Directed Evolution of Glutathione Transferases Guided by Multivariate Data Analysis

Kurtovic, Sanela

January 2008

<p>Evolution of enzymes with novel functional properties has gained much attention in recent years. Naturally evolved enzymes are adapted to work in living cells under physiological conditions, circumstances that are not always available for industrial processes calling for novel and better catalysts. Furthermore, altering enzyme function also affords insight into how enzymes work and how natural evolution operates. </p><p>Previous investigations have explored catalytic properties in the directed evolution of mutant libraries with high sequence variation. Before this study was initiated, functional analysis of mutant libraries was, to a large extent, restricted to uni- or bivariate methods. Consequently, there was a need to apply multivariate data analysis (MVA) techniques in this context. Directed evolution was approached by DNA shuffling of glutathione transferases (GSTs) in this thesis. GSTs are multifarious enzymes that have detoxication of both exo- and endogenous compounds as their primary function. They catalyze the nucleophilic attack by the tripeptide glutathione on many different electrophilic substrates. </p><p>Several multivariate analysis tools, <i>e.g.</i> principal component (PC), hierarchical cluster, and K-means cluster analyses, were applied to large mutant libraries assayed with a battery of GST substrates. By this approach, evolvable units (quasi-species) fit for further evolution were identified. It was clear that different substrates undergoing different kinds of chemical transformation can group together in a multi-dimensional substrate-activity space, thus being responsible for a certain quasi-species cluster. Furthermore, the importance of the chemical environment, or substrate matrix, in enzyme evolution was recognized. Diverging substrate selectivity profiles among homologous enzymes acting on substrates performing the same kind of chemistry were identified by MVA. Important structure-function activity relationships with the prodrug azathioprine were elucidated by segment analysis of a shuffled GST mutant library. Together, these results illustrate important methods applied to molecular enzyme evolution.</p>

Biochemistry

DNA shuffling

substrate selectivity

mutant library

glutathione transferase

multivariate data analysis

prodrug

Biokemi

Influence des phénomènes d'oxydation lors de l'élaboration des moûts sur la qualité aromatique des vins de Melon B. et de Sauvignon Blanc en Val de Loire / Influence of oxidation mechanisms during musts elaboration on the aromatic quality of Melon B. and Sauvignon Blanc wines from Loire Valley

Roland, Aurélie

04 November 2010

Afin de caractériser les moûts de Melon B. et de Sauvignon Blanc en composition et de modéliser leur profil d'oxydation, diverses méthodologies analytiques quantitatives ont été développées et validées. La quantification par dilution isotopique des précurseurs de thiols a nécessité la synthèse de molécules marquées qui ont également servies de traceurs lors d'études de filiation dans des milieux complexes. Ainsi, au cours de la fermentation alcoolique, nous avons pu démontrer que le S-3-(hexan-1-ol)-glutathion (G3MH) et la S-4-(4-méthylpentan-2-one)-glutathion (G4MMP) sont métabolisés par la levure et libèrent le 3-mercaptohexan-1-ol (3MH) et la 4-méthyl-4-mercaptopentan-2-one (4MMP) avec des rendements de conversion molaires proches de 4,4 % et 0,3 % respectivement. La modélisation des phénomènes d'oxydation à l'échelle laboratoire a permis par ailleurs de vérifier, comme le laissaient supposer leurs structures chimiques, que les précurseurs de thiols ne sont pas dégradés par les mécanismes oxydatifs affectant les moûts. Au contraire, une formation de G3MH concomitante avec le pic de production du Grape Reaction Product (GRP) est observée. La validation de ces observations à l'échelle industrielle a été conduite par comparaison des pressurages traditionnel et inerté. L' élaboration d'un moût de Melon B. sous gaz inerte n'est pas favorable à la production de G3MH d'origine pré-fermentaire, et a pour conséquence une diminution des teneurs en 3MH dans les vins correspondants, sans pour autant, déprécier les qualités organoleptiques des vins jeunes. Pour le Sauvignon Blanc, le potentiel aromatique de type thiol n'est pas affecté par le type de pressurage, mais une diminution très significative en 3MH dans les vins issus des cuvées obtenues sous gaz inerte est observée. La voie du (E)-2-hexènal qui est certainement impliquée, pourrait expliquer cette perte aromatique. Ainsi, de manière globale, dans nos conditions expérimentales, une oxydation ménagée et raisonnée des moûts de Melon B., et dans une moindre mesure de Sauvignon Blanc, est favorable à la qualité aromatique des vins du Val de Loire. / In order to characterize Melon B. and Sauvignon Blanc musts in composition and to study their oxidation profiles, several analytical methodologies have been developed and validated. The quantification of thiols precursors by Stable Isotope Dilution Assay required the synthesis of labeled molecules, which have been used either as analytical standards or as tracers for relationship studies in complex matrices. Thus, we established that, during the alcoholic fermentation, the S-3-(hexan-1-ol)-glutathione (G3MH) and the S-4-(4-méthylpentan-2-one)-glutathione (G4MMP) are metabolized by the yeast to release the 3-mercaptohexan-1-ol (3MH) and the 4-méthyl-4-mercaptopentan-2-one (4MMP) with molar conversion yields close to 4.4 % and 0.3 % respectively. Oxidation mechanisms study at laboratory scale demonstrated that aromatic potential was not affected by oxidative reactions, as expected in regard to their chemical structures. On the contrary, the G3M H was produced in the same time as the Grape Reaction Product peak (GRP). The validation of these observations at industrial scale was conducted by comparing traditional and inerted pressing systems. The elaboration of a Melon B. must under inert gas was not in favor of a G3MH pre-fermentary production, which induced a decrease of 3MH concentration in wine without affecting the organoleptic qualities of young wines. For Sauvignon Blanc must, the aromatic potential was not affected by the kind of pressing systems but a significant decrease in 3MH was observed in the wines obtained with juices from the beginning of pressing. The E-(2)-hexenal pathway could certainly explain such aromatic losses. Thus, under our experimental conditions, a mild and controlled oxidation of Melon B. must and, in a certain extend of Sauvignon Blanc must, is in favor of the aromatic quality of wines from Loire Valley.

Oxydation

Glutathion

Thiols variétaux

Potentiel aromatique

Oxidation

Glutathione

Varietal thiols

Aromatic potential

Studies on Human and Drosophila melanogaster Glutathione Transferases of Biomedical and Biotechnological Interest

Mazari, Aslam M.A.

January 2016

Glutathione transferases (GSTs, EC.2.5.1.18) are multifunctional enzymes that are universally distributed in all cellular life forms. They play important roles in metabolism and detoxication of endogenously produced toxic compounds and xenobiotics. GSTs have gained considerable interest over the years for biomedical and biotechnological applications due to their involvement in the conjugation of glutathione (GSH) to a vast array of chemical species. Additionally, the emergence of non-detoxifying functions of GSTs has further increased their biological significance. The present work encompasses four scientific studies aimed at investigating human as well as fruit fly Drosophila melanogaster GSTs. Paper I presents the immobilization of GSTs on nanoporous alumina membranes. Kinetic analyses with 1-chloro-2,4-dinitrobenzene followed by specificity screening with alternative substrates showed a good correlation between the data obtained from immobilized enzymes and the enzymes in solution. Furthermore, immobilization showed no adverse effects on the stability of the enzymes. Paper II presents inhibition studies of human hematopoietic prostaglandin D2 synthase (HPGDS), a promising therapeutic target for anti-allergic and anti-inflammatory drugs. Our screening results with an FDA-approved drug library revealed a number of effective inhibitors of HPGDS with IC50 values in the low micromolar range. Paper III concerns the toxicity of organic isothiocyanates (ITCs) that showed high catalytic activities with GSTE7 in vitro. The in vivo results showed that phenethyl isothiocyanate (PEITC) and allyl isothiocyanate in millimolar dietary concentrations conferred toxicity to the adult fruit flies leading to death or shortened life-span. The transgenic female flies overexpressing GSTE7 showed increased tolerance against PEITC toxicity compared to the wild-type. However, the effect was opposite in male flies overexpressing GSTE7 after one week exposure. Notably, the transgene enhanced the oviposition activity of flies with and without ITCs exposure. Paper IV highlights Drosophila GSTs as efficient catalysts of the environmental pollutant and explosive 2,4,6-trinitrotoluene and the related 2,4-dinitrotoluene degradation. This result suggests the potential of GST transgenes in plants for biotransformation and phytoremediation of these persistent environmental pollutants.

glutathione transferases

detoxication

hpgds inhibition

immobilization

isothiocyanates

drosophila GSTs

environmental pollutants

Metabolomics Investigation of Glyceollins by On-Line Liquid Chromatography-Electrospray Ionization Tandem Mass Spectrometry and Fungal Metabolite Identification by Thermal Desorption Analysis Coupled with Gas Chromatography-Mass Spectrometry

Quadri, Syeda

08 August 2013

Metabolomics is an emerging field that entails the detailed characterization of the ensemble of metabolites produced by living organisms; subfields include drug metabolism and natural environmental toxin production. The first part of the dissertation pursued metabolism of glyceollins, i.e., isoflavones produced by soybeans, that are potential cancer therapy agents. In vivo glyceollin metabolites produced in rats were investigated by on-line Liquid Chromatography-Electrospray Ionization Tandem Mass Spectrometry. An odd-electron fragment ion at m/z 148, formed in violation of the even-electron rule, and diagnostic of the glyceollin backbone, was discovered. Based on this finding, a negative mode precursor ion scanning method was developed to screen for glyceollins and their metabolites from biological samples. Products of both Phase I and Phase II metabolism were identified, none of which have been previously reported. Sulfated metabolites were confirmed by accurate mass measurement, while glucuronide conjugation was confirmed by enzyme-assisted glucuronidation by rat liver microsomes. Intact GSH-glyceollin conjugates were not observed, but breakdown products of the GSH pathway, i.e., cysteinylglyceine, cysteine, and acetylated cysteine, were identified as conjugates of oxygenated glyceollins. The identification of GSH by-product conjugates was confirmed in product ion spectra acquired in the negative mode (where peptide anions, and glyceollin-bearing cleaved peptide portions were observed), as well as in the positive mode (where intact oxygenated glyceollin fragments appeared without the initially-present peptide portion). Mass spectral evidence strongly supports a metabolic pathway involving initial epoxidation of glyceollins followed by GSH addition at the epoxidation site. The second part of the dissertation undertook the investigation of secondary metabolites called microbial volatile organic compounds (MVOCs) produced by fungi (mold) that have been reported to have adverse human health effects. MVOCs were collected onto different sorbent materials and analyzed by Thermal Desorption Analysis coupled with on-line Gas Chromatography-Mass Spectrometry. Fungal MVOCs were characterized from various simulated flooding conditions (brackish, freshwater, and saltwater) and different substrates (nutrient rich vs. low nutrient) to determine diagnostic MVOCs. Ten fungi from simulated environments were identified by genetic sequencing. Cladosporium sp. and Chaetomium sp. were cultivated and their emitted MVOCs, 3-furaldehyde and 3-(4-hydroxy-3-methoxyphenyl)-2-propenal, were proposed as diagnostic indicators of these fungi.

Medicine and Health Sciences

Exploring Catalytic Tellurium-Based Antioxidants : Synthesis and Evaluation

Poon, Jia-fei

January 2016

This thesis is concerned with the synthesis and evaluation of various tellurium-based chain-breaking antioxidants. The purpose is to find novel regenerable compounds with improved radical-trapping capacity. In the first part of this work, we explore the possibilities to incorporate tellurium into tocopherols and aromatic amines. Overall, tocopherols carrying alkyltelluro groups are better radical-trapping agents than the corresponding sulfur- and selenium analogues. Among them, 7-octyltelluro δ-tocopherol showed a ca. 17-fold higher reactivity than recorded for α-tocopherol and much better regenerability. Even longer inhibition times were recorded for the corresponding bis(tocopheryl) tellurides. In the aromatic amine series, diphenyl amines carrying alkyltelluro groups were shown to function as efficient radical-quenchers capable of inhibiting peroxidation for 460 min in the presence of N-acetylcysteine. Thiol-consumption experiments suggested that the long inhibition times are due to efficient quenching of in-situ formed alkoxyl radicals in a solvent cage. In the second part of the thesis, we study how the antioxidant properties are affected by variations in the electron density at tellurium and the number of alkyltelluro substituents in the molecule. Evaluation of a series of aryltelluro phenols carrying electron donating and electron withdrawing groups in the para-position of the aryl moiety suggested that a high electron density at the heteroatom prolonged the inhibition time. Among alkyltelluro phenols, alkyltelluro resorcinols and bis(alkyltelluro) phenols, phenols carrying alkyltelluro groups in both ortho positions were superior when it comes to radical-trapping activity and regenerability.

antioxidant

tellurium

selenium

radical-trapping

chain-breaking

ROS

glutathione peroxidase

tocopherol

aromatic amine

oxidative stress

Application of redox biosensor mouse models to study redox processes in cardiomyocytes

Nanadikar, Maithily

11 June 2019

No description available.

610

Reactive oxygen species

Glutathione redox potential

Cardiomyocytes

Redox biosensor

GOK-MEDIZIN

A mixed-charge cluster facilities glutathione transferase dimerisation

Walters, John Clive

14 November 2006

Student Number : 0213014A - MSc dissertation - School of Molecular and Cell Biology - Faculty of Science / Cytosolic glutathione transferases (GSTs) are obligate stable homo- and heterodimers comprising two GST subunits. Interactions across the subunit interface play an important role in stabilising the subunit tertiary structure and maintain the dimeric structure required for activity. The crystal structure of a rat Mu class GST consisting of two type one subunits (rGST M1-1) reveals a lock-and-key motif and a mixedcharge cluster at the subunit interface. Previous investigations revealed the lock-andkey motif was not essential for dimerisation. It was therefore postulated that the mixed-charge cluster at the dimer interface is primarily responsible for subunit association. Statistical analyses of individual rGST M1-1 chains did not predict the presence of any charge clusters. This suggests that the mixed-charge cluster forms only upon dimerisation and reinforces the probability that quaternary structure stabilisation is a major role of the mixed-charge cluster. Arginine 81 (Arg-81), a structurally conserved residue in the GST family involved in the mixed-charge cluster, was mutated to alanine. Phenylalanine 56 (Phe-56), the ‘key’ residue in the lock-and-key motif, was mutated to serine. These changes were engineered to disrupt the mixed-charge cluster and the lock-and-key motif situated at the dimer interface of rGST M1-1. Sizing by gel filtration chromatography of the mutant GST identified that these engineered amino acids resulted in a stable monomeric protein (F56S/R81A rGST M1). The F56S/R81A rGST M1 displayed almost no catalytic activity, suggesting perturbations of the active site or substrate binding sites. Structural investigations of the monomer by far- and near-UV circular dichroism revealed a similar secondary structural content to the wild-type. However, the tryptophan fluorescence properties suggested the tryptophans were situated in more hydrophilic environments than in the wild-type. ANS binding studies indicated a large increase in the accessible hydrophobic surface area of the monomer. Ureainduced equilibrium unfolding of F56S/R81A rGST M1 follows a cooperative twostate unfolding model. The unfolding data indicates decreased conformational stability and a large increase in the solvent exposed surface area of the monomer. In conclusion, the mixed-charge cluster at the dimer interface of rGST M1-1 is essential for monomeric association, which subsequently contributes to catalytic activity of the dimer and the stabilities of individual rGST M1-1 subunits.

oligomerisation

oligomeric assemblies

Cytosolic glutathione transferases

GST

charge clusters

filtration chromatography

Folding mechanism of Glutaredoxin 2

Gildenhuys, Samantha

19 May 2008

ABSTRACT Equilibrium unfolding, single- and double-jump kinetic studies were conducted to determine the unfolding and refolding pathway of glutaredoxin 2. Structural changes for wild-type glutaredoxin 2 were monitored by far-ultraviolet circular dichroism and intrinsic tryptophan fluorescence for equilibrium unfolding and intrinsic tryptophan fluorescence for single- and double-jump kinetics studies. Glutaredoxin 2 possesses two tryptophan residues in domain 2. In order to monitor changes in domain 1, cysteine 9 at the active site cysteines, situated in domain 1, was labelled with an extrinsic fluorophore, AEDANS, and a mutant was created (Y58W glutaredoxin 2). The AEDANS labelled protein displayed decreased alpha-helical secondary structure and conformational stability. A high degree of cooperativity and similar conformational stability was observed during the two-state transition of the urea-induced equilibrium unfolding of both the wild-type and Y58W glutaredoxin 2 proteins therefore Y58W glutaredoxin 2 could be used to assess structural changes in the local environment of domain 1 during unfolding and refolding. Two phases of unfolding, the fast and slow phase, occurred for both the wild-type and Y58W proteins. The slow phase involves structural rearrangements that expose small amounts of surface area while the fast phase represents gross structural unfolding exposing large amounts of surface area. The isomerization of the Val48-Pro49 peptide bond to the trans conformation occurs during the slow phase and this isomerization is coupled to conformational unfolding of the protein. The structural separation of these phases could be represented by two structural units (unit x and unit y), these units do not represent domain 1 and 2. The units could also result in parallel refolding pathways with the folding of the x unit involving the fast and slow refolding phases and the folding of the y unit of structure is represented by the medium phase of refolding. The fast and slow phases are further separated as the fast phase represents the gross structural folding of glutaredoxin 2 for species with the Val48-Pro49 peptide bond in the native cis conformation. The development of the slow phase after extended unfolding delay periods during double-jump refolding studies, as well as the acceleration of the rate of the phase by the peptidyl prolyl isomerase hFKBP-12 proved that the phase involves a proline peptide bond iv isomerization. This phase represents a slow isomerization coupled with conformational folding similar to the slow unfolding phase. Complex unfolding and refolding kinetics indicated the involvement of kinetic intermediates during (un)folding.

protein folding

Thioredoxin

Glutathione-S-transferases

Glutaredoxin 2

cis-trans Isomerization

Avaliação dos polimorfismos do Ácido Delta-aminolevulínico desidratase (ALAD) e Glutationa peroxidase (GPx) sobre estresse oxidativo em trabalhadores ocupacionalmente expostos ao chumbo / Evaluation of delta aminolevulinic acid (ALAD) and glutathione peroxidase (GPx) polymorphisms on oxidative stress in workers occupationally exposed to lead

Martins Júnior, Airton da Cunha

04 July 2014

O chumbo (Pb) é um metal altamente tóxico no qual os sinais de intoxicação variam bastante ao considerar as diferenças interindividuais. Um dos principais mecanismos de toxicidade do Pb ocorre pela inibição da enzima ácido delta aminolevulínico desidratase (ALAD) no sistema hematopoiético. O Pb também desempenha um importante papel no desbalanço do estado redox, pois sabe-se que ele tem o potencial de aumentar a concentração de espécies reativas de oxigênio (EROS) e inibir enzimas antioxidantes, como por exemplo a glutationa peroxidase (GPx). No entanto, poucos estudos avaliaram estes parâmetros em população ocupacionalmente exposta brasileira. Assim, o presente estudo, objetiva estudar a correlação entre as concentrações de Pb no sangue (Pb-S) de trabalhadores de fábricas de bateria e as atividades das enzimas ALAD e GPx associados com os polimorfismos genéticos da ALAD e GPx. Para tal, foram utilizadas 278 amostras de sangue de trabalhadores expostos ao Pb. As determinações de Pb foram realizadas por espectrometria de massas com plasma acoplado indutivamente (ELAN DRCII Perkin- Elmer). As genotipagens dos polimorfismos genéticos da ALAD e da GPx foram realizadas pela Reação em Cadeia da Polimerase (PCR) em tempo real e as atividades das enzimas ALAD e GPx foram determinadas no sangue por espectrofotometria de UV/VIS. A média da concentração de Pb-S foi de 22,8 ± 14,7 ?g/dL. Foram observadas correlações negativas entre Pb-S e atividade da ALAD (rs -0,24 p<0,01) e Pb-S e atividade de GPx (rs -0,27 p<0,05). Também foi verificada correlação negativa entre a porcentagem de inibição da ALAD e a atividade de GPx (rs -0,21 p<0,01). Em relação aos polimorfismos genéticos, não observamos associação entre os genótipos do ALAD (? -0,19 P>0,05) e GPx (genótipo CT: ? -1,37 P>0,05; genótipo TT: ? -8,37 P>0,05) e a concentração de Pb-S. Não foram observadas associações entre o polimorfismo rs1800668 e a atividade de GPx (genótipo CT: ? -0,016 P>0,05; genótipo TT: ? -0,004 P>0,05). No entanto, foi constatada uma associação entre o genótipo ALAD 1-1 do polimorfismo rs1800435 e a atividade da enzima ALAD (? 3,5 P<0,05). Neste sentido, os resultados deste estudo mostram que o genótipo ALAD 1-1 do polimorfismo rs1800435 do gene ALAD está associado a uma maior atividade da enzima ALAD nos indivíduos expostos ao Pb. Além disso, o polimorfismo rs1800668, localizado no gene que codifica a enzima GPx, não modula a atividade desta enzima nos indivíduos expostos ao metal. Ambos os polimorfismos dos genes ALAD e GPx parecem não influenciar nas concentrações de Pb-S na população estudada. / Lead (Pb) is a highly toxic metal which signs of intoxication vary greatly when considering the interindividual differences. One of the main mechanism of toxicity of Pb is due to inhibition of the enzyme acid delta aminolevulinic dehydratase (ALAD) in the hematopoietic system. Pb also plays an important role in the redox state of unbalance, since it is known that it has the potential of increasing the concentrations of reactive oxygen species (ROS) and inhibit antioxidant enzymes such as glutathione peroxidase (GPx). However, few studies have evaluated these parameters in Brazilian population occupationally exposed. Thus, the present study aims to study the correlation between the concentrations of Pb in the blood (B-Pb) of workers of battery factories and the activities of ALAD and GPx enzymes associated with genetic polymorphisms in ALAD and GPx. Then, blood samples of 278 workers exposed to Pb were collected. Pb was measured by Inductively Coupled Plasma-Mass Spectrometry (Perkin-Elmer ELAN DRCII). The genotyping of genetic polymorphisms of ALAD and GPx was performed by Real-Time Polymerase Chain Reaction (PCR) and activity of ALAD and GPx enzymes in the blood was determined by spectrophotometry UV / VIS. The mean concentration of B-Pb was 22.81 ± 14.73 mg / dL. Negative correlation was found between B-Pb and ALAD activity (rs -0.24 p < 0.01) and B-Pb and GPx activity (rs -0.27 p < 0.05). There was also a negative correlation between the percentage of inhibition of ALAD and GPx activity (rs -0.21 p < 0.01). Considering the genetic polymorphisms, no association between ALAD genotypes (? -0.19 P < 0.05) and GPx (CT genotype: ? -1.37 P > 0.05, TT genotype : ? -8.37 P > 0.05 ) and the concentration of B-Pb. No association between rs1800668 polymorphism and GPx activity (CT genotype: ? -0.016 P > 0.05, TT genotype : ? -0.004 P > 0.05). However an association was found between ALAD 1-1 rs1800435 genotype and ALAD enzyme activity (? 3.5 P < 0.05). Accordingly, the results of this study show that the ALAD 1-1 genotype of rs1800435 polymorphism in ALAD gene is associated with increased activity of ALAD enzyme in individuals exposed to Pb. Furthermore the rs1800668 polymorphism located in a gene encoding the enzyme GPx does not modulate the activity of this enzyme in individuals exposed to the metal. Both polymorphisms of ALAD and GPx genes seem to have no influence in the concentrations of B-Pb in the population studied.

acid delta aminolevulinic dehydratase

chumbo

glutathione peroxidase

glutationa peroxidase

lead

toxicogenetic

toxicogenética

Efeito da glutationa reduzida (GSH) na criopreservação de espermatozóides da espécie canina: avaliação in vitro e in vivo. / Effect of reduced glutathione (GSH) in the cryopreservation of canine spermatozoa: in vitro and in vivo evaluation.

Lúcio, Cristina de Fatima

12 June 2012

O presente experimento teve por objetivos comparar a adição de diferentes concentrações de glutationa reduzida (GSH) no diluidor para criopreservação do sêmen de cães, considerando-se as características morfofuncionais pós-descongelação; e verificar os índices de gestação e número de filhotes por ninhada obtidos a partir da inseminação artificial intra-uterina, por cateterização cervical endoscópica, com sêmen criopreservado contendo diferentes concentrações de glutationa. Na primeira fase do experimento, foram realizadas duas colheitas seminais de 11 reprodutores com intervalo mínimo de uma semana entre os procedimentos. Foram empregadas três concentrações diferentes de glutationa reduzida (0, 10 e 20 mM) ao meio de congelação tris-gema-citrato. O sêmen fresco, refrigerado, glicerolizado e descongelado foram avaliados por citometria de fluxo com uso de sondas específicas para determinar a integridade das membranas plasmática e acrossomal, potencial de membrana mitocondrial e fragmentação de DNA. Também foi realizada dosagem de substâncias reativas ao ácido tiobarbitúrico (TBARS) para avaliar os níveis de estresse oxidativo. Na segunda fase do experimento, foram inseminadas 6 fêmeas, alocadas em dois grupos: inseminação intra-uterina com sêmen congelado em diluidor contendo 10 mM (IA-GSH10, n=3) e sem a adição de glutationa (IA-GSH0, n=3). O acompanhamento do ciclo estral foi realizado por citologia vaginal, vaginoscopia, dosagem de progesterona e LH. Foram realizadas duas inseminações no 5o e 6o dias após pico de LH e a gestação diagnosticada aos 30 dias. A adição de 10 e 20 mM de GSH ao diluidor para criopreservação promoveu queda na motilidade espermática nas amostras descongeladas, sendo o maior prejuízo observado na concentração de 20 mM. Foi detectada maior porcentagem de acrossomos íntegros nos grupos tratados. A glicerolização e, principalmente, a exposição do espermatozóide ao nitrogênio líquido e posterior descongelação foram responsáveis pela diminuição da motilidade espermática, em consequência ao prejuízo da função mitocondrial promovida pela produção de radicais livres durante o processamento seminal. A gestação foi diagnosticada em duas fêmeas do grupo IA-GSH10 e duas do grupo IA-GSH0. Em conclusão, a adição de 10 e 20 mM de GSH ao diluidor para criopreservação seminal não promoveu os efeitos protetores esperados na espécie canina, sendo a concentração de 20 mM responsável por maiores prejuízos à amostra seminal. A adição de 10 mM de GSH ao diluidor para criopreservação seminal na espécie canina manteve o índice de fertilidade semelhante ao obtido com sêmen criopreservado sem a suplementação antioxidante. / The present experiment aimed to compare the addition of different concentrations of reduced glutathione (GSH) on frozen-thawed canine semen, considering the morphofunctional characteristics; and to verify the pregnancy rate and number of puppies per litter obtained from intrauterine insemination by endoscopic catheterization of the cervix, with frozen-thawed semen containing different concentrations of glutathione. During the first phase of the experiment, two seminal samples collected weekly from 11 mature dogs were used. Three different concentrations of reduced glutathione (0, 10 and 20 mM) were supplemented in a tris-citrate egg yolk extender. The fresh, chilled, glycerolized and post-thawed semen were assessed by flow cytometry using specific probes to determine plasma membrane and acrosomal integrity, mitochondrial membrane potential and DNA fragmentation. Thiobarbituric acid reactive substances (TBARS) assay was also performed to assess the occurrence of oxidative stress. In the second phase of the experiment, six canine females were allocated into two groups: intrauterine insemination with frozen-thawed semen containing 10 mM GSH (IA-GSH10, n = 3) and without the addition of glutathione (IA-GSH0, n = 3). Bitches were monitored by vaginal cytology, vaginoscopy, progesterone and LH assays. Two inseminations were performed on days 5 and 6 post LH peak. We verified that the addition of 10 and 20 mM of GSH to semen extender promoted a decrease in post-thaw sperm motility, as well as a higher damage degree at the 20 mM concentration. We also detected a higher percentage of acrossomal integrity in treated groups. At glycerolization and moreover, the sperm exposure to liquid nitrogen and further thawing, were responsible for the decrease in sperm motility, due to the loss of mitochondrial function through the free radicals production. Gestation was diagnosed in two female from IA-GSH10 group and two bitches of the IA-GSH0 group. In conclusion, we did not observe the expected protective effects of the addition of 10 and 20 mM GSH to semen extender. Furthermore, the concentration of 20 mM was responsible for the more extreme damage to semen sample. The supplementation of 10 mM GSH to semen extender for cryopreservation maintained the fertility rates similar to the ones observed for cryopreservation without antioxidant supplementation in dogs.

Artificial insemination

Criopreservação seminal

Endoscopia trancervical

Glutationa reduzida

Inseminação artificial

Reduced glutathione

Semen cryopreservation

Transcervical endoscopy