EXPRESSÃO E CARACTERIZAÇÃO DE UM FRAGMENTO DA GLICOPROTEÍNA E DO HERPESVÍRUS BOVINO TIPO 1 E USO EM UM TESTE SOROLÓGICO DIFERENCIAL / EXPRESSION AND CHARACTERIZATION OF A TRUNCATED FORM OF BOVINE HERPESVIRUS TYPE 1 ENVELOPE GLYCOPROTEIN E AND ITS USE IN A DIFFERENTIAL SEROLOGICAL TEST

Oliveira, Stephan Alberto Machado de

05 March 2012

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / Bovine herpesvirus type 1 (BoHV-1) is distributed worldwide and produces high economic losses to the in livestock industry. BoHV-1 infection causes respiratory, reproductive and may also be associated with neurological signs. There are several tests that can diagnose the infection, however, serological techniques currently used are not able to differentiate antibodies produced by vaccination from those produced in response to natural infection. What is sought is a mean to differentiate vaccinated animals of those infected by the field strain. Vaccines with deletion in the glycoprotein E (gE) gene have been developed for this purpose. However, this also requires the development of tests capable to differentiate the serological response between infected and vaccinated animals. To this end, a 651 nucleotide fragment corresponding to the amino-terminal third (217 amino acids) of the BoHV-1 gE gene - that shares a high identity with the homologous BoHV-5 counterpart - was cloned as a 6×His-tag fusion protein in an Escherichia coli expression vector pET16b. A soluble protein of approximately 25 kDa was purified from lysates of transformed E. coli. The recombinant protein was detected in Western blot (WB) by anti-6-his tag and anti BoHV-1 gE monoclonal antibodies. Antibodies present in the sera of cattle infected with BoHV-1 and BoHV-5 reacted specifically with the 25 kDa recombinant protein in WB. Moreover, mice immunized with the purified protein developed antibodies that recognized the viral gE in lysates of cell monolayers infected with BoHV-1 and BoHV-5. An indirect ELISA for gE antibodies, based on the expressed protein, was able to differentiate serologically calves vaccinated with a gE-deleted BoHV- 5 strain from calves experimentally infected with BoHV-1 or BoHV-5. These data demonstrate that the antigen retained its immunological properties and, thus, can be used in serological tests for bovine herpesvirus infections. It has a potential use in a indirect ELISA to differentiate naturally infected animals from those vaccinated whit the recombinant, gE-negative strains. / O herpesvírus bovino tipo 1 (BoHV-1) é um vírus de distribuição mundial e produz grandes prejuízos econômicos em rebanhos de corte e de leite. A infecção pelo BoHV-1 produz manifestações respiratórias, reprodutivas e também pode cursar com sinais nervosos. Existem diversos testes laboratoriais capazes de diagnosticar a infecção. Contudo, as técnicas sorológicas empregadas atualmente não são capazes de diferenciar anticorpos produzidos pela vacinação daqueles produzidos em resposta à infecção natural. Assim, vacinas diferenciais com deleção da glicoproteína E (gE) têm sido desenvolvidas com essa finalidade. No entanto, necessita-se também de testes capazes de diferenciar a produção de anticorpos vacinais dos induzidos pelo vírus vacinal. Com essa finalidade, essa dissertação relata a expressão e caracterização de um fragmento da glicoproteína E do BoHV-1 e seu uso no desenvolvimento e padronização de um ELISA indireto para detecção de anticorpos anti-gE. Um fragmento de 651 nucleotídeos correspondente ao terço amino-terminal (217 aminoácidos) do gene da gE do BoHV-1, que possui uma alta identidade com o homólogo herpesvírus bovino tipo 5 (BoHV-5), foi clonado com proteína de fusão 6xHis-tag em Escherichia coli utilizando vetor de expressão pET16b. Uma proteína solúvel de aproximadamente 25kDa foi purificada a partir de lisados de E. coli transformadas. A proteína recombinante foi detectada por Western blot (WB) por anticorpos monoclonais anti-histidina e anti-gE do BoHV-1. Anticorpos presentes no soro de animais infectados com BoHV-1 e BoHV-5 reagiram especificamente com a proteína recombinante no WB. Além disso, camundongos imunizados com a proteína purificada desenvolveram anticorpos que reconheceram a gE viral proveniente de lisados de monocamadas celulares infectadas com BoHV-1 e BoHV-5. Um ELISA indireto para detecção de anticorpos anti-gE, baseado na proteína expressa, foi capaz de diferenciar sorologicamente animais vacinados com a cepa gE deletada do BoHV-5 dos animais experimentalmente infectados com BoHV-1 ou BoHV-5. Esses resultados demonstram que o antígeno obtido conservou suas características imunológicas e pode ser utilizado na detecção sorológica das infecções por herpesvírus bovinos. Possui potencial para uso em grande escala como antígeno em testes de ELISA para diferenciar animais naturalmente infectados de animais vacinados com a cepas defectivas na gE

Teste imunoenzimático

BoHV-1

BoHV-5

Antígeno

Proteína recombinante

Enzyme-linked immunosorbent assay

BoHV-1

BoHV-5

Antigen

Recombinant protein

Gelatinases, their tissue inhibitors and p53 in lymphomas

Kyllönen, H. (Heli)

26 May 2009

Abstract Lymphomas are a heterogeneous group of malignancies, which usually have a good prognosis and high cure rates. Lymphomas are sensitive to chemotherapy and radiotherapy, and many patients can be cured even after a relapse, resulting in a need for effective follow-up. However, the cost-benefit ratio of radiological imaging in predicting the forthcoming relapses is poor. Consequently, there is a need for biological prognostic and predictive markers to distinguish patients at the highest risk of relapse at the time of diagnosis or during follow-up. Despite rapid progress in lymphoma treatments, some patients still die from lymphoma. Thus, more data on the basic biological features of lymphomas are also needed. Gelatinases (MMP-2 and MMP-9) and their tissue inhibitors (TIMP-1 and TIMP-2) have been found to play a role in the progression of solid tumours. TP53 is a tumour suppressor gene, the mutations and protein over-expression of which have been demonstrated to be associated with survival in most cancer types. There is also some evidence that these proteins could have prognostic significance in lymphomas as well. In the present study, the tissue expression, plasma concentrations and clinical value of gelatinases and their tissue inhibitors were evaluated in lymphomas. 249 primary tissue samples from patients with Hodgkin, follicular, or diffuse large B-cell lymphoma were analysed for expression of gelatinases and/or their inhibitors using immunohistochemistry. In follicular lymphoma, p53 protein expression was also investigated. The plasma samples of 126 lymphoma patients and a control group of 44 healthy volunteers were collected and studied by ELISA. TIMP-1 expression correlated with bulky tumour and nodular sclerosis subtype of Hodgkin lymphoma. In follicular lymphoma, p53 over-expression was an independent adverse prognostic factor for survival and a predictor of histological transformation. Plasma MMP-2-TIMP-2 complex appeared to be a potential follow-up marker predicting the risk of relapse in lymphoma patients. Plasma levels of the MMP-2-TIMP-2 complex, proMMP-2, TIMP-2 and proMMP-2/TIMP-2 ratio were at abnormal levels both in patients with newly diagnosed lymphoma and those in remission compared to healthy controls. The clinical significance of these markers needs further studies.

biological marker

enzyme-linked immunosorbent assay

immunohistochemistry

lymphoma

matrix metalloproteinase 2

matrix metalloproteinase 9

prognosis

survival

tissue inhibitor of metalloproteinase-1

tissue inhibitor of metalloproteinase-2

tumor suppressor protein p53

Uso do óleo de arroz na cicatrização de úlceras cutâneas em ratos (Rattus norvegicus albinus) / Use of rice oil for treatment of cutaneous ulcers (Rattus norvegicus albinus)

Lania, Bruno Grosselli, 1987-

22 August 2018

Orientadores: Paulo Eduardo Neves Ferreira Velho, Maria Letícia Cintra / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Ciências Médicas / Made available in DSpace on 2018-08-22T07:25:40Z (GMT). No. of bitstreams: 1 Lania_BrunoGrosselli_M.pdf: 3238329 bytes, checksum: 957e602fc97c4a033665229ade46faca (MD5) Previous issue date: 2013 / Resumo: Introdução: o processo de cicatrização é longo e complexo, dura meses nos humanos, e depende de diversos fatores locais e gerais. Ele pode ser divido em três fases: inflamatória, proliferativa e de remodelação. Para que ocorra, é necessária uma cascata de eventos e a participação de diversos tipos de células, bem como de substâncias por elas secretadas. Entre estas destacam-se as substâncias pró-cicatriciais, como a leptina, IL-2, IL-4, IL-6 e o IGF-1, as anti-cicatriciais, como a adiponectina, IL-12, o IFN-?, o IFN-? e, finalmente, o TNF-?, que possui ação variável, de acordo com a concentração circulante desta substância. Muito há para se pesquisar nesse campo, e o desenvolvimento de produtos, com princípios ativos que estimulam a cicatrização, mas de baixo custo, que aproveite matérias-primas encontradas na região, poderia beneficiar um número grande de indivíduos. Foi demonstrado que o uso do óleo do farelo de arroz induz a proliferação de linfócitos, a síntese de citocinas, o aumento da hematopoese e a atividade fagocítica de macrófagos. Objetivos: testar a efetividade do óleo de arroz na cicatrização de feridas cutâneas, e avaliar, tanto no tecido lesado, como no sangue, a sua ação em fatores que atuam na cicatrização. Material e métodos: sobre feridas cirúrgicas circulares produzidas pela exérese da pele, com bisturi, no dorso de ratos, (45 animais, divididos em três grupos) foi aplicado um produto à base de óleo de arroz (patente BR 10 2012 008718 9). O processo de cicatrização foi avaliado por meio do estudo histológico e da quantificação tissular (por meio da PCR real time) e sérica (por meio da técnica Elisa), de fatores que atuam na cicatrização: leptina, IL-2, IL-4, IL-6, IGF-1, adiponectina, IL-12, IFN-?, IFN- ? e TNF- ?. Resultados e conclusões: comparativamente com o controle, foi encontrada diferença significante na celularidade das feridas e detectada ação sistêmica do produto, face ao aumento dos níveis séricos de adiponectina, leptina, IL-2, IL-6, TNF-? e IFN-?. Os resultados deste trabalho poderão ser úteis para a indústria farmacêutica e cosmecêutica brasileira ou internacional / Abstract: The wound healing process is long and complex, lasts months and depends on many local and general factors. It can be divided into three phases: inflammatory, proliferative and remodeling. For that to occur, it is necessary a cascade of events involving several cell types, as well as substances secreted by them. Among these we highlight the pro-healing substances such as leptin, IL-2, IL-4, IL-6 and IGF-1, anti-scarring such as IL-12, IFN-?, IFN- ? and, finally, TNF-?, which possesses variable action, according to the circulating concentration of this substance. More research is needed in this field, and the development of products with active ingredients that stimulate healing, but of low cost, which uses raw materials found in the region, could benefit a large number of individuals. It has been shown that the use of rice bran oil induces lymphocyte proliferation, cytokine synthesis, increased hematopoiesis and phagocytic activity of macrophages. The objectives of this study were to test the effectiveness of rice oil topical use and assess both the injured tissue and blood to evaluate its action on factors that act in healing. Methods: Circular surgical wounds were produced by excision of skin with a scalpel in the back of rats (45, divided into three groups), then applied saline solution or essentials fatty acids or rice bran oil (patent BR 10 2012 0087 18 9). The healing process was evaluated by histological examination and quantification of tissue (by real time PCR) and serum (by ELISA technique), factors that act in healing, namely leptin, IL-2, IL -4, IL-6, IGF-1, adiponectin, IL-12, IFN-?, IFN-? and TNF-?. Compared with control, there was significant difference in the cellularity of the wound healing area and systemic action of the product detected by the increases in serum levels of adiponectin, leptin, IL-2, IL-6, TNF-? and IFN -?. The results of this study may be useful to the Brazilian or international pharmaceutical and cosmeceutical industry / Mestrado / Clinica Medica / Mestre em Clinica Medica

Ensaio de imunoadsorção enzimática

Mediadores da inflamação

Dermatologia

Enzyme-linked immunosorbent assay

Inflammation mediators

Real-time polymerase chain reaction

Dermatology

Desenvolvimento de modelo animal de leucemia linfóide aguda pediátrica : teste ELISA para monitorar a progressão da leucemia / Acute lymphoblastic leukemia animal model development : leukemia progression monitoring by ELISA

Milani, Mateus, 1985-

02 December 2014

Orientador: José Andrés Yunes / Dissertação (mestrado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-24T08:28:04Z (GMT). No. of bitstreams: 1 Milani_Mateus_M.pdf: 3959646 bytes, checksum: a36674e099fefbc487286cdc33006c0a (MD5) Previous issue date: 2014 / Resumo: A leucemia linfoide aguda (LLA) é o câncer mais comum na infância. O transplante de células primárias de LLA humana em camundongos imunosuprimidos tem sido de suma importância para o entendimento da fisiopatologia da doença e para o teste de novos fármacos. Ao contrário de modelos animais de tumores sólidos, cujo volume é facilmente medido na superfície dos animais, a LLA infiltra órgãos inacessíveis ao exterior, daí a necessidade de definir métodos adequados para o monitoramento da progressão da doença. Resultados aqui apresentados indicam que proteínas secretadas pela LLA podem servir como marcadores quantitativos da carga leucêmica, facilmente aferidos por ELISA de amostras de plasma sanguíneo. Dentre três proteínas testadas (B2M, IGFBP2 e Hsp90), o ELISA de Hsp90 apresentou sensibilidade superior à análise da porcentagem de células leucêmicas no sangue dos animais, por citometria de fluxo de células marcadas com anti-huCD45. Os níveis de Hsp90 humano no plasma sanguíneo mostraram-se positivamente correlacionados com o porcentual de células leucêmicas na medula óssea e fígado e em menor grau com os níveis do baço e sangue periférico (SP) ao longo do tempo, tanto nas LLA de linhagem B quanto nas LLA-T. O ELISA de Hsp90 permite detectar a instauração da leucemia nos animais transplantados, até duas semanas antes da detecção pelo método tradicional de análise de sangue periférico por citometria de fluxo. Ao contrário do observado para IGFBP2, o tratamento dos animais leucêmicos com Dexametasona ou um inibidor da PI3K não interferiu nos níveis de Hsp90, que se mantiveram proporcionais à porcentagem de células leucêmicas huCD45+ no sangue periférico. No conjunto, os resultados demonstram que a análise do plasma dos animais por ELISA de Hsp90 é um método melhor do que os atualmente utilizados, para diagnóstico precoce e acompanhamento de LLA humana quando em níveis de doença residual mínima, ou seja, quando a porcentagem de células de LLA é inferior a 5% do total de células da medula óssea / Abstract: Acute lymphoblastic leukemia (ALL) is the most common type of childhood cancer . The transplantation of human primary ALL cells in immunodeficient mice has been of much importance for understanding the disease's pathophysiology and testing new drugs. Unlike animal models of solid tumors whose volume is easily measured on the animal surface, the ALL infiltrates organs that are inaccessible to external antigens, hence the need to define more suitable methods for monitoring the disease's progression. Results presented here indicate that proteins secreted by the ALL can serve as quantitative markers of leukemic burden and are easily measured by ELISA of blood plasma samples. Among three tested proteins (B2M, IGFBP2 and Hsp90), Hsp90 ELISA analysis showed higher sensitivity than the analysis of leukemic cells on animal blood by flow cytometry of anti- huCD45 labeled cells. The levels of Hsp90 in human blood plasma were shown to be positively correlated with the percentage of leukemic cells in the bone marrow and liver and to a lesser extent with the levels in the spleen and peripheral blood (PB) over time, both in B-lineage ALL as in ALL-T. The Hsp90 ELISA allows the leukemia's engraftment detection in transplanted animals up to two weeks prior to detection by the traditional method of peripheral blood analysis by flow cytometry. Unlike observed for IGFBP2, treatment of leukemic animals with Dexamethasone or PI3K inhibitors did not interfere in Hsp90 levels, which remained proportional to the percentage of huCD45+ leukemic cells in the peripheral blood. Taken together, the results demonstrate that the analysis of animal plasma by Hsp90 ELISA is a better method than those currently used for early diagnosis and monitoring of human ALL on minimal residual disease levels, when the percentage of ALL cells is less than 5 % of the total bone marrow cells / Mestrado / Genetica Animal e Evolução / Mestre em Genética e Biologia Molecular

Leucemia linfóide aguda - Diagnóstico

Proteínas de choque térmico HSP90

Ensaio de imunoadsorção enzimática

Modelos animais

Acute lymphoblastic leukemia - Diagnosis

HSP90 heat-shock proteins

Enzyme-linked immunosorbent assay

Animal models

The development of a university-based sex counselling programme in the age of AIDS.

Nicholas, Lionel John

January 1993

Philosophiae Doctor - PhD / The sexual behaviours, attitudes, beliefs and communication of 1896 black first-year university students were examined by means of a structured questionnaire for their contribution to the development of a university-based sex counselling programme. The areas of sexuality investigated included intra-familial communication about contraception and sexuality, belief in sex myths, knowledge of and myths about AIDS and the manner of acquisition of sex knowledge. The results of this study are consistent in reflecting much greater deficits in the knowledge of respondents about sexuality than encountered in the literature. Statistically significant gender differences were found for intra-familial communication about contraception, prejudice towards AIDS victims, knowledge of the modes of HIV infection, prejudice towards homosexuals, belief in myths about sexuality, age at which sex information was acquired, the preferred source of information about sexuality, attitude towards pre-marital intercourse, experience of pre-marital intercourse, belief about the acceptability of abortion, experience of pre-marital intercourse and worry about masturbation. No gender differences were found for belief in myths about high-risk AIDS infection, exposure to sex information within educational institutions and approval of sex education. The statistically significant gender differences which were found for most of the questionnaire items reflect the different sexual socialization experiences of respondents. Male and female students may therefore require counselling interventions geared to their respective needs Concern about AIDS has become central to university student sexual behaviour as well as protection against rape and sexual harassment and male responsibility for contraception. All campus counsellors will eventually experience the impact of AIDS and other sexually·transmitted diseases in their sessions with clients. Sexual harassment, rape, contraceptive failure and abortion will also increasingly impact on counselling sessions and require the university-based counsellor's involvement in broader university-wide prevention programmes as well as group based interventions. The development of a university-based sex counselling programme requires comprehensive interventions ranging from individual counselling to human sexuality courses. An awareness of the high profile sexuality problems as perceived by students, is essential for the development of preventive programmes at the group and academic class level as well as at the level of inf luencing uni versi ty policy. Knowledge of the merits of different theoretical positions and interventions for particular sexual problems is crucial for counselling intervention or referral. A systemic model of intervention for sexuality problems is proposed. The task of university-based sex counselling programmes is made more onerous by the paucity and ineffectiveness of sex information students are exposed to, the lack of sex education in the schools and the inadequate quality and degree of intrafamilial communication about sexuality. A significant proportion of respondents engage in pre-marital sexual intercourse without the benefit of adequate sex knowledge. The results of this study emphasize the need for research on the sexuality of, black South Africans, the particular vulnerabilities of first-year university students to sexuality problems and the dire need for structured sex education programmes at school as well as university.

Sexually Transmitted Diseases (STD’s

Psychoanalytic

Counselling

Psychosocial

Attitudes

Beliefs

Communication

Black first-year University students

Mitigating the impact of antidrug antibodies against insulin on ELISA assay

Bøwadt, Thea

January 2021

Diabetes has, in the past three decades, surged immensely. Because of this, new insulin analogues are constantly in the making.  In clinical studies, the presence of antidrug antibodies can prove a challenge when measuring insulin. In order to overcome the interference from antidrug antibody complexes on the total insulin measurement in human serum, several pre-treatment methods on insulin and polyclonal antibodies spiked samples were tried using ELISA analysis. Several different methods were tried, acid dissociation using a glycine buffer with and without ethanol in different concentrations, high ionic strength dissociation using MgCl2, Polyethylene glycol (PEG) and filtration. The best results were found when using the acid dissociation technique. Using glycine promising results were achieved, especially when 20 % ethanol was added to the acid mixture. Pre-treatment using PEG, MgCl2 and filtration was unsuccessful with the methods used. The main goal was reached through the use of glycine with the addition of 20% ethanol for acid dissociation. The proposed method still leaves significant room for optimisation and needs further verification on real patient samples. However, it is a good step in the direction of a global methodology using ELISA to overcome antidrug antibody interference for total insulin measurement in human serum.

Enzyme-Linked Immunosorbent Assay

ELISA

Antidrug antibodies

ADA

Insulin

Polyethylene glycol

PEG

Acid dissociation

MgCl2.

Biomedical Laboratory Science/Technology

Release kinetics of tumor necrosis factor-α and interleukin-1 receptor antagonist in the equine whole blood

Rütten, Simon, Schusser, Gerald F., Abraham, Getu, Schrödl, Wieland

21 June 2016

Background: Horses are much predisposed and susceptible to excessive and acute inflammatory responses that cause the recruitment and stimulation of polymorphnuclear granulocytes (PMN) together with peripheral blood mononuclear cells (PBMC) and the release of cytokines. The aim of the study is to develop easy, quick, cheap and reproducible methods for measuring tumor necrosis factor alpha (TNF-α) and interleukin-1 receptor antagonist (IL-1Ra) in the equine whole blood cultures ex-vivo time- and concentration dependently. Results: Horse whole blood diluted to 10, 20 and 50 % was stimulated with lipopolysaccharide (LPS), PCPwL (a combination of phytohemagglutinin E, concanavalin A and pokeweed mitogen) or equine recombinant TNF-α (erTNF-α). TNF-α and IL-1Ra were analyzed in culture supernatants, which were collected at different time points using specific enzyme-linked immunosorbent assays (ELISA). Both cytokines could be detected optimal in stimulated 20 % whole blood cultures. TNF-α and IL-1Ra releases were time-dependent but the kinetic was different between them. PCPwL-induced TNF-α and IL-1Ra release was enhanced continuously over 24–48 h, respectively. Similarly, LPS-stimulated TNF-α was at maximum at time points between 8–12 h and started to decrease thereafter, whereas IL-1Ra peaked later between 12–24 h and rather continued to accumulate over 48 h. The equine recombinant TNF-α could induce also the IL-1Ra release. Conclusions: Our results demonstrate that similar to PCPwL, LPS stimulated TNF-α and IL-1Ra production time-dependently in whole blood cultures, suggesting the suitability of whole blood cultures to assess the release of a variety of cytokines in health and diseases of horse.

Pferd

TNF-alpha

Interleukin-1-Rezeptor-Antagonist

Enzyme-linked Immunosorbent Assay

Vollblut

Entzündung

horse

TNF-α

IL-1receptor antagonist

Whole blood culture

Inflammation

ddc:636

Influence d'un phosphate de calcium substitué en strontium sur la physiologie de l'ostéoblaste humain en culture et évaluation de son potentiel de réparation osseusse chez la souris / Strontium substituted calcium phosphate influence on human osteoblasts physiology and evaluation of his potential bone healing capability on a mouse model.

Braux, Julien

02 February 2011

Les phosphates de calcium sont des biomatériaux couramment utilisés dans de nombreuses spécialités médicales. L'amélioration de ces biomatériaux vise à augmenter leur ostéointégration et leur bioactivité. Le strontium possédant d'intéressantes capacités de modification de la physiologie osseuse, l'incorporation de ce dernier au sein de phosphates de calcium par substitution ionique pourrait permettre un déplacement de la balance osseuse vers la formation osseuse.Notre travail a permis de démontrer la capacité des particules de phosphates de calcium substitués en strontium à augmenter la prolifération des ostéoblastes en culture et à modifier l'expression et la synthèse des principales protéines impliquées dans la physiologie osseuse (Collagène de type I, Serpine H1, métalloprotéinases matricielles 1 et 2, inhibiteurs tissulaires des MMPs). Par ailleurs, la poudre de phosphates de calcium ne contenant pas de strontium a entrainé une sécrétion accrue de chimiokines pro-inflammatoires (MCP-1 et GRO-?) qui n'a pas été observée pour la poudre substituée. Enfin, des études in-vivo réalisées dans un modèle de défaut osseux murin a permis de démontrer une plus grande résorbabilité de la poudre contenant du strontium et sa plus grande capacité à stimuler la réparation osseuse. / Calcium phosphate are widely used in medicine. Their upgrade tend to enhance their biocompatibility and their bioactivity. Strontium has interesting capability to modify the bone physiologie. Its incorporation in calcium phosphates could lead to modify the bone balance toward osteogenesis.The present work reveal the capacities of such biomaterials to enhance the replication of osteoblasts ant to modify the expression and the synthesis of proteins implicated in the bone balance (type I collagen, serpinH1, Matrix metalloproteinases 1 and 2, tissular inhibitors of MMPs). Moreover, non substituted calcium phosphate powders enhance the expression and synthesis of inflammatory cytokines (MCP-1 and Gro-a). This fact was not observed with the non substituted powder. In-vivo studies on a mouse model permit us to demonstrate the higher resorbability and the higher bone healing capability of the substituted powder.

Os et tissu osseux

Metalloproteases

Souris de lignée C57BL

Collagène de type1

Strontium

Ostéoblastes

Phosphate de sodium

Matrix metalloproteinases

Test ELISA

Chimiokine CXCL1

Bone and bones

Metalloproteases

Mice, inbred c57bl

Collagen type I

Strontium

Osteoblasts

Sodium phosphate

Matrix metalloproteinases

Enzyme-Linked immunosorbent assay

Chemokine cxcl1

Electrochemical Immunosensor based on Cyclodextrin Supramolecular interactions for the detection of human chorionic gonadotropin

Wilson, Lindsay

January 2012

>Magister Scientiae - MSc / Glucose oxidase (GOx) and horseradish peroxidase (HRP) are important enzymes for the development of amperometric enzyme linked immunosensors. The selectivity of each enzyme towards its analyte deepens its importance in determining the sensitivity of the resultant immunosensor. In designing immunosensors that have customized transducer surfaces, the incorporation with FAD and iron based enzymes ensures that electron kinetics remains optimal for electrochemical measurement. Various different immobilization strategies are used to produce response signals directly proportional to the concentration of analyte with minimal interferences. The combination of self-assembled monolayers and supramolecular chemistry affords stability and simplicity in immunosensor design. In this work, two electrochemical strategies for the detection of human chorionic gonadotropin(hCG) is presented. This involves the modification of a gold surface with a thiolated β-cyclodextrin epichlorohydrin polymer (βCDPSH) to form a supramolecular inclusion complex with ferrocene (Fc)-functionalised carboxymethyl cellulose polymer (CMC). Cyclic voltammetry indicated that ferrocene is in close proximity to the electrode surface due to the supramolecular complex formed with βCDPSH. Furthermore, strategy (a) for the detection of hCG used α-antihCG labelled (HRP) as reporter conjugate. Strategy (b) maintained the CMC bifunctionalised with Fc and recognition antibody for hCG hormone. However, the system was functionalised with a HRP enzyme and detection is done by using GOx reporter conjugates for in situ production of hydrogen peroxide. The reduction of H2O2 was used for the amperometric detection of hCG by applying a potential of 200 mV. The sensitivity and limit of detection of both strategies were calculated from calibration plots. For strategy (a) the LOD was found to be 3.7283 ng/mL corresponding to 33.56 mIU/mL and a sensitivity of 0.0914 nA ng-1 mL-1. The corresponding values for strategy (b) are 700 pg/mL (6.3 mIU/mL) and 0.94 nA ng-1 mL-1.

Biosensor

Immunosensor

β-Cyclodextrin

β-Cyclodextrin epichlorohydrin polymer

Ferrocene

Carboxymethyl cellulose

Supramolecular

Host-guest

Self-assembled monolayers

Bienzymatic

Co-operative effect

Cyclic Voltammetry

Square Wave Voltammetry

Enzyme Linked Immunosorbent Assay

Amperometric

Human Chorionic Gonadotropin

Resposta imune celular a diferentes antígenos micobacterianos em indivíduos infectados por Mycobacterium tuberculosis: avaliação por elispot, elisa e linfoproliferação

Tanji, Maury Massani

02 March 2005

A tuberculose é uma doença crônica granulomatosa caracterizada por um déficit de imunidade antígeno específica do hospedeiro, cuja resposta imune é ativamente regulada por citocinas. No Brasil há mais de 50 milhões de habitantes infectados pelo Mycobacterium tuberculosis. O objetivo foi avaliar a linfoproliferação e a produção de citocinas por células mononucleares do sangue periférico (PBMC) estimuladas por quatro diferentes antígenos do M. tuberculosis, um complexo, o antígeno sonicado, e três purificados, ESAT-6, antígeno 85B e antígeno HBHA, eventuais candidatos à vacina anti-tuberculose. Para avaliação da produção de IFN-g e IL-10 foram utilizados dois métodos: Elispot e Elisa à partir de sobrenadante de cultura de PBMC. Para essas avaliações, os pacientes com tuberculose ativa (TB-A) foram comparados a dois subgrupos de indivíduos controles. O primeiro subgrupo foi constituído por indivíduos saudáveis PPD+ e o segundo por indivíduos curados de um episódio de tuberculose (TB-C). Nossos resultados de linfoproliferação e de Elisa revelaram diminuição da resposta linfoproliferativa e da produção de IFN-g dos pacientes em comparação com os indivíduos PPD+, enquanto os indivíduos TB-C apresentaram em geral resultados intermediários. Observou-se também que as respostas à PHA não diferiam significativamente entre os grupos, ressaltando a natureza antígeno específica da hiporreatividade na tuberculose. Adicionalmente, verificamos maior reatividade ao antígeno complexo, sonicado, que aos antígenos purificados, e entre estes, a reatividade foi maior para ESAT-6 e 85B que para HBHA, A resposta ao HBHA pode ter sido eventualmente subestimada por razões técnicas, como utilização de dose sub-ótima ou perda da atividade biológica. Em relação ao Elispot para IFN-g, não pudemos observar diferenças entre os grupos, tanto quando se considerou o número total de spots, como quando se contou apenas spots com diâmetro > 65 mm, apresentando portanto uma sensibilidade aparentemente menor comparado aos outros 2 métodos. A comparação entre os métodos revelou pouca correlação entre seus resultados, que pode ser eventualmente explicado pela diferente contribuição das populações celulares (T CD4+ e T CD8+) para cada uma das provas munológicas. Finalmente, a análise da produção de IL-10 medida por Elisa no sobrenadante de cultura e por spots de IL10, também não revelou diferenças entre os grupos. Convém notar que o Elisa detectou baixas concentrações de IL-10 nos sobrenadantes, porém o Elispot demonstrou número elevado de spots e boa correlação entre as resposta aos antígenos. Em conclusão, nossos resultados sugerem que métodos \'clássicos\', e já estabelecidos, como linfoproliferação e Elisa, persistem válidos para se avaliar a imunidade celular, e que em nossas condições laboratoriais, a técnica de Elispot não representou, até o momento, uma melhora na qualidade da avaliação imunológica. / Tuberculosis is a chronic granulomatous disease characterized by a deficit of the antigen-specific immunity of the host, whose immune response is actively regulated by cytokines. In Brazil there are 50 million people infected with Mycobacterium tuberculosis. The objective of the present work was to evaluate the lymphoproliferative response e the IFN-g response by peripheral blood mononuclear cells (PBMC) indiced with 4 different antigens isolated from Mycobacterium tuberculosis: a complex, crude, the sonicate antigen, and 3 other, purified ones, Esat-6, 85B, and HBHA, the last 3 eventual candidates to the design of a vaccine against tuberculosis. We used 2 methods to evaluate the IFN-g and IL-10 productions, namely Elispot and Elisa of supernatant of PBMC cultures. We studied a group of active tuberculosis patients (TB-A), and compared them with controls individuals comprising 2 groups, one made of healthy PPD+ individuals and the second one of individuals who have been cured from an episode of tuberculosis in the past (TB-C). Our results of lymphoproliferation and Elisa revealed decrease in the lymphoproliferative and IFN-g responses by patients\' PBMC as compared to the PPD+ group, with the TB-C group in general presenting intermediate results. We also observed that the responses to the mitogen PHA were not statisically different among the groups, denoting the antigen-specific nature of the immune deficit in tuberculosis. In addition, we verified that stronger reactivity to the complex antigen than with the purified antigens, and, among the latter, the reactivity was stronger with Esat-6 and 85B as compared to HBHA, Reactivity to HBHA may have been understimated due to technical reasons, such as loss of .the biological activity of the molecule or use of a sub-optimal dose. By using the Elispot for IFN-g we were not able to detect differences among the groups, even when we counted all spots formed or spots with more than > 65 mm in diameter. Thus our Elispot for IFN-g apparently showed lower sensitivity than the other 2 methods. Furthermore, comparisons between the methods revealed low correlation between their results, a finding that may be explained by the differning contribution of different subpopulations (T CD4+ and T CD8+) to each of the results. Finally, analysis of the production of IL-10 as measured by Elisa in the culture supernatants as well as by Elispot revealed no differences among the groups. It is noteworthy that the levels of IL-10 detected by Elisa were low, but the Elispot revealed high number of spots and a good correlation between the antigen responses. In conclusion, we may say that our well standardized \'classical\' methods Elisa and lymphoproliferation persist useful to evaluate cellular immunity responses, and that the Elispot technique, up to now and in our laboratorial conditions, did not represent an improvement in the quality of the immunological evaluation.

Citocinas/análise

Cytokines/analysis

Elisa/métodos

Interleucina-S/análise

Interleukin-5/analysis

Leucócitos mononucleares/imunologia

Leukocytes mononuclear/immunology

Micobacteriose/imunologia

Mycobacterium infections/immunology

Mycobacterium tuberculosis/immunology

Mycobacterium tuberculosis/imunologia

Tuberculose/imunologia

Tuberculosis/immunology