Replikation, Differenzierbarkeit und Proteinausstattung von Klonen chondrogener Progenitorzelllinien / Replication, differentiability, and protein equipment of clones of chondrogenic progenitor cell lines

Kizildere, Tolga Raoul

10 February 2014

Die progrediente, muskuloskelettale Erkrankung Ostheoarthrose wird aufgrund der immer älter werdenden Weltbevölkerung im Jahre 2020 einer der häufigsten Invaliditätsgründe sein. Koelling et al. beschrieb 2009 eine migrierende, chondrogene Progenitorzelllinie (CPC) im Reparaturgewebe der fortgeschrittenen Gonarthrose des Menschen, die Stammzelleigenschaften besitzt. Sie sind multipotent, klonal und besitzen ein osteochondrogenes Expressionsmuster, wodurch sie sich für neue Behandlungsmöglichkeiten bei der Ostheoarthrosetherapie eignen könnten. In dieser Arbeit wurden in vitro drei Klone einer humanen CPC-Population aus osteoarthrotisch verändertem Knorpel hinsichtlich ihrer multipotenten Eigenschaften, Proliferationsgeschwindigkeit und unterschiedlicher Phänotypen gegenübergestellt, da sich bei anderen Stammzelllinien Zusammenhänge zwischen diesen Eigenschaften zeigen, die mit fortgeschrittener Ausdifferenzierung der Stammzellen begründet wird. Die drei Klone IF-8, IIB-6 und IID-4 wurden 12 Tage unter Standardbedingungen in 2D-Flaschenkultur gehalten und anschließend ihr normaler Phänotyp ausgewertet. Dabei zeigte sich, dass IF-8 und IIB-6 eher einen fibroblastenartigen Phänotyp ausbildeten, während sich bei IID-4 erst kugelige Zellen bildeten, die später teils in eine längliche Form übergingen. Die fibroblastenartige Form entsprach der von CPCs aus heterogenen Kulturen, wohingegen der Phänotyp von IID-4 auf Dedifferenzierung oder fortgeschrittenere Differenzierung schließen ließ. Die Klone für die Differenzierungsversuche wurden mit zwei verschiedenen Zelldichten ausgesät, um auch eventuelle Einflüsse der Zelldichte mit in die Untersuchung einzubeziehen. Es wurde pro Well einmal die Anfangskonzentration von 1000 Zellen gewählt und einmal 3000 Zellen pro Well. Nach sechs Tagen wurden morphologische Veränderungen unter dem Mikroskop ausgewertet. Die Differenzierung in Adipozyten und Osteoblasten erfolgte insgesamt über zehn Tage mit anschließendem Differenzie- rungsnachweis mittels Oil-Red-Färbung von Adipozyten, bzw. der Alkalischen-Phosphatase-Reaktion der Osteoblasten. Es wurde zusätzlich mit der Immunfluoreszenzzytochemie kontrolliert, ob in den differenzierten Zellen auch spezifische Proteine exprimiert wurden und sich zwischen den Klonen ein quantitativer Unterschied ergibt, der auf einen veränderten Differenzierungsgrad der Klone schließen konnte. Für die Adipozyten wurden Antikörper gegen dieLipoproteinlipase und PPARγ gewählt, bei den Osteoblasten kamen Antikörper gegen Osteocalcin und den osteogenen Transkriptionsfaktor runx-2 zum Einsatz. Allen Differenzierungsversuchen wurden jeweils Kontrollgruppen gegenübergestellt. Die Ergebnisse zeigten morphologische Unterschiede zwischen den Klonen und den verschiedenen Zelldichten, die bei der osteogenen Differenzierung nicht so stark ausgeprägt waren wie bei der adipogenen. Der Klon-IID-4 zeigte auch hier die am Stärksten ausgeprägtesten morphologischen Unterschiede zwischen den Zellen selber und der verschiedenen Dichtegrade. Die quantitative Auswertung mittels Oil-Red und Alkalischer-Phosphatase, bzw. die Ergebnisse der Immunzytochemie ergaben hingegen keine Abweichungen zwischen den Klonen und keine Veränderung in Abhängigkeit zur Zelldichte. Dadurch konnte gezeigt werden, dass bei den CPCs ein veränderter Phänotyp kein Hinweis auf eine fortgeschrittene Zellalterung und verminderte Differenzierbarkeit ist. Auch die Zelldichte nimmt auf die Differenzierung in andere Zelllinien keinen positiven oder negativen Einfluss. Deutliche Unterschiede zwischen den Klonen zeigten sich hinsichtlich ihrer Proliferationsgeschwindigkeit und ihres osteochondrogenen Grundmusters. Für das Proliferationsassay wurden über den Zeitraum von sieben Tagen die Zellzahlen gemessen. Dabei wurde festgestellt, dass sich Klon-IF-8 am langsamsten teilte, danach folgte IID-4 und am Ende IIB-6. Im Zusammenhang mit dem Western-Blot, bei dem der osteogene Transkriptionsfaktor runx-2 und der chondrogene Transkrip-tionsfaktor sox-9 miteinander verglichen wurden, konnte eine Beziehung zwischen Proliferationsgeschwindigkeit und der Ausprägung der Transkriptionsfaktoren festgestellt werden. Mit Abnahme der Proliferationsgeschwindigkeit nimmt die Expression von runx-2 zu, während die Expression von sox-9 abnimmt. Dadurch konnte nachgewiesen werden, dass die CPCs mit abnehmender Zellteilung in einen vermehrt osteogenen Zustand übergehen und ihren osteochondrogenen Charakter verlieren. Dieser Übergang hat jedoch keinen Einfluss auf ihre multipotenten Eigenschaften. Mit den Ergebnissen konnte gezeigt werden, dass sich CPCs, ähnlich wie andere Progenitorzellen auch, in ihrer Entwicklung weiter ausdifferenzieren und sich dadurch innerhalb einer Population verschiedene Entwicklungszustände ergeben, die eine genauere Charakterisierung der CPCs weiter erschweren.

610

chondrogene Progenitorzellen

Klone

Knorpel

Osteoarthrose

Stammzellen

Stammzell-Differenzierung

chondrogenic progenitor cell line,

cartilage

osteoarthritis

stem cell

stem cell differentiation

Medizin (PPN619874732)

Biochemical, Cytotoxic And Genotoxic Effects Of Aescin On Human Lymphocytes And Hl-60 Promyeloid Leukemia Cell Line

Topsoy Kolukisa, Serap

01 July 2005

Aescin is a mixture of several acidic triterpenoid saponin glycosides found in the extracts of the horse chestnut tree. Horse chestnut, Aesculus Hipoocastanum, is one of the 25 domestic species of Aesculus that are mostly large, ornamental shade trees. Although known to be poisonous, the nuts of the horse chestnut are used by Amerindians, after detoxification. Horse chestnuts are said to have several traditional medicinal usages including even cancer. In this study the biochemical, genotoxic, and cytotoxic effects of aescin was studied using isolated lymphocytes, whole blood lymphocytes and HL-60 promyeloid leukemia cell lines. Cytotoxicity of aescin was examined by trypan blue viability staining of the cells in culture treated with varying aescin concentrations. It was observed that aescin was cytotoxic at all concentrations, for all cell types studied, except whole blood lymphocytes, where it was not cytotoxic at 10-9 and 10-10 M concentrations. Genotoxicity of aescin was examined by sister chromatid exchange and micronucleus. The genotoxic effect of Aescin was observed to be more significant over isolated lymphocytes compared to other cell lines. On the otherhand, aescin at 10-8 M and lower concentrations were observed to be non-genotoxic over whole blood lymphocytes whereas this concentration was considerably toxic for isolated lymphocytes and for HL-60 cell lines. Apoptotic properties of aescin were determined by DNA fragmentation, cytochrome c release and negative NAPO staining. All the Aescin concentrations tested resulted in apoptosis over HL-60 cell lines, whereas necrosis was not observed. However, isolated lymphocytes showed both apoptosis and necrosis upon treatment with 10-6 M to 10-8 M aescin, exhibiting apoptosis only at 10-9 M and 10-10 M. Biochemical effects of aescin were investigated by following GST and NAT enzyme activities. An increase in GST enzyme activity was observed over all cell lines treated with increasing aescin concentrations for 72 hours. Whereas NAT activity was decreased upon treatment with aescin in similar manner.

QH General Biology 301-705

Src kinase inhibitors for the treatment of sarcomas : cellular and molecular mechanisms of action

Shor, Audrey Cathryn.

January 2007

Dissertation (Ph.D.)--University of South Florida, 2007. / Title from PDF of title page. Document formatted into pages; contains 192 pages. Includes vita. Includes bibliographical references.

Characterization of the dopaminergic potential of the human NTera2/d1 (NT2) cell line in vitro /

Misiuta, Iwona E.

January 2005

Thesis (Ph.D.)--University of South Florida, 2005. / Includes vita. Includes bibliographical references. Also available online.

The immortalization process of T cells with focus on the regulation of telomere length and telomerase activity /

Degerman, Sofie,

January 2010

Diss. (sammanfattning) Umeå : Umeå universitet, 2010.

Expressão da quimiocina SDF-1, (CXCL12) e seu respectivo receptor CXCR4  em células de pacientes com mieloma múltiplo em linhagem de células mieloma múltiplo humano (RPMI-8226) após tratamento com talidomida / Expression of the chemokine SDF-1 and its receptor CXCR4 in the cells of patients with multiple myeloma and line cell of the multiple myeloma after treatment of thalidomide

Adriana Morgan de Oliveira

27 August 2008

Mieloma Múltiplo é a segunda doença com maior prevalência nas doenças malignidades hematológica, incurável com média de sobrevivência de 3-5 anos. MM é uma malignidade das células do plasma caracterizada pela destruição e reabsorção óssea e supressão da formação do osso. A quimiocina SDF-1 (CXCL12) e seu receptor CXCR4 têm um importante papel direcional na migração, homing das células do plasma em mieloma múltiplo e mobilização das células de MM para fora da medula óssea. A talidomida tem sido usada com êxito no tratamento de pacientes com mieloma múltiplo. Neste estudo verificamos o efeito da talidomida na expressão da quimiocina SDF-1 e seu receptor CXCR4 em pacientes com mieloma múltiplo e em linhagem de células de mieloma múltiplo humano (RPMI-8226) tratados e sem tratamento de talidomida. Nossos resultamos mostraram uma expressão heterogênea na expressão da quimiocina SDF-1 e seu receptor CXCR4 nos pacientes com mieloma múltiplo estudado (n= 79). Entretanto, pacientes com mieloma múltiplo tratados com talidomida mostraram uma baixa expressão da quimiocina SDF-1 e seu receptor CXC4 quando comparados com pacientes recém diagnosticados para mieloma múltiplo e pacientes com mieloma múltiplo tratados com outros medicamentos. Nossos resultados sugerem que o tratamento com talidomida induz uma baixa regulação na expressão no ligante SDF-1 e seu receptor CXCR4 em pacientes com mieloma múltiplo / Multiple Myeloma (MM) is a second most prevalent hematological malignancy and remains incurable with a median survival of 3-5 years. MM is a plasma cell malignancy characterized by devastating bone destruction due to the enhanced bone resorption and suppressed bone formation. The chemokine stromal-derived factor-1 (SDF-1) and its receptor CXCR4 play an important role in directional migration, homing of plasma cells in multiple myeloma (MM) and mobilization of MM cells out of the bone marrow. The drug thalidomide has been successfully used in the treatment of patients with MM. In this study, we assessed the effect of thalidomide on SDF-1 and CXCR4 expression in MM patients and human myeloma-derived cell line, RPMI 8226 treated with or without thalidomide. A heterogeneous expression pattern of chemokines SDF-1 and CXCR4 receptor were observed for all MM patients studied. However, patients treated with thalidomide showed a significantly decrease in expression of SDF-1 and CXCR4 as compared to newly diagnosed MM patients and MM patients treated with other drugs. RPMI 8226 cell line treated with 10, 20 and 100µM thalidomide also demonstrated decrease in SDF-1 and CXCR4 expression as compared with cell control (RPMI-8226 without thalidomide). Ours results indicate that thalidomide therapy induces down-regulation of CXCR4 and its ligand SDF-1 in multiple myeloma

Linhagem de células RPMI-8226

Mieloma múltiplo

Quimiocinas SDF-1/ CXCR4

Talidomida

Chemokine SDF-1 and CXCR4 receptor

Multiple myeloma

RPMI-8226 cell line

Thalidomide

Avaliação da ação antitumoral in vitro da pterocarpanoquinona LQB 118 e estudo de alguns mecanismos de ação / Evaluation of antitumor action in vitro of the Pterocarpanoquinone LQB 118 and study of some mechanisms of action

Thiago Martino Martins

07 March 2013

Conselho Nacional de Desenvolvimento Científico e Tecnológico / Tem sido descrito que o acúmulo de mutações em proto-oncogenes e genes supressores de tumor contribui para o direcionamento da célula à carcinogênese. Na maioria dos casos de câncer, as células apresentam proliferação descontrolada devido a alterações na expressão e/ou mutações de ciclinas, quinases dependentes de ciclinas e/ou inibidores do ciclo celular. Os tumores sólidos figuram entre o tipo de câncer mais incidente no mundo, sendo a quimioterapia e/ou hormônio-terapia, radioterapia e cirurgia os tratamentos mais indicados para estes tipos de tumores. Entretanto, o tratamento quimioterápico apresenta diversos efeitos colaterais e muitas vezes é ineficaz. Portanto, a busca por novas moléculas capazes de conter a proliferação destas células e com baixa toxicidade para o organismo se faz necessário. Este trabalho teve por objetivo avaliar a ação antitumoral in vitro de um novo composto sintético, a pterocarpanoquinona LQB118, sobre algumas linhagens tumorais humanas de alta prevalência e estudar alguns dos seus mecanismos de ação. As linhagens tumorais estudadas neste trabalho foram os adenocarcinomas de mama (MCF7) e próstata (PC-3), e carcinoma de pulmão (A549). A citotoxicidade foi avaliada pelo ensaio do MTT e a proliferação celular pela contagem de células vivas (exclusão do corante azul de tripan) e análise do ciclo celular (citometria de fluxo). A expressão gênica foi avaliada por RT-PCR e a apoptose foi avaliada por condensação da cromatina (microscopia de fluorescência-DAPI), fragmentação de DNA (eletroforese) e marcação com anexina V (citometria de fluxo). Das linhagens tumorais testadas, a de próstata (PC3) foi a que se mostrou mais sensível ao LQB 118, e em função deste resultado, os demais experimentos foram realizados com esta linhagem tumoral. O efeito citotóxico do LQB 118 se mostrou tempo e concentração dependente. Esta substância inibiu a proliferação celular e prejudicou a progressão do ciclo celular, acumulando células nas fases S e G2/M. Buscando esclarecer os mecanismos desta ação antitumoral, demonstrou-se que o LQB 118 inibe a expressão do mRNA do fator de transcrição c-Myc e das ciclinas D1 e B1, e induz a apoptose de tais células tumorais. Em suma, o LQB 118 é capaz de inibir a proliferação das células tumorais de próstata, alterando a expressão do mRNA de alguns genes reguladores do ciclo celular, resultando em interrupção do ciclo celular e indução de apoptose, indicando este composto como um potencial candidato a futuro medicamento no tratamento do câncer de próstata. / It has been reported that accumulation of mutation on proto-oncogenes and tumor suppressor genes directs cells to carcinogenesis. In most described cancer, cells display uncontrolled proliferation due to altered expression or mutations of cyclins, cyclin-dependent kinases and cell cycle inhibitors. The solid tumors are the most common cancer type in world. Chemotherapy and/or hormone-therapy, radiotherapy and surgery are the suitable treatment for this disease. However, chemotherapy has been shown several side effects and often ineffective. Therefore, the search for new molecules with antitumoral activity low cytotoxicity is needed. The aim of this work was to evaluate the in vitro antitumoral effects of a new synthetic compound, the pterocarpanquinone LQB 118, on tumor cell lines of high prevalence in the world and to study some mechanisms of action. Tumor cell lines of breast (MCF7), lung (A549) and prostate (PC3) were cultivated at RPMI medium with 10% of serum fetal bovine. The cytotoxicity was evaluated by MTT assay and the cell proliferation by cell counting (trypan blue exclusion) and cell cycle analysis (flow cytometry). Apoptosis was evaluated by chromatin condensation (fluorescence microscopy with DAPI), DNA fragmentation (electrophoresis) and annexin-V and iodide propidium staining. Gene expression was studied by RT-PCR. As LQB 118 (5 g/ml) induced cytotoxic effect mainly on prostate tumor cells, further experiments were then performed only with this tumor cell line. The LQB 118 cytotoxic effects were time and concentration-dependent. Furthermore, this substance inhibited cell proliferation and promoted cell cycle arrest, increasing cell number in S and G2/M phases. Studying the mechanisms of the LQB 118 antitumoral action, it was demonstrated that this substance inhibited the mRNA expression of the transcription factor c-Myc, cyclin D1 and cyclin B1 and also induced apoptosis of PC3. Concluding, LQB 118 impairs prostate tumor cells proliferation due to altered mRNA expression of some cell cycle regulator genes, resulting in cell cycle arrest and apoptosis induction, suggesting this compound as a good candidate for a future drug in prostate cancer treatment.

Pterocarpanoquinona LQB 118

Apoptose

Ciclo cellular

Pterocarpanquinone LQB 118

Apoptosis

Cell cycle

Prostate cancer and cell line PC3

BIOQUIMICA

Substituição gênica ortotópica de porco para humano baseada em CRISPR/Cas9 e recombinases para xenotransplante / CRISPR/Cas9 and recombinase based pig-to-human orthotopic gene exchange for xenotransplantation

Rafael Miyashiro Nunes dos Santos

11 August 2017

Modelos humanizados de porco são muito importantes para pesquisa biomédica e desenvolvimento de novas drogas e tratamentos. Além de ser um melhor modelo para doenças humanas do que animais de menor porte devido sua maior semelhança fisiológica, anatômica, de metabolismo e tempo de vida, o modelo suíno ainda permite suprimento ilimitado de órgãos para transplante. Apesar dessas vantagens, a expressão gênica inconsistente de animais transgênicos tornam a criação e avaliação desses animais muito dispendiosas, imprevisível e não permite a comparação de resultados de animais diferentes de maneira apropriada. Nesse estudo descrevemos uma nova técnica utilizando o promoter endógeno para a geração de um protocolo de substituição de genes com padrão clonal (transplante clonal de genes) sem clonagem de células, preservando a expressão genética e sua regulação intactas. Esse protocolo é reprodutível e pode ser aplicado para mais de um alvo genético, permitindo geração rápida de linhas transgênicas de animais (14-20 dias) com potencial de se tornar o novo padrão para geração de animais transgênicos de grande porte Suínos / Humanized pig models are very important for biomedical research, and drugs and treatment development. Not only it is a better model for diseases than smaller animals because of its closer physiology, anatomy, metabolism and life span, it also may provide unlimited organs for transplantation. In spite of all this advantages, inconsistent gene expression in transgenic animals make its generation and evaluation expensive, unpredictable and do not allow proper outcome comparison between different animals. In this report we describe a reproducible technique utilizing the endogenous promoter for generation of a clonal pattern gene replacement protocol (clonal gene transplant) without cell cloning, maintaining the normal gene expression and its regulation. This protocol is reproducible and applicable to more than one gene target, allowing fast generation of transgenic animals cell lines (as low as 14-20 days) and could become the new standard for transgenic large animal generation

Linhagem celular

Sistemas CRISPRCas

Técnicas de transferência de genes

Transfecção

Transplante heterólogo

Trombomodulina

Cell line

CRISPR-Cas systems

Gene transfer techniques

Thrombomodulin

Transfection swine

Transplantation heterologous

Propriedades citotóxicas da Beta-Lapachona em células de osteossarcoma in vitro / Citotoxic properties of β lapachone in osteosarcoma cells cultured in vitro

Gabriel, Gabriela Hadler

09 March 2017

Submitted by JÚLIO HEBER SILVA (julioheber@yahoo.com.br) on 2017-04-13T17:22:48Z No. of bitstreams: 2 Dissertação - Gabriela Hadler Gabriel - 2017.pdf: 1069284 bytes, checksum: 7c190e383bf6069f54d2eff26158427f (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) / Approved for entry into archive by Luciana Ferreira (lucgeral@gmail.com) on 2017-04-17T11:13:33Z (GMT) No. of bitstreams: 2 Dissertação - Gabriela Hadler Gabriel - 2017.pdf: 1069284 bytes, checksum: 7c190e383bf6069f54d2eff26158427f (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) / Made available in DSpace on 2017-04-17T11:13:33Z (GMT). No. of bitstreams: 2 Dissertação - Gabriela Hadler Gabriel - 2017.pdf: 1069284 bytes, checksum: 7c190e383bf6069f54d2eff26158427f (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) Previous issue date: 2017-03-09 / Conselho Nacional de Pesquisa e Desenvolvimento Científico e Tecnológico - CNPq / Osteosarcoma is the main primary bone tumor, with unfavorable prognosis, high mortality and high incidence of metastases. The treatment of choice is the removal of the tumor associated with combined chemotherapy, whose adverse effects allude to the increasing need to develop new drugs. The plants constitute a large natural reserve of compounds that have medicinal and therapeutic properties, such as lapachol and its derivative, β-lapachone. The aim of this study was to evaluate the cytotoxic effects of β-lapachone in osteosarcoma cells cultured in vitro. Cells were cultured and treated with β-lapachone at different concentrations and times of exposure. Tripan blue exclusion, tetrazolium reduction and cell survival assay methods were performed to evaluate the effects of the compound on the cells. Cells treated with 0,1μM β-lapachone showed lower initial cytotoxicity in the 24h time, whereas those submitted to 1,0μM showed less viability after 72h of treatment. Cytotoxicity increased as the concentration and time of exposure increased. The lowest IC50 (0,148μM) was observed in treated cells for 72h. Cell growth after treatment was lower in the 1.0μl group after 72h and the highest cell growth was observed under a concentration of 0.1μl after 24h. There was no difference between groups for cell proliferation after treatment, and the cell survival fraction was lower after 72h of exposure. It was concluded that β-lapachone has cytotoxic effects on osteosarcoma cells cultured in vitro. / O osteossarcoma é o principal tumor ósseo primário, com prognóstico desfavorável, alta mortalidade e elevada incidência de metástases. O tratamento de escolha é remoção do tumor associada à quimioterapia combinada, cujos efeitos adversos aludem à necessidade crescente de desenvolver novos medicamentos. As plantas constituem grandes reservas naturais de compostos que possuem propriedades medicinais e terapêuticas, como o lapachol e seu derivado, a β lapachona. O objetivo desse estudo foi avaliar os efeitos citotóxicos da β lapachona em células de osteossarcoma cultivadas in vitro. As células foram cultivadas e tratadas com a β lapachona em diferentes concentrações e tempos de exposição. Foram realizados os métodos de exclusão com azul de Tripan, redução do tetrazólio e ensaio de sobrevivência celular para avaliar os efeitos do composto sobre as células. As células tratadas com 0,1μM de β lapachona apresentaram menor citotoxicidade inicial, no tempo de 24h, enquanto aquelas submetidas a 1,0μM apresentaram menor viabilidade após 72h de tratamento. A citotoxicidade aumentou de acordo com o aumento da concentração e tempo de exposição. O menor IC50 (0,148μM) foi observado nas células tratadas por 72h. O crescimento celular após o tratamento foi menor grupo sob concentração de 1,0µl após 72h e o maior crescimento celular foi observado sob concentração de 0,1µl após 24h. Não houve diferença entre grupos quanto à proliferação celular após o tratamento tendo a fração de sobrevivência das células sido menor após 72h de exposição. Concluiu-se que β lapachona apresenta efeitos citotóxicos em células de osteossarcoma cultivadas in vitro.

Cultivo celular

Linhagem MG-63

Naftoquinona

Neoplasia óssea

Bone tumor

Cell culture

MG-63 cell line

Naphthoquinone

MEDICINA VETERINARIA::PATOLOGIA ANIMAL

Sistema lipossomal de ftalocianina de cloro-alumínio, contendo ácido fólico, aplicada à terapia fotodinâmica / Chloro-aluminum phthalocyanine liposomal system, containing folic acid, applied to photodynamic therapy

Camila Vizentini Silva

20 August 2013

A Terapia Fotodinâmica (TFD) é um tratamento usado principalmente na terapia anticâncer e que depende da retenção de um composto fotossensibilizante nas células tumorais e posterior irradiação dessas células com luz visível. Após ativação, o fármaco pode gerar espécies reativas de oxigênio (EROs), como o oxigênio singlete (1O2) e radicais (O2-, OH), que são capazes de danificar membranas, DNA e outras estruturas celulares, induzindo a apoptose ou necrose das células tumorais. O ácido fólico, por ser super expressado na superfície das células de alguns tipos de cânceres (principalmente os ginecológicos), pode desempenhar o papel de vetorizador, tornando-se um importante aliado aos sistemas de liberação de fármacos. Neste trabalho foi avaliado o uso de ácido fólico como aditivo aos lipossomas contendo ftalocianina de cloro-alumínio como fármaco fotossensibilizante, aplicados em TFD com células MCF7. Os estudos demonstraram que os sistemas lipossomais desenvolvidos apresentam tamanho nanométrico (menor que 200 nm) e possuem biocompatibilidade quando avaliados em cultura celular de monocamada. Além disso, foi possível observar o efeito fototóxico satisfatório das formulações e o aumento da internalização do fármaco, quando utilizado o ácido fólico como vetorizador. / Photodynamic Therapy (PDT) is mainly used in anticancer therapy. The efficiency of this treatment is dependent on retention of photosensitizer compound at the tumor cells and posterior irradiation of these cells with visible light. After activation, the drug may generate reactive oxygen species (ROS) such as singlet oxygen (1O2) and radicals (O2-, OH), which are capable of damaging membranes, DNA and other cell structures, inducing apoptosis or necrosis of tumor cells. Folic acid is super-expressed on the surface of some cancers cells (especially gynecological cancer cells) and can play the role of target system, becoming an important ally for drug delivery systems. This study evaluated the use of folic acid as an additive to liposomes containing chloro-aluminum phthalocyanine as a photosensitizer drug, applied in PDT with MCF7 cells. These studies showed that liposomal systems have nanometer size (less than 200 nm) and have biocompatibility when evaluated in monolayer cell culture. Moreover, it was possible to observe satisfactory phototoxic effect of the formulations and increased internalization of the drug when folic acid is used.

ácido fólico

câncer de mama

células MCF7

ftalocianina de cloro-alumínio

lipossoma

Terapia Fotodinâmica

breast cancer

cell line MCF7

chloro-aluminum phthalocyanine

folic acid

liposome

Photodynamic Therapy