Reproductive biology and nectary structure of <i>Lythrum</i> in central Saskatchewan

Caswell, Wade Devin

26 August 2008

This project examined multiple aspects of the reproductive biology of the wetland invasive species, purple loosestrife (<i>Lythrum salicaria</i> L.), in central Saskatchewan. An examination of insect taxa visiting the three floral morphs of <i>Tristylous</i> L. <i>salicaria</i>, as well as a ranking of the pollination efficiency of individual insect species, an apparent first for L salicaria, was undertaken. Surface features of the floral nectary of L. <i>salicaria</i>, as well as floral nectar secretion dynamics, were also investigated. This project also re-visited some of the previous work done on this invasive species, including various floral organ morphometrics in relation to heterostyly, and aspects of the tristylous breeding system including self-fertilization, and fertilization potential of both illegitimate pollination and legitimate pollination.<p>The trimorphic nature of the sexual floral organs of L. <i>salicaria</i> were well defined in Saskatchewan. Significant differences in length (long-, intermediate- and short-style lengths) exist between all three floral morphs. Lengths of the staminal filaments (long, intermediate, and short) were also significantly different. Also the floral nectary in L. <i>salicaria</i> is located in a depression formed at the interface of the hypanthium and the gynoecium. Several stomata are located at regular intervals along the nectary surface, and may constitute the escape route for floral nectar. No morphological differences in nectary structure were apparent among the three floral morphs.<p>Nectar secretion dynamics of L. <i>salicaria</i> were examined between the three floral morphs throughout two summer days in 2006. Peak average nectar volumes and nectar sugar quantities were detected at 3:00 pm, and, interestingly, no significant differences were detected between floral morphs, in accordance with nectary morphology. The estimated secretion rates for L. <i>salicaria</i> ranged from 61 83 µg of nectar sugar per flower per hour.<p>Hand-pollination experiments carried out over the summers of 2006 and 2007 at three field sites in and around Saskatoon have verified the strong self-incompatibility in the breeding system of this tristylous species. Intramorph pollination, using illegitimate pollen, did not result in fertilisation, whereas legitimate hand-pollination experiments yielded multiple pollen tubes at the style base, without exception.<p><i>Lythrum salicaria</i> in central Saskatchewan was visited by several bee taxa including honeybees (<i>Apis mellifera</i> L.), bumblebees (Bombus spp.), leafcutter bees (Megachile spp.), and sweat bees (Lasioglossum spp.). A single visit by <i>Anthophora furcata</i> (Panzer) was also recorded in 2007. Generally, bee visits led to high levels of pollination success as determined by fluorescence microscopy of pollen tubes following single insect visits to previously-unvisited flowers. However, most visits by hoverflies (Syrphidae) were non-pollinating. Visits by Pieris rapae (L.), yellowjacket wasps (Vespidae) and some non-syrphid flies (Diptera) also yielded no pollen tubes at the style base.<p>A study of the ultrastructure and development of the floral nectary of the purple loosestrife cultivar Morden Gleam (<i>Lythrum virgatum</i> L. x L. alatum Pursh.) showed that starch build up in pre-secretory nectary tissues declined throughout secretion, and is virtually absent in post-secretory nectary tissues. The lack of a direct vascular supply to the floral nectary suggests that the starch breakdown products likely make up most of the floral nectar carbohydrates. Surface features of the floral nectary in Morden Gleam closely resembled those of L. salicaria, located in the valley formed between the hypanthium and gynoecium. Nectary stomata, occasionally in pairs, likely serve as outlets for nectar in this cultivar.

transmission electron microscopy

scanning electron microscopy

Lythrum salicaria

Morden Gleam

nectary ultrastructure

invasive species

insect pollination

pollination biology

nectar secretion

bumble bees

honey bees

leafcutter bees

Halictidae

light microscopy

Syrphidae

fluorescence microscopy

Comparative Neurotoxicity of Methylmercury and Mercuric Chloride In Vivo and In Vitro

Thuett, Kerry A.

2009 August 1900

It is impossible to remove methylmercury (MeHg) from biological systems because MeHg is found throughout our environment in many fresh and salt water fish. The consumption of fish is important to human nutrition and health. The mechanism of MeHg neurotoxicity must be understood to minimize adverse exposure consequences. The dissertation objective was to: 1) compare mechanisms of MeHg neurotoxicity between animals exposed as adults and those exposed during gestation, and 2) develop an in vitro test model of in vivo MeHg exposure. Total mercury (Hg) levels in tissue / cells were determined by combustion / trapping / atomic absorption. Cell death was determined by Fluoro-Jade histochemical staining and activated caspase 3 immunohistochemistry for in vivo studies, and Trypan blue exclusion, lactate dehydrogenase activity, and cytotoxicity assays for in vitro studies. Mitochondrial membrane potential (MMP), intracellular calcium ion concentration ([Ca2+]i), and production of reactive oxygen species (ROS) were determined using fluorescence microscopy or microplate reader assays. Young adult C57Bl/6 mice were exposed to a total dose of 0, 1.0, or 5.0 mg/kg body weight MeHg divided over postnatal days (P)35 to 39. Pregnant female mice were exposed to a total does of 0, 0.1, or 1.0 mg/kg body weight MeHg divided over gestational days (G)8 to 18. SY5Y cells were exposed to 0, 0.01, 0.1, or 1.0 ?M MeHg or HgCl2 for 24, 48, or 72 hours. Total Hg in brains of young adult mice, mouse pups, and SY5Y cells accumulated in a dose-dependent manner. Cell death increased in SY5Y cells exposed to the highest concentrations of MeHg and HgCl2 used in this study. Cell death increased in the molecular and granule cerebellar cell layers of young adult mice exposed to the highest doses of MeHg used in this study. P0 mouse pups showed no increase in cell death within the cerebellum following MeHg exposure. Cerebella of mice at P10 exhibited decreased dying cells only in the external germinal layer. Low concentrations of MeHg affected MMP in both in vivo and in vitro studies, but did not result in decreased MMP typically associated with higher MeHg concentrations. [Ca2+]i was increased throughout the in vivo experiments in an age- , sexand brain region-dependent manner. Generation of ROS was decreased in both in vivo and in vitro studies with both the MeHg and HgCl2 (in vitro) treatments. In summary, low and moderate MeHg exposure, both in vivo and in vitro, altered mitochondrial function, Ca2+ homeostasis, and ROS differently than what is reported in the literature for higher MeHg exposure concentrations. SY5Y cells were sensitive to low-levels of MeHg and HgCl2 and responded similarly to cells in the whole animal studies, thus making SY5Y cells realistic candidates for mechanistic MeHg studies. Cell culture and whole animal neuronal functional studies at chronic low-level MeHg exposure are limited. These data suggest that low-levels of MeHg may affect neuronal function. Therefore, further chronic low-level MeHg neuronal functional studies are warranted.

methylmercury

mercury

mercuric chloride

development

SY5Y

rodent

cell culture

mitochondrial membrane potential

intracellular calcium ion concentration

reactive oxygen species

cell death

apoptosis

Fluoro-Jade

caspase 3

immunohistochemistry

fluorescence microscopy

Interaction of the human N-Ras protein with lipid raft model membranes of varying degrees of complexity

Vogel, Alexander, Nikolaus, Jörg, Weise, Katrin, Triola, Gemma, Waldmann, Herbert, Winter, Roland, Herrmann, Andreas, Huster, Daniel

07 December 2015

Ternary lipid mixtures composed of cholesterol, saturated (frequently with sphingosine backbone), and unsaturated phospholipids show stable phase separation and are often used as model systems of lipid rafts. Yet, their ability to reproduce raft properties and function is still debated. We investigated the properties and functional aspects of three lipid raft model systems of varying degrees of biological relevance – PSM/POPC/Chol, DPPC/POPC/Chol, and DPPC/DOPC/Chol – using 2H solidstate nuclear magnetic resonance (NMR) spectroscopy, fluorescence microscopy, and atomic force microscopy. While some minor differences were observed, the general behavior and properties of all three model mixtures were similar to previously investigated influenza envelope lipid membranes, which closely mimic the lipid composition of biological membranes. For the investigation of the functional aspects, we employed the human N-Ras protein, which is posttranslationally modified by two lipid modifications that anchor the protein to the membrane. It was previously shown that N-Ras preferentially resides in liquid-disordered domains and exhibits a time-dependent accumulation in the domain boundaries of influenza envelope lipid membranes. For all three model mixtures, we observed the same membrane partitioning behavior for N-Ras. Therefore, we conclude that even relatively simple models of raft membranes are able to reproduce many of their specific properties and functions.

Kernresonanz-Spektroskopie (NMR)

Atomkraftmikroskopie (AFM)

Membranprotein

Ordnungsparameter

atomic force microscopy (AFM)

membrane protein

order parameter

ddc:570

Probing vesicle dynamics within small synapses / Untersuchung der Vesikelbewegung in kleinen Synapsen

Lemke, Edward A.

27 April 2005

No description available.

540 Chemie

Mathematics and Computer Science

Fluoreszenz Mikroskopie

Positionsbestimmung

Fluoreszenz Spektroskopie

einzelne Vesikel

Synapsen

fluorescence microscopy

fluorescence spectroscopy

particle tracking

single vesicles

synapses

35.22

33.07

35.06

35.70

44.33

SD 000: Physikalische Chemie

Molecular dynamics of clathrin proteins at endocytic sites studied with evanescent-wave microscopy / Untersuchung der molekularen Dynamik von Clathrin mit Totalreflektionsmikroskopie

Loerke, Dinah

12 February 2004

No description available.

530 Physik

Mathematics and Computer Science

Clathrin

light chain

heavy chain

FRAP

Photobleichen

Austausch

Totalreflektion

Fluoreszenz

Mikroskopie

clathrin

light chain

heavy chain

FRAP

photobleaching

exchange

evanescent

fluorescence microscopy

33.05

42.03

42.12

RPV 720: Mikroskopie {Physik}

WC 000: Biophysik

Einfluss des Zellkortex auf die Plasmamembran: Modulation von Mikrodomänen in Modellmembranen / Influence of the Cell Cortex on the Plasma Membrane: Modulation of Microdomains in Model Membranes

Orth, Alexander

10 April 2012

Die Struktur der Plasmamembran ist von deren Lipid- und Proteinzusammensetzung abhängig und wird durch die Anbindung an das unterliegende Zytoskelett beeinflusst. Das Ziel der vorliegenden Arbeit war die Untersuchung eines neuen Modellsystems basierend auf po­ren­über­span­nen­den Membranen, welches sowohl die heterogene Lipidzusammensetzung als auch den Einfluss eines unterliegenden Netzwerks berücksichtigt. Lipidmembranen, zusammengesetzt aus der „raft“-ähnlichen Lipidmischung DOPC/Sphingo­myelin/Cho­les­terin (40:40:20), wurden auf porösen, hochgeordneten Siliziumsubstraten mit Po­ren­durch­messern von 0.8, 1.2 und 2.0 µm durch Spreiten und Fusion von Riesenvesikeln (giant unilamellar vesicles, GUVs) präpariert. Die mikroskopische Phasenseparation in koexistierenden flüssig-geordneten (liquid ordered, lo) und flüssig-ungeordneten (liquid disordered, ld) Domänen wurde stark durch das unterliegende poröse Substrat beeinflusst. Die Größe der lo-Domänen konnte durch die Porengröße des Siliziumsubstrats, die Temperatur und den Cholesteringehalt der Membran, welcher durch Zugabe von Methyl-β-Cyclodextrin moduliert wurde, kontrolliert werden. Die Bindung der Shiga Toxin B-Untereinheit (STxB) an po­ren­überspannende Membranen, dotiert mit 5 mol% des Rezeptorlipids Gb3, führte zu einem Anstieg des Anteils der lo-Phase. Außerdem wurde die Bildung von lo-Domänen in nicht-phasenseparierten Membranen, zusammengesetzt aus DOPC/Sphingomyelin/Cholesterin/Gb3 (65:10:20:5), durch die Shiga Toxin-Bindung induziert. Ein Anstieg des Anteils der lo-Phase konnte ebenfalls bei der Bindung der pentameren Cholera Toxin B-Untereinheit (CTxB) an po­ren­überspannende Membranen, dotiert mit 1 mol% des Rezeptorlipids GM1, beobachtet werden. Des Weiteren wurde der Einfluss der chemischen Struktur des Gb3-Moleküls auf die Shiga Toxin-Bindung und die Reorganisation von festkörperunterstützten Membranen (solid supported membranes, SSMs) untersucht. Die STxB-Bindung an α-hydroxyliertes Gb3 erhöhte signifikant den Anteil der lo-Phase, während eine cis-Doppelbindung zur Bildung einer weiteren lo-Phase führte, die vermutlich ungesättigte (Glyko-)Sphingolipide und Cholesterin enthält. Im Falles des ungesättigten Gb3 konnte außerdem eine Kondensation zu größeren Domänen nach der STxB-Bindung beobachtet werden. Die genaue Phasenzuordnung der eingesetzten Glykospingolipide vor der Proteinbindung ist bisher unbekannt. Daher wurde das Phasenverhalten eines fluoreszierenden Polyen-Ga­lac­to­ce­re­bro­sids untersucht, welches bevorzugt in der lo-Phase von GUVs angereichert war. Dieser neue, intrinsische Fluorophor vermag als Grundlage für weitere Studien zum Phasenverhalten von Glykosphingolipiden dienen.

540

Porenüberspannende Membranen

Lipiddomänen

Phasenseparation

Glykolipide

Shiga Toxin

STxB

Cholera Toxin

CTxB

Fluoreszenzmikroskopie

Rasterkraftmikroskopie

AFM

pore-spanning membranes

lipid domains

phase separation

glycolipids

Shiga Toxin

STxB

Cholera Toxin

CTxB

fluorescence microscopy

atomic force microscopy

AFM

Chemie  (PPN62138352X)

Étude du réseau d'interactions entre les protéines du Virus de l'Hépatite C

Racine, Marie-Eve

January 2007

Mémoire numérisé par la Division de la gestion de documents et des archives de l'Université de Montréal

VHC

HCV

Interactions protéine-protéine

Protein-protein interactions

NS3/4A

NS3/4A

NS4B

NS4B

NS5A

NS5A

BRET

BRET

Microscopie de fluorescence

Fluorescence microscopy

Localisation subcellulaire

Subcellular localization

Co-immunoprécipitation

Co-immunoprecipitation

Mutagénèse

Mutagenesis

Emprego de microscopia de fluorescência para a quantificação microbiana em amostras salinas da indústria do petróleo / Use of fluorescence microscopy for microbial quantification in the saline samples of the petroleum industry

Denise da Piedade Silva

09 December 2010

Os micro-organismos constituem um grande problema em termos econômicos para a indústria petrolífera. Estes são responsáveis pela produção de substâncias corrosivas e a formação de biofilmes, que causam deterioração dos materiais metálicos. Os principais grupos microbianos presentes em amostras ambientais da indústria do petróleo são as bactérias anaeróbias heterotróficas totais (BANHT) e as bactérias redutoras de sulfato (BRS). Atualmente, a quantificação desses grupos microbianos é realizada através da técnica do Número Mais Provável (NMP) que estima o resultado em aproximadamente 28 dias. Neste trabalho foi otimizada uma metodologia para a microscopia de fluorescência de amostras salinas provenientes de tanques de armazenamento de água/óleo. As condições testadas foram o tipo de óleo de imersão, o tipo de diluente, o volume do corante, o volume da amostra corada e a concentração do fixador (glutaraldeído) numa tentativa de correlacionar com resultados de quantificação de BANHT e BRS através da técnica convencional do NMP. Nesse caso, as células totais foram quantificadas por microscopia de fluorescência utilizando o corante fluorescente laranja de acridina (AO). Verificou-se que houve uma correlação entre os resultados da quantificação de células totais por microscopia de fluorescência e os resultados de BANHT pela técnica do NMP, devido a pouca variação de valores expressos em ambas as quantificações. Entretanto, não foi possível correlacionar os resultados da quantificação de células totais com os resultados de BRS por NMP devido à grande variação dos valores de quantificação de BRS. Na microscopia de fluorescência, foi possível, quantificar os micro-organismos em aproximadamente 30 minutos e através das fotografias, verificou-se ainda que as amostras apresentaram-se nítidas e os micro-organismos com uma boa fluorescência / Microbial cells constitute a severe problem, from the economic point of view, for the petroleum industry. They are responsible for the production of corrosive metabolites and for the formation of biofilms, causing deterioration in the surface of metallic materials. The main microbial groups present in environmental samples from the petroleum industry include total anaerobic heterothrophic bacteria (TANHB) and sulfate-reducing bacteria (SRB). Nowadays, the quantification of those microbial groups is performed through the use of the most probable number technique (MPN), providing the final quantification after 28 days. In the present work a new methodology, based on fluorescence microscopy, was optimized on saline samples from water/oil storage tanks. The conditions tested were the type of immersion oil, type of diluent, the volume of the dye, the stained sample volume and concentration of fixative (glutaraldehyde) in order to quantify total cells, in an attempt to correlate with TANHB and SRB quantification through MPN. In that case, total cells were quantified with the help of acrydine orange as fluorescent dye. It could be observed a clear correlation between the results obtained for total cells quantification by fluorescence microscopy and the results obtained for TANHB through MPN technique, due to the negligible differences observed in both quantifications. However, when a correlation with SRB cells was tried results of total cells through fluorescence microscopy did not fit entirely. With the use of fluorescence microscopy, it was possible to quantify microbial cells in around 30 minutes and with the help of photographic reports obtained, it could be observed that the samples were clearly observed and the microbial cells indicated a good fluorescence

Laranja de acridina

Número Mais Provável

Bactérias redutoras de sulfato

Micro-organismos totais

Quantificação microbiana

Microscopia de fluorescência

Acrydine orange

Most probable number

Sulfate-reducing cells

Total microorganisms

Microbial quantification

Fluorescence microscopy

TECNOLOGIA QUIMICA

Avaliação in vitro da viabilidade de Enterococcus faecalis e Candida albicans nos túbulos dentinários após a aplicação de hidróxido de cálcio e clorexidina gel 2% / In vitro evauluation of the viability of Enterococcus faecalis and Candida albicans in dentinal tubules after placement of calcium hydroxide and chlorhexidine gel 2%

Ronan Jacques Rezende Delgado

12 June 2007

Uma infecção pulpar pode resultar na colonização microbiana de todo sistema de canais radiculares incluindo os túbulos dentinários. Estes microorganismos e seus produtos tóxicos são responsáveis pelo desenvolvimento e persistência da periodontite apical de origem endodôntica. O presente estudo objetivou avaliar a viabilidade de E. faecalis e C. albicans em túbulos dentinários após a aplicação de hidróxido de cálcio, clorexidina gel 2%, hidróxido de cálcio associado à clorexidina gel 2% e soro fisiológico, através da análise por cultura microbiológica e microscopia de fluorescência. Para tanto 120 raízes de dentes humanos foram padronizadas e autoclavadas, sendo posteriormente divididas em 2 grupos (n= 60) para contaminação com E. faecalis e C. albicans por 21 dias. Em seguida, foram divididas em 8 grupos (n= 15) para aplicação das substâncias antimicrobianas nos canais radiculares e posterior incubação em estufa por 14 dias. Amostras da dentina radicular na extensão de 0 - 100 µm e de 100 - 200 µm foram coletadas e submetidas à cultura microbiológica através do plaqueamento em meios de cultura. Após 48 horas de incubação promoveu-se a avaliação das UFC. Paralelamente, as amostras foram processadas para análise em microscopia de fluorescência com auxílio de marcadores fluorescentes específicos, a fim de se determinar a proporção de microorganismos viáveis e não viáveis. Outros 6 espécimes foram preparados para análise em MEV. Os resultados mostraram uma maior capacidade de penetração intratubular para E. faecalis quando comparado a C. albicans. A aplicação de medicação intracanal resultou em significativa redução da viabilidade dos microorganismos quando comparado ao grupo controle independente da medicação aplicada e em ambas as porções da dentina radicular avaliadas. Entretanto, ao compararmos individualmente as medicações, observamos o melhor desempenho da clorexidina gel 2 % e da associação de hidróxido de cálcio e clorexidina gel 2% sem diferença significante entre elas. O hidróxido de cálcio apresentou os piores resultados para desinfecção dos canais radiculares contaminados com E. faecalis e C. albicans. Estes achados foram confirmados tanto pela cultura microbiológica quanto pela microscopia de fluorescência. A cultura microbiológica e a microscopia de fluorescência são métodos adequados e complementares para avaliação da viabilidade de E. faecalis e C. albicans e a eficácia da clorexidina gel 2% e da associação hidróxido de cálcio e clorexidina gel 2% justificam seu uso em endodontia como medicação intracanal. / A pulp infection can result in a microbial colonization of the entire root canals system, including dentinal tubules. These microorganisms and their toxic product are responsible for the development and persistence of apical periondontitis from endodontic source. The present study aimed to evaluate E. faecalis and C. albicans viability in dentinal tubules after the application of calcium hydroxide, chlorhexidine gel 2%, calcium hydroxide associated to chlorhexidine gel 2% and physiological solution, through the analysis by microbiological culture and fluorescence microscopy. For that, 120 human teeth root were standardized and submitted to autoclave, and after ere divided into 2 groups (n=60) for E. faecalis and C. albicans contamination for 21 days. Following this, they were divided into 8 groups (n=15) for application of antimicrobial substances in the root canals and subsequent incubation for 14 days. Samples from root dentin with 0 - 100 µm and 100 - 200 µm of extension were collected and submitted to microbiological culture.After 48 hours of incubation, it was performed the evaluation of colony-forming units (CFU). At the same time, the samples were processed for fluorescence microscopic analysis with the assistance of specific fluorescent markers, in order to determine the proportion of viable and non-viable microorganisms. Other 6 specimens were prepared for the analysis of scanning electron microscopy. Results demonstrated a higher capacity of penetration in the tubules for E. faecalis than for C. albicans. The application of intracanal medication resulted in significant reduction of microorganisms viability when compared to the control groups independently of the medication used and in both evaluated portions of root dentin. However, when one compares individually the medications, it was observed a better performance of chlorhexidine gel 2% and the association of calcium hydroxide with chlorhexidine gel 2% without a significant difference between them. Calcium hydroxide had the worst results for disinfection of root canal contaminated with E. faecalis and C. albicans. These findings were confirmed for the microbiological culture as well as for the fluorescence microscopy. The microbiological culture and the fluorescence microscopy are adequate methods and complementary for the evaluation of E. faecalis and C. albicans viability and the efficacy of chlorhexidine gel 2% and the association of calcium hydroxide with chlorhexidine gel 2% warrant their use in Endodontics as an intracanal medication.

Candida albicans

Clorexidina

Endodontia

Enterococcus faecalis

Hidróxido de cálcio

Infecção do canal radicular

Microscopia de fluorescência

Viabilidade microbiana

Calcium hydroxide

Candida albicans

Chlorhexidine

Endodontics

Enterococcus faecalis

Fluorescence microscopy

Microbial viability

Root canal infection

Estudo, via simulação molecular, da interação de dois peptídeos da região 115-129 da miotoxina II do veneno da serpente Bothrops asper com membranas celulares. / Estudo, via simulação molecular, da interaão de dois peptídeos da região 115-129 da miotoxina II do veneno da serpente Bothrops asper com membranas celulares

Marcos Roberto Lourenzoni

13 June 2005

As ligações de hidrogênio (LH), fundamentais na determinação da estrutura da água, proteínas, etc., são muito importantes no reconhecimento molecular e nos mecanismos de reações enzimáticas. A determinação da energia das LHs intramoleculares em proteínas e intermoleculares entre uma proteína e o solvente água, porque fornece informações sobre a estrutura secundária, terciária e quaternária das proteínas. Um método para quantificar e qualificar as LHs foi desenvolvido utilizando critérios de distância, geométricos e energéticos a partir das trajetórias obtidas por simulações de dinâmica molecular. O método foi testado com o monômero de uma fosfolipase A2 homodimérica, sem atividade catalítica, isolada do veneno da Bothrops asper(BaspMT-II). No dímero, a análise das LHs mostrou que elas são também essenciais na manutenção da estrutura quaternária. Essa análise permitiu identificar movimentos do tipo dobradiça acompanhados da formação transitória, na interface dimérica, de LHs controladas pelo triptofano na posição 77. Esses movimentos podem estar associados à ação danosa às membranas, uma vez que podem promover a inserção da região C-terminal na membrana. Estudos prévios mostraram que o peptídeo sintético (3Y codificado pelos aminoácidos 115-129 da BaspMT-II) apresenta atividade bactericida e citolítica. Um outro peptídeo (3W), mutante de 3Y, no qual três resíduos tirosina são substituidos por triptofano, apresenta um aumento do dano às membranas e do efeito miotóxico. Os mecanismos de ação desses peptídeos e as suas estruturas foram estudados por dinâmica molecular, dicroísmo circular (DC), microscopia de fluorescência e monocamadas de Langmuir (Mlang). As adsorções dos peptídeos em monocamadas de ácido dimiristoil fosfatídico (DMPA) e dimiristoilfosfatidilcolina (DMPC) se processam por mecanismos diferentes ocasionados pelas diferentes naturezas físico-químicas dos resíduos tirosina e triptofano. A microscopia de fluorescência acoplada a Mlang de DMPA com 3W adsorvido mostra um aumento da fluidez da monocamada, enquanto que o 3Y modifica os domínios do DMPA para pequenas estruturas circulares. Foram realizadas simulações dos peptídeos 3Y e 3W em meio aquoso e nas regiões interfaciais água/n-hexano e água/bicamadas de DMPC. Os resultados confirmam os obtidos por Mlang, demonstrando que os peptídeos interagem diferentemente com as membranas por adotar conformações alternativas definidas previamente. Essas conformações, diferentes das observadas em meio aquoso, dependem da natureza da interface. As estruturas encontradas no final das simulaçoes corroboram o mecanismo proposto por Mlang, assim como as estruturas sugeridas por DC. Isso sugere que a atividade biológica reduzida do peptídeo 3Y ocorre porque os seus dois resíduos Leu se adsorvem na interface sem penetrá-la. Ao contrário de 3W, os resíduos carregados do peptídeo 3Y não estão localizados corretamente para promover uma interação suficientemente atrativa para permitir a sua inserção na membrana celular. / Hydrogen bonds (HB) are highly important in the determination of the structure of the water and proteins. They also play a important role in molecular recognition and in enzyme reaction mechanisms. The determination of protein/water intermolecular and protein intramolecular HB energies provide information with respect to the formation and stabilization of secondary, tertiary and quaternary protein structure. A method that quantifies and qualifies the properties of HB was developed using distance, geometric and energy criteria as applied to data obtained from the atomic trajectories generated by molecular dynamics simulations. The method was tested with a monomer of a catalytically inactive homodimeric phospholipase A2 from Bothrops asper(BaspMT-II) venom. HBs at dimmer interface are essential for maintaining the quaternary structure, and are highly conserved during hinge-like movements of the dimmer. HB formed by tryptophan residue at position 77 controls this movement. These motions can be associated to the membrane damaging action since they facilitate the insertion of the C-terminus into the cellular membrane. Previous studies have shown that synthetic peptide (3Y, coding the amino acids 115-129 of BaspMT-II ) presents bactericidal and cytolitic activities. A peptide variant ( 3W ), in which tyrosine residues were substituted by tryptophan residues, presents an enhanced membrane damaging activity increased miotoxic effect. The mechanism of action of the peptides and their structures were studied by molecular dynamics simulations, circular dichroism (CD), fluorescence microscopy and Langmuir monolayers (Mlang). The adsorption of the peptides on a monolayer composed of dimiristoyl phosphatidic acid (DMPA) and dimiristoylphosphatidyl choline (DMPC) occurs through different processes due to the differences in the physic-chemical nature of the tyrosine and tryptophan residues. Fluorescence microscopy together with Mlang of DMPA with adsorbed 3W indicates an increase of the membrane fluidity while small circular domains are formed with DMPA. Simulations were conducted with the 3Y and 3W peptides in aqueous media, is a water/n-hexane and water/DMPC bilayers. The results confirm the Mlang results, showing that the peptides interact differently with the membranes by adopting alternative previously defined conformations. These two conformations, both of which are different to those observed in water, are dependent of the nature of the interfaces. The final simulated configurations confirm the mechanism proposed by Mlang and the structures proposed by CD. It is suggest that the reduced biological activity of the 3Y peptide is due to the two Leu residues that only adsorb to the cellular membrane without penetrating the bilayer. In contrast to the 3W peptide, no charged residue is correctly located to promote the interaction and insertion of the 3Y peptide into the membrane.

dicroísmo circular

Dinâmica Molecular

estrutura de proteínas

fosfolipase A2

ligações de hidrogênio

microscopia de fluorescência

circular dichroism

fluorescence microscopy

Hydrogen bonds

Molecular Dynamic

phospholipase A2

protein structure