The early effects of phorbol esters in the lymphocyte membrane

Kwong, Cheung Hing.

January 1982

Thesis (Ph. D.)--University of Wisconsin--Madison, 1982. / Typescript. Vita. eContent provider-neutral record in process. Description based on print version record. Includes bibliographical references.

Role of protein kinase C isoforms in the agonist-stimulated activity of phospholipase D in glia

Mallon, Barbara S.

January 1996

No description available.

572

Preconditioning of Isolated Rabbit Cardiomyocytes: Effects of Glycolytic Blockade, Phorbol Esters, and Ischaemia

Armstrong, Stephen, Ganote, Charles E.

01 January 1994

Objective: The aim was to discriminate among several hypotheses of preconditioning of isolated rabbit cardiomyocytes and to determine if ischaemic preincubation would evoke a protective response. Methods: Isolated myocytes were subjected to 5 min of preincubation, in the presence or absence of glucose, and incubated in the presence of 1 mM iodoacetic acid during the final sustained ischaemic period. In a second series, the protein kinase C (PKC) activators phorbol 12-myristate 13-acetate (PMA), ingenol 3, 20-dibenzoate, and thymeleatoxin were added during preincubation. In a third series, preincubation periods were substituted by brief ischaemic pelleting of cells. Final prolonged ischaemic pelleting was preceded by a 30 min postincubation period. Rate and extent of injury was determined by sequential sampling and assessment of trypan blue permeability following 85 mOsM swelling. Results: Myocytes were preconditioned by a 5 min glucose-free preincubation. Addition of iodoacetic acid into the final ischaemic pellet increased the rates of rigor contracture and injury, but did not abolish the protective response. Direct protein kinase C activation with PMA, a non-selective phorbol ester, and ingenol, an ε, δ-PKC isozyme selective activator, protected cells, but thymeleatoxin, an α,β,γ-PKC isozyme selective activator, did not. A 10 min ischaemic preincubation preconditioned, but the protection was not enhanced when ischaemia was extended to 30 min, or when PMA was included during the initial ischaemic preincubation. Adenosine partially inhibited the response. Conclusions: (1) Preconditioning of isolated myocytes is not dependent on glycolysis or glucose transport. (2) Preconditioning appears dependent on activation of the ε-PKC isoformn. (3) Ischaemia is capable of preconditioning isolated myocytes in vitro, and initiation of this effect is modified by simultaneous additional of adenosine but not by direct protein kinase C activation with PMA. Induction of protection by PMA and ingenol shows that protection requires protein kinase C activation, but direct potassium channel activation by regulatory G proteins is not critical.Cardiovascular Research 1994;28:1700-1706.

adenosine receptors

glycolysis

ischaemic injury

ischaemic preconditioning

isolated myocyte

phorbol esters

protein kinase C

Protein Kinase C-Mediated Contractile Response of the Rat Vas Deferens

Abraham, S. T., Rice, Peter J.

06 August 1992

The role of protein kinase C (PKC) in mediating contractile responses in the rat vas deferens was studied. Phorbol-12,13-di-acetate (PDA) in the presence of 20 mM K+ elicited a concentration-dependent response with an EC50 of 190 nM. The non-PKC activator 4α-phorbol (2 μM) was unable to elicit contraction in 20 mM K+ buffer. Incubation of rat vas deferens with the PKC inhibitor iso-H7 (30 μM) attenuated the response to norepinephrine (NE) ane neurokinin A, with maximal effects depressed to 42 and 39% of control, respectively. Responses to 60 mM K+ and 2 μM PDA (20 mM K+) was also significantly inhibited by iso-H7. In the presence of 2 μM PDA and 20 mM K+, the NE concentration-effect curve was shifted 3,6-fold to the right of the control curve in a parallel manner. 4α-Phorbol (20 mM K+) at the same concentration did not produce this effect. These results suggest a significant role for PKC in the contractile response of the rat vas deferens.

phorbol esters

protein kinase C

vas deferens (rat)

α -Adrenoceptors 1

Localisation of protein kinase C in apoptosis and neurite outgrowth

Schultz, Anna.

January 2005

Thesis (Ph. D.)--Lunds universitet, 2005. / Title from title screen. Description based on contents viewed May 20, 2005. Includes bibliographical references (p. [36]-[48]).

Proteomic analysis of plastids the endosperm of developing seeds of Jatropha (Jatropha curcas L.) / AnÃlise proteÃmica de plastÃdeos do endosperma de sementes em desenvolvimento de pinhÃo manso (Jatropha curcas L.)

Camila Barbosa Pinheiro Jereissati

24 February 2015

CoordenaÃÃo de AperfeiÃoamento de Pessoal de NÃvel Superior / Jatropha curcas L. is a plant native to America and belongs to the Euphorbiaceae family. Currently it is gaining economical interest mainly because it is an oilseed crop with potential to produce biodiesel. However, presence of phorbol esters (a class of diterpenes) that are the major toxic constituents of the seeds, limits a better usage of the plant, by making the use of the residue, obtained after the oil extraction from the seeds, unfeasible for animal feed, due to its pro-carcinogenic activity and inflammatory action. Proteomic analysis of the plastids isolated from developing seeds of Jatropha is important because the synthesis of fatty acid as well as phorbol esters, the two most attractive compounds in the study of Jatropha curcas, occur in plastids. Proteomic analysis of this organelle is crucial to better understand and explore not only the biosynthetic pathway of these two compounds but other metabolic pathways , and addtionaly providing foundation for researchs that aimed to develope genotypes with more suitable characteristics for industrial applications. In this study, we performed a proteomic analysis of plastids isolated from the endosperm of developing Jatropha curcas seeds that were in the initial stage of deposition of protein and lipid reserves. Proteins extracted from the plastids were digested with trypsin, and the peptides were applied to an EASY-nano LC system coupled online to an ESI-LTQ-Orbitrap Velos mass spectrometer, and this led to the identification of 1103 proteins representing 804 protein groups, of which 923 were considered as true identifications, and this considerably expands the repertoire of J. curcas proteins identified so far. Of the identified proteins, only five are encoded in the plastid genome, and none of them are involved in photosynthesis, evidentiating the nonphotosynthetic nature of the isolated plastids. Homologues for 824 out of 923 identified proteins were present in three different plastids proteins databases i.e. PPDB, SUBA and PlProt, while homologues for 13 proteins were not found in any of these three databases but were marked as plastidial by at least one of the three prediction programs used (TargetP, ChloroP and PlantMPloc). Functional classification showed that proteins belonging to amino acids metabolism comprise the main functional class, followed by carbohydrate, energy, and lipid metabolisms. The small and large subunits of Rubisco were identified, and their presence in plastids is considered to be an adaptive feature counterbalancing for the loss of one-third of the carbon as CO2 as a result of the conversion of carbohydrate to oil through glycolysis. While several enzymes involved in the biosynthesis of several precursors of diterpenoids were identified, we were unable to identify any terpene synthase/cyclase, which suggests that the plastids isolated from the endosperm of developing seeds do not synthesize phorbol esters. In conclusion, this study provides insights into the major biosynthetic pathways and certain unique features of the plastids from the endosperm of developing seeds at the whole proteome level. / O pinhÃo manso (Jatropha curcas L.) à uma planta nativa da AmÃrica, pertencente à famÃlia Euphorbiaceae. Atualmente, ela desperta interesse econÃmico principalmente por se tratar de uma oleaginosa com potencial para a produÃÃo de biodiesel. Entretanto, a presenÃa de Ãsteres de forbol (uma classe de diterpeno), que sÃo os principais constituintes tÃxicos das sementes, limita uma melhor utilizaÃÃo dessa planta, por inviabilizar o uso do resÃduo de extraÃÃo do Ãleo das sementes na alimentaÃÃo animal, bem como, por apresentar atividade prÃ-carcinogÃnica e aÃÃo inflamatÃria. A anÃlise proteÃmica de plastÃdeos, isolados de sementes em desenvolvimento de pinhÃo manso, à uma importante vertente de estudo, pois tanto a sÃntese de Ãcidos graxos como dos Ãsteres de forbol, os dois compostos mais atrativos no estudo de Jatropha curcas, ocorrem nos plastÃdeos. O estudo proteÃmico dessa organela torna-se crucial para melhor compreender e explorar nÃo somente as vias biossintÃticas desses dois compostos, como de outras vias metabÃlicas, alÃm de proporcionar um conjunto de dados que pode ser utilizado em pesquisas voltadas para o desenvolvimento de genÃtipos com caracterÃsticas mais adequadas para aplicaÃÃes industriais. No presente trabalho, realizou-se uma anÃlise proteÃmica de plastÃdeos isolados do endosperma de sementes em desenvolvimento do pinhÃo manso, que estavam nos estÃgios iniciais de deposiÃÃo de lipÃdios e proteÃnas de reserva (25-30DAA), confirmados por meio de anÃlises histolÃgica e histoquÃmica. As proteÃnas extraÃdas dos plastÃdeos foram digeridas com tripsina e os peptÃdeos foram aplicados no sistema de nano-LC EASYII acoplado online ao espectrÃmetro de massa nano ESI LTQ-Orbitrap velos, o que resultou na identificaÃÃo 1103 proteÃnas, representando 804 grupos de proteÃnas, dos quais 923 foram consideradas identificaÃÃes verdadeiras. Isso expandiu consideravelmente o repertÃrio de proteÃnas do pinhÃo manso atà agora identificas. Dentre as proteÃnas identificadas, apenas 5 sÃo codificadas pelo genoma plastidial, e nenhuma delas està envolvida na fotossÃntese, o que evidencia a natureza nÃo fotossintÃtica dos plastÃdeos isolados. HomÃlogos de 824, dentre as 923 proteÃnas identificadas, estavam presentes nos bancos de dados PPDB, SUBA e PlProt, enquanto homÃlogos para 13 proteÃnas nÃo foram encontrados em nenhum dos trÃs bancos de dados plastidiais, mas foram detectados como plastidiais por pelo menos um dos trÃs programas de prediÃÃo de localizaÃÃo subcelular utilizados (TargetP, ChloroP, PlantMPloc). A classificaÃÃo funcional mostrou que a maioria das proteÃnas identificadas pertencia ao metabolismo dos aminoÃcidos, seguido dos metabolismos dos carboidratos, energÃtico e dos lipÃdios. As subunidades maiores e menores da Rubisco foram identificadas, e sua presenÃa nos plastÃdeos foi considerada uma caracterÃstica adaptativa para contrabalancear a perda de um terÃo do carbono na forma de CO2 como um resultado da conversÃo de carboidratos em Ãleo atravÃs da glicÃlise. Apesar de enzimas envolvidas na biossÃntese de diversos precursores dos diterpenÃides terem sido identificadas, nÃo foi detectado nenhuma terpeno sintase/ciclase, o que sugere que os plastÃdeos isolados do endosperma de sementes em desenvolvimento nÃo sintetizam Ãsteres de forbol, apesar de uma grande quantidade desse composto ser encontrada neste tecido. Como conclusÃo, o presente trabalho proporciona insights sobre as principais vias biossÃntÃticas, e sobre caracterÃsticas peculiares dos plastideos isolados do endosperma de sementes em desenvolvimento.

Jatropha curcas

ProteÃmica de oleaginosas

ProteÃmica plastidial

ProteÃmica de plantas

Ãsteres de forbol

Jatropha curcas

Proteomics of oil crop

Plastid proteomics

Plant proteomics

Phorbol esters

BIOQUIMICA

Espectrometria de massas por probe electrospray ionization (PESI-MS) com polímero molecularmente impresso (MIP) para determinação de ésteres de forbol em folhas de Jatropha curcas / Molecularly imprinted polymer-coated probe electrospray ionization mass spectrometry (MIPCPESI-MS) for determination of phorbol esters in Jatropha curcas leaves

Silva, Lidya Cardozo da

20 July 2018

Submitted by Luciana Ferreira (lucgeral@gmail.com) on 2018-08-20T13:36:48Z No. of bitstreams: 2 Dissertação - Lidya Cardozo da Silva - 2018.pdf: 2382834 bytes, checksum: e5a79619d923d442540c5bf0549318bd (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) / Approved for entry into archive by Luciana Ferreira (lucgeral@gmail.com) on 2018-08-20T13:38:04Z (GMT) No. of bitstreams: 2 Dissertação - Lidya Cardozo da Silva - 2018.pdf: 2382834 bytes, checksum: e5a79619d923d442540c5bf0549318bd (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) / Made available in DSpace on 2018-08-20T13:38:04Z (GMT). No. of bitstreams: 2 Dissertação - Lidya Cardozo da Silva - 2018.pdf: 2382834 bytes, checksum: e5a79619d923d442540c5bf0549318bd (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) Previous issue date: 2018-07-20 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPES / Jatropha curcas L. is a euphorbiaceous oilseed plant considered toxic to humans and animals due to the presence of phorbol esters (PEs). Traditionally, the detection of these toxic compounds has been done in J. curcas seeds and derivates via chromatographic separation methods such as HPLC-UV and HPLC-MS. Although efficient, these techniques are laborious and require high time and solvent consumption, thus it would be interesting the development of new analytical methods to determine these compounds with more practicality. Probe electrospray ionization is frequently used in ambient mass spectrometry allowing analysis with minimum sample preparation. However, for complex samples analysis, this technique presents low sensitivity and ionization suppression. In this study, a molecularly imprinted polymer-coated probe electrospray ionization mass spectrometry (MIPCPESI-MS) method was developed for determination of phorbol esters in methanolic extracts of Jatropha curcas leaves with direct extraction form the ionization source. The synthesized molecularly imprinted polymer (MIP) proved to be adequate for extraction of the PEs in methanolic extracts of J. curcas leaves with better performance as extraction phase in comparison with the non-imprinted polymer (NIP). The MIPCPESI method allowed detection of phorbol 12,13-diacetate (PDA) and other three PEs metabolite ions from Jatropha leaves with minimal sample preparation, and with higher signal intensities compared to analysis with conventional PESI. For the PDA, calibration curve exhibited linearity with R2 > 0.99, LOD and LOQ in µg.mL-1 range, precision and accuracy values, respectively, between 4.06 to 13.49% and -1.60 to -15.26 %. Finally, MIPCPESI was employed for PDA quantification in methanolic extracts of six different J. curcas leaves genotypes resulting in concentrations ranging from 222.19 ± 23.55 to 528.23 ± 19.72 µg.g-1 for toxic samples. / A Jatropha curcas L. é uma oleaginosa euforbiácea considerada tóxica para humanos e animais devido à presença de ésteres de forbol (PEs). Tradicionalmente, a detecção destes compostos tóxicos tem sido feita em tortas e sementes de J. curcas por meio do uso de técnicas de separação cromatográfica como HPLC-UV e HPLC-MS que apesar de eficientes são laboriosas e requerem alto consumo de tempo e solventes. Dessa forma, seria interessante o desenvolvimento de novas técnicas analíticas para determinação desses compostos com maior praticidade. Probe electrosrpay ionization (PESI) é uma das técnicas de ionização utilizadas na espectrometria de massas ambiente que permite análises rápidas com mínimo preparo de amostras. No entanto, para análise de amostras complexas essa técnica apresenta baixa sensibilidade e supressão iônica. Neste estudo, foi desenvolvido um método de análise por espectrometria de massas por Probe electrospray revestido com polímero molecularmente impresso (MIPCPESI-MS) para determinação de ésteres de forbol em extratos metanólicos de folhas de Jatropha curcas com extração direta da fonte de ionização. O polímero molecularmente impresso (MIP) sintetizado mostrou-se adequado para extração de PEs em extratos metanólicos de folhas de J. curcas tendo melhor desempenho como fase extratora quando comparado ao polímero não molecularmente impresso (NIP). O método MIPCPESI-MS possibilitou a detecção do forbol 12,13-diacetato (PDA) e de outros três íons metabólitos presentes nas folhas de J. curcas com mínimo preparo de amostras e com maior intensidade de sinais quando comparado às análises com PESI convencional. Para o PDA, a curva de calibração apresentou linearidade com R2 > 0.99, LOD e LOQ na faixa de µg.mL-1, valores de precisão entre 4.06 e 13.49 % e exatidão entre -1.60 e -15.26 %. Posteriormente, o método MIPCPESI foi empregado na quantificação de PDA em seis extratos metanólicos de diferentes genótipos de folhas de J. curcas resultando em valores concentrações entre 222.19 ± 23.55 a 528.23 ± 19.72 µg.g-1 nas amostras tóxicas.

Espectrometria de massas ambiente

Probe electrospray ionization

Polímero molecularmente impresso

Jatropha curcas

Ésteres de forbol

Ambient mass spectrometry

Probe electrospray ionization

Molecularly imprinted polymer

Jatropha curcas

Phorbol esters

CIENCIAS EXATAS E DA TERRA::QUIMICA

Aberrations in Cytokine Signaling in Leukemia: Variations in Phosphorylation and O-GlcNAcylation

Tomic, Jelena

31 August 2012

Tumor-induced immunosuppression can occur by multiple mechanisms, each posing a significant obstacle to immunotherapy. Evidence presented in this dissertation suggests that aberrant cytokine signaling, as a result of altered metabolism of Chronic Lymphocytic Leukemia (CLL) cells, confers a selective advantage for tumor survival and growth. Cells from CLL patients with aggressive disease (as indicated by high-risk cytogenetics) were found to exhibit prolongation in Interferon (IFN)-induced STAT3 phosphorylation, and increased levels of reactive oxygen species (ROS) in these cells reflected these signaling processes. Changes in the relative balance of phospho-STAT3 and phospho-STAT1 levels, in response to combinations of IL-2 + Toll-like receptor (TLR)-7 agonist + phorbol esters, as well as IFN, were associated with the immunosuppressive and immunogenic states of CLL cells. In addition, immunosuppressive leukemic cells were found to express high levels of proteins with O-linked N-acetylglucosamine (O-GlcNAc) modifications, due to increased metabolic activity through the Hexosamine Biosynthetic Pathway (HBP), which caused impaired intracellular signaling responses and affected disease progression. A conclusion of the studies presented here is that the intrinsic immunosuppressive properties of leukemic cells may be overcome by agents such as Resveratrol that target metabolic pathways of these cells.

Chronic Lymphocytic Leukemia

Immunogenicity

Interferon (IFN)

STAT3

Reactive Oxygen Species (ROS)

Tumor suppressor p53

phosphatases

Toll-like receptor (TLR)-7 agonist

phorbol esters

immunosuppressive cytokines

O-GlcNAc

Hexosamine Biosynthetic Pathway (HBP)

Glucosamine

Resveratrol

Friend Erythroleukemia

RL2 antibody

cancer vaccines

IL-2

tumor immunosuppression

phosphorylation

O-GlcNAcylation

cytotoxic T lymphocytes (CTLs)

Ataxia telangiectasia mutated (ATM)

Antigen presenting cell (APC)

Immunotherapy

OGT

OGase

glucose

tumor metabolism

PKC

CD83

Warburg effect

tumor microenvironment

IL-10

tumor-reactive T cells

Aberrations in Cytokine Signaling in Leukemia: Variations in Phosphorylation and O-GlcNAcylation

Tomic, Jelena

31 August 2012

Tumor-induced immunosuppression can occur by multiple mechanisms, each posing a significant obstacle to immunotherapy. Evidence presented in this dissertation suggests that aberrant cytokine signaling, as a result of altered metabolism of Chronic Lymphocytic Leukemia (CLL) cells, confers a selective advantage for tumor survival and growth. Cells from CLL patients with aggressive disease (as indicated by high-risk cytogenetics) were found to exhibit prolongation in Interferon (IFN)-induced STAT3 phosphorylation, and increased levels of reactive oxygen species (ROS) in these cells reflected these signaling processes. Changes in the relative balance of phospho-STAT3 and phospho-STAT1 levels, in response to combinations of IL-2 + Toll-like receptor (TLR)-7 agonist + phorbol esters, as well as IFN, were associated with the immunosuppressive and immunogenic states of CLL cells. In addition, immunosuppressive leukemic cells were found to express high levels of proteins with O-linked N-acetylglucosamine (O-GlcNAc) modifications, due to increased metabolic activity through the Hexosamine Biosynthetic Pathway (HBP), which caused impaired intracellular signaling responses and affected disease progression. A conclusion of the studies presented here is that the intrinsic immunosuppressive properties of leukemic cells may be overcome by agents such as Resveratrol that target metabolic pathways of these cells.

Chronic Lymphocytic Leukemia

Immunogenicity

Interferon (IFN)

STAT3

Reactive Oxygen Species (ROS)

Tumor suppressor p53

phosphatases

Toll-like receptor (TLR)-7 agonist

phorbol esters

immunosuppressive cytokines

O-GlcNAc

Hexosamine Biosynthetic Pathway (HBP)

Glucosamine

Resveratrol

Friend Erythroleukemia

RL2 antibody

cancer vaccines

IL-2

tumor immunosuppression

phosphorylation

O-GlcNAcylation

cytotoxic T lymphocytes (CTLs)

Ataxia telangiectasia mutated (ATM)

Antigen presenting cell (APC)

Immunotherapy

OGT

OGase

glucose

tumor metabolism

PKC

CD83

Warburg effect

tumor microenvironment

IL-10

tumor-reactive T cells