g crude protein per kg DM, indicating its potential as a browse source for ruminants. It, also, contained high amounts of total phenolics (2.04 % DM) and low amounts of condensed tannins, both extracted (0.37 % DM) and unextracted (1.83 % DM). Increasing the level of Acacia nilotica leaf meal supplementation to 120 g increased (P<0.05) crude protein intake (38 g/kg DM) when compared to 80 g supplementation (34 g/kg DM). Supplementation with 23 g PEG 4000 increased (P<0.05) the crude protein intake where goats were supplemented with 120 g of A. nilotica leaf meal. However, PEG 4000 supplementation did not have an effect (P>0.05) on intake when goats were supplemented with 80 g of Acacia nilotica leaf meal. Supplementation with 120 g of Acacia nilotica leaf meal increased (P<0.05) diet digestibility of DM (0.57), OM (0.60) and CP (0.71) by the goats. Similarly, supplementation with 23 g PEG 4000 increased (P<0.05) DM (0.65), OM (0.66) and v CP digestibilities (0.76) where goats were supplemented with 120 g of A. nilotica leaf meal. Polyethylene glycol 4000 also increased (P<0.05) diet CP digestibility where goats were supplemented with 80 g of Acacia nilotica leaf meal. However, 23 g PEG 4000 did not have a significant (P>0.05) effect on diet digestibility of DM and OM where goats were supplemented with 80 g of Acacia nilotica leaf meal. In vivo NDF and ADF digestibility were not affected by the treatments. Level of Acacia nilotica leaf meal supplementation plus 23 g of PEG 4000 had a significant (P<0.05) effect on the daily live weight change of the goats. The effect was higher where goats were supplemented with 120 g of A. nilotica leaf meal when compared to 80 g supplementation. Blood urea concentrations were improved (P<0.05) by level of A. nilotica supplementation and PEG supplementation. It is concluded that PEG 4000 has the potential to improve the feeding value of Acacia nilotica leaf meal and can, therefore, be used in the feeding systems for ruminant animals. The second experiment determined the effect of A. nilotica leaf meal supplementation and PEG 4000 supplementation on in vitro diet digestibility. Level of Acacia nilotica leaf meal supplementation plus 23 g PEG supplementation improved (P<0.05) in vitro diet DM, OM and CP digestibilities where 120 g Acacia nilotica leaf meal was supplemented. Similarly, 23 g PEG 4000 supplementation also improved (P<0.05) in vitro diet CP digestibility where 80 g Acacia nilotica leaf meal was supplemented. However, level of A. nilotica supplementation plus PEG 4000 supplementation had no vi effect (P>0.05) on in vitro NDF and ADF digestibilities. In vivo diet DM, OM and CP digestibilities were positively and significantly (P<0.05) correlated with in vitro diet DM, OM and CP digestibilities. It is, therefore, concluded that in vitro diet DM, OM and CP digestibilities have good capacity to predict in vivo diet DM, OM and CP digestibilities. / National Research Foundation. Working Solutions International

Polyethylene glycol 4000

Indigenous Pedi goats

Acacia nilotica

Buffalo grass

Conception et Synthèse de Nouvelles Molécules Cages pour des Applications en IRM du Xénon

Delacour, Léa

19 September 2011

L'Imagerie par Résonance Magnétique (IRM) est une technique d'imagerie médicale largement répandue dans les milieux hospitaliers pour le diagnostic de pathologies. Elle repose classiquement sur la détection du proton (IRM 1H) et permet de visualiser des tissus en profondeur avec une très bonne résolution temporelle et spatiale. Cependant, cette méthode souffre encore de sa faible sensibilité. Une des solutions consiste en l'introduction et la détection de xénon hyperpolarisé. En effet, le xénon est un gaz non toxique, très sensible à son environnement chimique et adapté pour l'IRM. Cependant, il n'est spécifique d'aucun récepteur biologique et nécessite des molécules particulièrement adaptées pour son encapsulation. La détection de cibles spécifiques se fait par des biosondes constituées de molécules cages fonctionnalisées par une antenne de reconnaissance d'un récepteur spécifique. Le xénon vient s'encapsuler dans cette molécule hôte et permet la localisation de la cible biologique. Parmi les molécules cages répertoriées dans la littérature, les cryptophanes présentent la plus forte affinité connue pour le xénon et sont donc les plus prometteuses. Les cryptophanes sont constitués de deux unités de type cyclotribenzylène reliées entre elles par trois chaînes pontantes. Ils ont été synthétisés pour la première fois par l'équipe d'A. Collet au Collège de France au début des années 1980. L'objectif de cette thèse a été de synthétiser et de fonctionnaliser de nouveaux cryptophanes.

IRM

cryptophane

xénon

biosonde

hyperpolarisation

molécule höte

cyclotribenzylène

fonctionnalisation

polyéthylène glycol

Couches moléculaires sur silicium pour la détection sélective de protéines

Perez, Emmanuel

25 November 2011

Les biopuces sont des outils d'analyse et de diagnostic de plus en plus utilisés dans le domaine médical et celui de la sécurité. Les puces à protéines sont particulièrement intéressantes car les protéines sont les manifestations directes de l'activité cellulaire. Ces puces sont généralement constituées d'un support sur lequel sont déposés des sondes possédant une affinité particulière avec les cibles à détecter. Cependant, leur sélectivité et sensibilité n'est parfois pas suffisante pour détecter de manière fiable les concentrations létales des certaines toxines, en particulier à cause de l'adsorption non spécifique des cibles sur la surface et de le fragilité de la chimie d'immobilisation des sondes. Cette thèse s'est attelée à améliorer ces paramètres en proposant une chimie contrôlée sur silicium qui, en utilisant des molécules composées d'un alcène et d'une chaîne poly(éthylène glycol), a permis de très largement limiter cette adsorption indésirable, tandis que la présence d'un groupement acide carboxylique en surface a permis l'immobilisation covalente des sondes aptamères capables de reconnaître des protéines.

Biocapteur

Protéines

Poly(éthylène glycol)

Silicium

Fluorescence

Aptamère

Pharmaceutical Properties of Nanoparticulate Formulation Composed of TPGS and PLGA for Controlled Delivery of Anticancer Drug

Mu, L., Chan-Park, Mary Bee-Eng, Yue, Chee Yoon, Feng, S.S.

01 1900

A suitable management of the pharmaceutical property is needed and helpful to design a desired nanoparticulate delivery system, which includes the carrier nature, particle size and size distribution, morphology, surfactant stabiliser according to the technique applied, drug-loading ratio and encapsulation efficiency, surface property, etc. All will influence the in vitro release, in vivo behaviour and tissue distribution of administered particulate drug loaded nanoparticles. The main purpose of the present work was to determine the effect of drug loading ratio when employing TPGS as surfactant stabiliser and/or matrix material to improve the nanoparticulate formulation. The model drug employed was paclitaxel. / Singapore-MIT Alliance (SMA)

biomaterials

drug delivery

surfactant stabiliser

Paclitaxel

Probing Protein Adsorption Modes onto Poly(Ethylene Glycol) Brushes by Neutron Reflection

Schollier, Audrey

18 March 2011

Adsorption of proteins at interfaces has an important role in biotechnological and pharmaceutical applications. Indeed, several undesirable processes are related to protein adsorption, as for example: fouling of contact lenses, clotting on blood contacting devices, triggering inammation around articial organs, diminished circulation time of therapeutic proteins and drug bearing liposomes. Neutral water soluble polymers, such as poly(ethylene glycol) (PEG), are used to repress protein adsorption: by coating the surface with a polymer brush, a "cushion" is created between the protein and the surface, that can reduce, or even completely repress the adsorption. Understanding the mechanism that inhibits the adsorption at interfaces is an active field of research, and could lead to relevant improvements in biomaterials performances and design. A clear understanding of the mechanism of protein adsorption onto polymer brushes is still missing. The first models describing the interactions of a polymer brush with adsorbing particles predicted two adsorption modes: primary adsorption at the grafting surface, and secondary adsorption at the outer edge of the brush (occurring for large cylindrical proteins). Primary adsorption can be repressed by increasing the grafting density of the brush, and secondary adsorption by increasing its thickness, in agreement with the experiments reported in the literature. But experimental evidences (a maximum in the adsorbed amount observed for long brushes) suggested then the existence of a third mode: ternary adsorption within the brush itself, due to attractive interactions between the protein and the brush. Standard techniques can in general only probe the total adsorbed amount. The aim of this work was to separate primary and ternary adsorption isotherms, by using neutron reectivity and deuterated proteins. As neutrons interact differently with hydrogen and deuterium atoms, the contrast between the hydrogenated brush and the deuterated protein is high enough to separate the two contributions. We studied the adsorption of deuterated myoglobin on PEG brushes with different degrees of polymerisation (N = 56, 146 and 770), and as a function of the area per grafted chain. The contribution of primary and ternary adsorption was separated for the different systems, and the adsorbed amount was extracted and the adsorption isotherms compared to the theoretical predictions. The ability to distinguish between the different adsorption modes, and the quantification of their relative contribution to the overall amount of adsorbed proteins, represents a major advance in optimising surface properties. In particular, the occurrence of ternary adsorption onto PEG brushes affects their status as tool for repressing protein adsorption. L’adsorption de protéines aux interfaces a un rôle important pour certaines applications pharmaceutiques ou biotechnologiques. En effet, plusieurs processus indésirables sont liés à l’adsorption de protéines, par exemple l’encrassement de lentilles de contact, la coagulation dans des appareils contenant du sang, l’inflammation d’organes artificiels ou encore la diminution du temps de circulation dans le corps de protéines ou liposomes thérapeutiques. Certains polymères, tels que le polyéthylène glycol (PEG), sont utilisés pour réprimer l’adsorption de protéines : en greffant une brosse de PEG sur la surface, une couche est créée entre la protéine et celle-ci qui diminue, voire même réprime complètement l’adsorption. Comprendre le mécanisme qui entrave l’adsorption aux interfaces est un sujet de recherche actif, qui pourrait mener à des améliorations significatives dans la conception de biomatériaux. À ce jour, la compréhension du mécanisme d’adsorption de protéines sur des brosses de polymère n’est pas claire. Les premiers modèles décrivant les interactions entre brosses de polymères et particules adsorbantes prédisaient deux modes d’adsorption : l’adsorption primaire sur la surface de greffage, et l’adsorption secondaire à l’extérieur de la brosse (pour les grandes protéines cylindriques uniquement). L’adsorption primaire peut-être réprimée en augmentant la densité de greffage de la brosse, et l’adsorption secondaire en augmentant son épaisseur, en accord avec les expériences reportées dans la littérature. Mais d’autres évidences expérimentales (un maximum dans la quantité adsorbée observé pour les brosses longues) ont ensuite suggéré l’existence d’un troisième mode : l’adsorption ternaire à l’intérieur même de la brosse, due aux interactions attractives entre la protéine et la brosse. Les techniques standards peuvent en général mesurer la quantité adsorbée totale. Le but de ce travail était de séparer les isothermes d’adsorption primaire et ternaire, en utilisant la réflectivité de neutrons et des protéines deutérées. Comme les neutrons interagissent différemment avec les atomes d’hydrogène ou de deutérium, le contraste entre la brosse hydrogénée et la protéine deutérée est ainsi suffisant pour séparer les deux contributions. Nous avons étudié l’adsorption de myoglobine deutérée sur des brosses de PEG avec différents degrés de polymérisation (N = 56, 146 and 770), en fonction de l’aire par chaîne Σ. La contribution des adsorptions primaire et ternaire put être séparée pour les différents systèmes, et les quantités adsorbées extraites pour finalement comparer les isothermes d’adsorption aux prédictions théoriques. La possibilité de distinguer les différents modes d’adsorption, et la quantification de leur contribution relative à la quantité totale de protéines adsorbées représente une avancée majeure dans l’optimisation des propriétés des surfaces. L’adsorption ternaire dans les brosses de PEG en particulier remet en question leur utilisation pour réprimer l’adsorption de protéines.

poly(ethylene glycol)

polymer

brush

protein

PEG

adsorption

neutron reflection

polymère

réflection de neutrons

protéine

brosse

Elaboration, structuration et propriétés rhéologiques de nanocomposites polymères modèles à base de Laponite

Abakar Adam, Omar

24 September 2012

Ce travail concerne l'étude du comportement rhéologique de nanocomposites modèles à base de Laponite dans du polyoxyde d'éthylène ou des mélanges polyoxyde d'éthylène avec du polyméthacrylate de méthyle. L'influence des paramètres moléculaires, masse molaire de la matrice et mode de protection des particules sur les propriétés rhéologiques a été étudiée. La meilleure dispersion est obtenue à partir d'une solution, la dilution d'un mélange maître conduisant à des matériaux hétérogènes. Les mélanges POE/PMMA sont compatibles à l'état fondu dans toute la gamme de concentrations mais hétérogènes à température ambiante au-dessus de 30% en poids de particules. En diluant un mélange Laponite/PEO dans le PMMA, nous avons montré que ces domaines se concentrent en particules en dessous de 30% de PEO et qu'une cocontinuité de phases PEO contenant les particules et PMMA essentiellement pur est formée au-dessus de 30% de PEO. La présence des particules diminue fortement la cristallinité.

[CHIM:OTHE] Chemical Sciences/Other

Laponite

Polymères nanocomposites

PEO

PMMA

Rhéologie

Polyméthacrylate de méthyle

Oxyde de polyéthylène

Polyéthylène glycol