Análise da expressão gênica por microarrays de células-tronco hematopoéticas e mesenquimais de pacientes com esclerose múltipla / Gene expression profiles of hematopoietic stem cells and mesenchymal stromal cells obtained from multiple sclerosis patients and detected by microarrays.

Gislane Lelis Vilela de Oliveira

22 February 2013

As células-tronco hematopoéticas (CTHs) e estromais mesenquimais multipotentes (CTMs) isoladas da medula óssea vêm sendo utilizadas como fonte autóloga no tratamento de doenças autoimunes, como a esclerose múltipla (EM). As CTHs dão origem a todas as células dos sistemas hematopoético e imunológico e as CTMs possuem propriedades imunomoduladoras pela liberação de fatores solúveis e interação célula-célula. Existem trabalhos que sugerem que as doenças autoimunes sejam provenientes de defeitos intrínsecos nas células-tronco precursoras da medula óssea. Com o intuito de avaliar se as CTHs e CTMs de pacientes com EM possuem alterações intrínsecas, o objetivo geral deste trabalho foi avaliar o perfil de expressão gênica diferencial por microarrays de CTHs e CTMs de pacientes com EM, além de avaliar o perfil de expressão gênica de CTMs após o transplante autólogo de CTHs e a capacidade imunomoduladora in vitro das CTMs de pacientes. As CTHs e CTMs foram isoladas da medula óssea de pacientes com EM e doadores saudáveis, após consentimento informado. As CTHs foram isoladas por colunas imunomagnéticas e as CTMs foram isoladas por gradiente de densidade e submetidas à caracterização morfológica, imunofenotípica e capacidade de diferenciação em adipócitos e osteócitos. O RNA das CTHs e CTMs foi extraído e purificado e o perfil de expressão gênica foi avaliado por microarrays, utilizando hibridações em lâminas contendo 44.000 sondas. A capacidade imunomoduladora das CTMs de pacientes e controles foi avaliada por ensaios de cocultivo com linfócitos alogênicos e as citocinas foram quantificadas no sobrenadante por CBA flex e ELISA. Este estudo foi aprovado pelo comitê de ética do Hospital das Clínicas da Faculdade de Medicina de Ribeirão Preto. Os resultados mostraram que as CTHs de pacientes possuem perfis de expressão gênica diferentes dos controles, com 2.722 genes diferencialmente expressos, envolvidos em vias de sinalização importantes para manutenção/proliferação das CTHs e diferenciação em linhagens específicas durante a hematopoese. Dentre essas sinalizações estão incluídas as vias da apoptose, Wnt, Notch, mTOR, PI3K/Akt e Ca/NFAT, sugerindo que as CTHs de pacientes com EM possuam alterações intrínsecas que podem estar relacionadas com a patogenia da doença autoimune. As CTMs isoladas de pacientes com EM exibiram aparência senescente e reduzida expressão de marcadores imunofenotípicos. Com relação à expressão gênica, as CTMs de pacientes possuem perfil diferente das CTMs controle, sendo detectados 618 genes diferencialmente expressos, incluindo genes relacionados à sinalização FGF, HGF, sinalização de moléculas de adesão e moléculas envolvidas nos processos de imunorregulação, como IL10, IL6, TGFB1, IFNGR1, IFNGR2 e HGF. O perfil de expressão gênica das CTMs de pacientes pós-transplante assemelhou-se ao perfil das CTMs pré-transplante. Ensaios de cocultivo de CTMs com linfócitos alogênicos mostraram que as CTMs de pacientes possuem capacidade antiproliferativa reduzida em relação às CTMs controle, e ainda, secreção reduzida de TGF- e IL-10 no sobrenadante das coculturas. Esses dados sugerem que as CTMs isoladas de pacientes com EM possuam alterações fenotípicas, transcricionais e funcionais. Embasados nesses achados, concluímos que as CTHs e as CTMs de pacientes com EM possuem alterações intrínsecas que podem estar relacionadas com a patogenia da doença. Uma vez que as CTMs sejam células com grande potencial terapêutico para controle da EM em pacientes refratários aos tratamentos convencionais, as alterações encontradas sugerem que CTMs de doadores saudáveis sejam mais adequadas em aplicações clínicas. / Bone marrow hematopoietic stem cells (HSCs) and mesenchymal stromal cells (MSCs) have been used as an autologous source to treat autoimmune diseases, such as multiple sclerosis (MS). HSC give rise to all hematopoietic and immune system cells, and MSCs exhibit immunomodulatory properties by releasing soluble factors and by cell-cell interactions. Evidence indicates that bone marrow stem cells obtained from patients with autoimmune diseases may present intrinsic defects. To assess whether or not HSC and MSC of MS patients have intrinsic defects, the main objective of this study was to evaluate the differential gene expression profiles of HSC and MSC from MS patients before and after autologous HSC transplantation, and additionally, to evaluate the in vitro immunomodulatory ability of patient MSCs. Bone marrow HSC and MSCs were isolated from MS patients and healthy donors. HSCs were isolated by immunomagnetic columns and MSCs were isolated by gradient density and cultured until the third passage. MSCs were characterized according to morphology, immunophenotypic markers and cell differentiation into adipocytes and osteocytes. HSC and MSCs mRNAs were extracted, purified, and the gene expression profile was evaluated by microarray hybridizations, using a platform containing 44.000 probes. The immunomodulatory activity of patient and control MSCs was assessed by coculture assays with allogeneic lymphocytes. Cytokines were quantified in coculture supernatants by ELISA and CBA flex. This study was approved by the Ethics Committee of the University Hospital of the School of Medicine of Ribeirão Preto. The results showed that the patient HSCs exhibited a distinctive gene expression profile when compared to healthy HSCs, yielding 2.722 differentially expressed genes, involved in essential HSC signaling pathways for maintenance, proliferation and differentiation into specific lineages during hematopoiesis. Among these signaling pathways were included, apoptosis, Wnt, Notch, mTOR, PI3K/Akt and Ca/NFAT, suggesting that patient HSCs have significant intrinsic transcriptional alterations that may be associated with MS pathogenesis. Regarding MSCs isolated from MS patients, they exhibited senescence appearance, decreased expression of immunophenotypic markers, and also exhibited a distinctive gene expression profile in relation to healthy MSCs, yielding 618 genes differentially expressed genes, included in FGF and HGF signaling pathways, adhesion molecules, and genes involved in immunoregulation processes, such as IL-10, IL-6, TGFB1, IFNGR1, IFNGR2 and HGF. Coculture assays of control or patient MSCs with allogeneic lymphocytes showed that patient cells exhibited reduced antiproliferative activity as compared with controls, and also exhibited reduced secretion of TGF- and IL-10 cytokines in coculture supernatants. These data suggest that MSCs isolated from MS patients have phenotypic, functional and transcriptional defects, highlighting genes related to MSC maintenance, adhesion and immunomodulatory effects. According to these results, we concluded that patient HSCs and MSCs have intrinsic defects that may be associated with the disease per se. Considering that MSCs exhibit great therapeutic potential to control MS patients refractory to conventional treatment, the major MSCs alterations observed in this study indicate that healthy MSCs may be more suitable for MS cell therapy.

células-tronco hematopoéticas

doenças autoimunes

esclerose múltipla

expressão gênica diferencial

autoimmune diseases

differential gene expression profile

hematopoietic stem cells

multiple sclerosis

multipotent mesenchymal stromal cells

Avaliação dos efeitos da sinvastatina via Inibidor do Ativador do Plasminogênio 1 (PAI-1) sobre a terapia celular com células estromais mesenquimais / Evaluation of the effects of simvastatin in mesenchymal stromal cell therapy through Plasminogen Activator inhibitor 1 (PAI-1)

Carolina Arruda de Faria

08 August 2016

A Doença Pulmonar Obstrutiva Crônica (DPOC) é caracterizada pela limitação persistente de trocas gasosas, usualmente progressiva e associada a uma resposta inflamatória crônica exacerbada das vias aéreas a partículas e gases nocivos. Apesar de prevenível e tratável, não se logrou até o presente uma terapêutica eficaz, que resulte na cura da doença. Neste cenário, a terapia celular apresenta-se como uma alternativa terapêutica potencialmente promissora em DPOC, bem como em outras doenças pulmonares degenerativas e de caráter inflamatório. Porém, vários aspectos da terapia celular carecem de um melhor entendimento. Um dos principais desafios ao sucesso da terapia celular são as baixas taxas de sobrevivência das células transplantadas. O Inibidor do Ativador de Plasminogênio 1 (Plasminogen Activator Inhibitor 1 - PAI-1) pode representar um potencial mediador da sobrevivência de células estromais mesenquimais (CTM) pós-transplante, pois tem sido proposto que anticorpos neutralizadores do PAI-1 auxiliam no aumento da sobrevivência de CTM no tecido-alvo da terapia celular. Desta forma, a diminuição dos níveis de PAI-1 possui um potencial terapêutico interessante, ao modular os principais processos envolvidos na criação de um ambiente pouco propício ao \"homing\" celular durante o processo de injúria. A diminuição dos níveis de PAI-1 é promovida, pela sinvastatina, fármaco da família das estatinas. Desta forma, objetivou-se com este trabalho analisar os efeitos da sinvastatina sobre a expressão do PAI-1, bem como sua influência na sobrevivência das células infundidas para terapia celular de enfisema pulmonar em modelo murino. Camundongos da linhagem FVB foram submetidos à instilação intranasal de elastase para indução de enfisema pulmonar e, posteriormente, tratados com CTM do tecido adiposo e sinvastatina. Os resultados mostraram que, quanto aos aspectos morfológicos e funcionais, considerando-se a análise conjunta de ambos os pulmões, não houve diferença estatisticamente significativa entre os grupos submetidos à instilação intranasal de elastase e submetidos à terapia celular com CTM tratados ou não com sinvastatina. Quando porém os pulmões foram analisados individualmente constatou-se que não houve diferença estatisticamente significativa entre os grupos controle e os resultados referentes ao lado direito do pulmão dos animais tratados com elastase e que receberam sinvastatina e infusão de CTM. Diferenças anatômicas entre os lados direito e esquerdo do pulmão, levaram a uma maior deposição de células no lado direito, como evidenciado pelos resultados obtidos nos ensaios de bioluminescência. Pode-se, portanto, inferir que a recuperação morfológica no lado direito do pulmão de animais com DPOC/enfisema poderia ser decorrente de um efeito regenerativo parácrino das CTM associadas à sinvastatina. / Chronic Obstructive Pulmonary Disease - COPD is characterized by the persistent limitation of gas exchange, is usually progressive, and associated to a chronic augmented inflammatory response of the airways to particles and noxious gases. Despite preventable e treatable, an effective, curative therapeutic approach is yet to be achieved. In this context, cell therapy presents itself as a promising therapeutic approach for COPD and other pulmonary inflammatory and degenerative diseases. However, many aspects of cell therapy with stem cells remain unclear. One of the major challenges to the success of cell therapy are the low survival rates of transplanted cells. The Plasminogen Activator Inhibitor 1 (PAI-1) is a potential mediator of the survival of mesenchymal stromal cells (MSC) after transplantation, since PAI-1 neutralizing antibodies have been shown to increase the survival rate of MSC in the target tissue of cell therapy. Thus, the decreased levels of PAI-1 has an interesting therapeutic potential to modulate key processes involved in creating an inhospitable environment, during the process of injury, to the homing of transplanted cells. Decreased levels of PAI-1 are promoted by simvastatin, a drug of the statins family. Thus, the goal of this work was to evaluate the effect of simvastatin in vivo on the expression of PAI-1, as well as its influence on the survival rate of infused cells in mice model of cell therapy for pulmonary COPD/emphysema. FVB mice were submitted pulmonary emphysema induction by means of intranasal instillation of elastase and than treated with adipose-derived mesenchymal stem cells and simvastatin. The results regarding morphological and functional aspects, when considering the analisys of both lungs, presented no statistically significant difference among the groups submitted to intranasal instillation of elastase and cell therapy with MSC, treated or not with simvastatin. However, when the lungs where analyzed individually, it was found that there was no statistically significant difference between the control group and the results regarding the right lung of animals treated with elastase and that received simvastatin and MSC infusion. Anatomical differences between the right and left sides of the lung lead to a higher deposition of cells in the right side, as observed in the bioluminescence assays. Thus, it is possible to infer that the morphological recovery in the right side of the lung of animals with DPOC/emphysema could be due to a regenerative paracrine effect of mesenchymal stem cells associated with simvastatin.

Plaminogen activator inhibitor 1 - PAI-1

Perfil transcricional de fibroblastos de tumor primário, linfonodo e medula óssea de pacientes com câncer de mama / Transcriptional profile of fibroblasts obtained from primary tumor, lymph node and bone marrow of breast cancer patients

Paulo Roberto Del Valle

01 March 2013

Introdução: Em câncer de mama, existem evidências de que o microambiente pode influenciar o desenvolvimento do tumor no sítio primário, bem como em metástases regionais e a distância. Neste contexto, fibroblastos são importantes células estromais que podem influenciar a proliferação e a migração de células do câncer e podem prover um nicho apropriado para o desenvolvimento tumoral. Objetivos:O principal objetivo deste trabalho é comparar células estromais obtidas do tumor primário (PT), metástase linfonodal (N+) e medula óssea (BM) de pacientes com câncer de mama, através do perfil de expressão gênica. Pacientes e Métodos: Foi analisada a expressão gênica de fibroblastos (cultura primária) de 11 pacientes com câncer de mama. O perfil de expressão foi determinado em PT (n=4), N+(n=3) e BM (n=4) através de uma plataforma de cDNA microarray customizada (contendo 4.800 sequencias imobilizadas, representando cerca de 4600 genes), e os genes diferencialmente expressos foram identificados pelo teste SAM multiclasse, seguido pelo teste SAM de duas classes (TMEV, FDR 0%). A análise funcional foi realizada pelo software DAVID v6.7. Validação técnica foi realizada em 6 amostras previamente analisadas no microarray e a validação biológica em fibroblastos obtidos de outros 16 pacientes utilizando-se de RT-qPCR. Resultados: O perfil de expressão gênica dos fibroblastos obtidos de diferentes sítios mostraram 267 genes diferencialmente expressos, os quais apropriadamente agruparam os fibroblastos de acordo com suas origens (PT vs. N+ vs. BM). Apesar das diferenças entre PT e N+ serem representadas por 20 genes, as diferenças entre PT vs. BM e N+ vs BM foram mais significantes (235 e 245 genes diferencialmente expressos respectivamente). Análise funcional dos genes diferencialmente expressos mostrou enriquecimento de funções relacionadas ao desenvolvimento e morfogênese.A seguir, a expressão de alguns genes selecionados foi analisada em uma série diferente de amostras (validação biológica). Desse modo observamos que NOTCH2 confirmou uma alta expressão em N+ (vs. PT), e ADCY2, HECTD1, HNMT, LOX, MACF1 e USP16 confirmaram alta expressão em BM (vs PT). Conclusão:Em pacientes com câncer de mama, células estromais obtidas de diferentes origens apresentam um perfil de expressão gênica diferencial, o qual pode influenciar o comportamento do tumor / may influence tumor development in the primary site of breast cancer, as well as in regional and distant metastatic sites. In this context, fibroblasts are important stromal cells which influence proliferation and migration of cancer cells and may also provide an appropriate niche to tumor development. Objectives: The main objective of this work is the comparison of stromal cells from the primary tumor (PT), lymph node metastasis (N+) and bone marrow (BM) obtained from breast cancer patients, through gene expression profile. Patients and Methods: The gene expression profile was analyzed in fibroblasts primary culture from 11 breast cancer patients. The expression profiles of PT cells (n=4), N+ cells (n=3) and BM cells (n=4) were determined through a customized cDNA microarray platform (containing 4800 immobilized sequences which represents 4600 genes approximately). The analysis were performed by SAM multiclass (TMEV; FDR 0%), followed by SAM two classes test (TMEV; FDR 0%). Functional analysis was performed using DAVID v6.7. Technical validation was performed in same 6 samples that were previously analyzed in microarray experiments and biological validation was performed in fibroblasts obtained from other group of 16patients by RT-qPCR Results: The expression profile of fibroblasts obtained from three sites revealed 267 differentially expressed genes, which appropriately clustered fibroblasts in three different branches, in accordance with their origin (PT vs. N+ vs. BM). Although the differences between PT and N+ were represented by 20 genes, differences between PT vs. BM and N+ vs. BM were more significant (235 and 245 differentially expressed genes respectively). Functional analysis revealed enrichment of functions related to development and morphogenesis. Afterwards, the expression of some selected genes were analyzed in a different batch of samples (biological validation).Thereby, NOTCH2 confirmed high expression in N+ (vs. PT), and ADCY2, HECTD1, HNMT, LOX, MACF1 and USP16 confirmed high expression in BM (vs. PT). Conclusion: In breast cancer patients, stromal cells obtained from different origins present a differential gene expression profile, which may influence tumor behavior

Células mesenquimais estromais

Fibroblastos

Linfonodos

Medula óssea

Microambiente tumoral

Neoplasias da mama

Bone marrow

Breast neoplasm

Fibroblasts

Gene expression profiling

Lymph node

Mesenchymal stromal cells

Tumor microenvironment

Développement de modèles précliniques humanisés autologues en immuno-oncologie

Moquin-Beaudry, Gaël

08 1900

La reconnaissance de l’implication du système immunitaire dans le cancer a guidé l’industrie vers de développement d’immunothérapies nombreuses et prometteuses. Or, à l’ère de l’immuno-oncologie, on constate un manque criant de modèles précliniques capables de simuler les interactions immunitaires entre un patient et sa tumeur. Pour remédier à cette situation, nous avons développé des modèles de souris humanisées combinant la reconstitution immunitaire de souris immunodéficiente et l’injection de lignées tumorales issues d’un même donneur. L’utilisation de cellules souches pluripotentes induites (iPSC) a permis notamment le développement de multiples lignées tumorales à partir d’un seul donneur sain, facilitant ainsi l’accès aux cellules immunitaires nécessaires à l’humanisation des souris. La transformation des cellules primaires ou dérivées d’iPSC a été faite par la transduction lentivirale des proto-oncogènes de la télomérase (hTERT), de Ras oncogénique (HRASV12) et de la région précoce du viruse simen 40 (SV40ER) encodant les gros et petits antigènes T (LgT et SmT). Cette approche permis de générer des tumeurs de haut grade, agressives et peu différenciées à l’aide de fibroblastes primaires et de cellules hépatiques, de cellules souches neurales et d’astrocytes dérivés d’iPSC. Dans tous les cas, les tumeurs ainsi générées ont été efficacement reconnues, infiltrées et souvent rejetées par le système immunitaire autologue implanté. Le rejet partiel de la plupart de ces tumeurs ouvre toutefois la porte à l’évaluation préclinique d’immunothérapies diverses reposant sur les réactions immunitaires anti-tumorales de l’hôte. Par exemple, nous avons pu étudier l’impact d’un traitement d’inhibition du point de contrôle immunitaire PD-1 sur la croissance de tumeurs d’origine fibroblastique où une augmentation marquée du taux d’infiltration immunitaire humaine a été observé sans toutefois mener à une réduction significative du fardeau tumoral. Nous avons aussi pu produire, de façon autologue, des lymphocytes T exprimant un récepteur d’antigène chimérique (CAR) contre le ganglioside GD2, un antigène tumoral préalablement identifié et détecté sur les tumeurs de cellules souches neurales générées par notre approche. L’efficacité cytotoxique de ces CAR a ainsi pu être validée in vitro dans un système autologue. Finalement, nous avons utilisé le modèle de tumeurs fibroblastiques dans des contextes immunitaires autologues et allogéniques pour déterminer si le potentiel immunomodulateur des cellules stromales mésenchymateuses (MSC) pouvait affecter la croissance tumorale. Selon nos résultats, les MSC n’auraient aucun effet ni sur le taux d’émergence et de croissance tumoral, ni sur l’infiltrat immunitaire, suggérant que leur utilisation thérapeutique serait sécuritaire en ce qui concerne ce type de tumeurs ayant préalablement un microenvironnement tumoral immunosuppresseur. En somme, les modèles innovateurs décrits dans cette thèse visent à améliorer la qualité prédictive des modèles murins précliniques en immuno-oncologie en récapitulant certaines interactions immunitaires entre un patient et sa tumeur. La grande flexibilité de cette approche permettra d’adapter aisément le modèle aux problématiques d’intérêt, tant fondamentales que précliniques. / Identification of the human’s immune system implication in cancer has guided the biotech industry towards the development of numerous and promising cancer immunotherapies. However, in the era of immuno-oncology, a distinct lack preclinical models can simulate the interactions between a patient’s tumor and immune cells. To tackle this issue, we developed humanized mouse models combining immune reconstitution of immunodeficient mice and injection of tumor cells lines from the same human donor. The use of induced pluripotent stem cells (iPSC) allowed the generation of multiple tumorigenic cell lines from a single donor, facilitating access to autologous immune cells necessary for mouse immune humanization. The transformation of primary or iPSC-derived cell lines was done using lentiviral transduction of proto-oncogenes telomerase (hTERT), oncogenic Ras (HRASV12) and simian virus 40 early region (SV40ER) encoding large and small T antigens (LgT and SmT). This approach allowed to generate high grade, aggressive and undifferentiated tumors from primary fibroblasts and iPSC-derived hepatic cells, neural stem cells and astrocytes. In all cases, such tumors were efficiently recognized, infiltrated and often rejected by the implanted autologous immune system. However, partial rejection of most tumors allows for preclinical evaluation of targeted immunotherapies relying on the hosts’ pre-existing immune response. For instance, we could study the impact of PD-1 checkpoint blockade inhibition on tumor growth in fibroblastic tumors where a significant increase in tumor infiltration was observed, but without an associated decrease in tumor burden. We could also produce autologous chimeric antigen receptor (CAR)-expressing T lymphocytes against GD2 ganglioside, a previously described tumor antigen detected on our neural stem cell-derived tumor cells. Cytotoxic efficiency of these autologous CAR T cells could thus be validated in vitro. Finally, we used our fibroblast-derived tumor models in autologous and allogeneic settings to determine if mesenchymal stem cells’ (MSC) immunomodulatory potential could impact tumor growth. Our results showed that MSC had no effect neither on tumor emergence and growth nor on immune infiltration, suggesting therapeutic use of these cells should be safe regarding such tumors already harboring a strongly immunodeficient microenvironment. Overall, the novel models described in this thesis aim at improving the predictive capacity of mouse pre-clinical models in immuno-oncology by recapitulating some immune interactions between a patient and its tumor. The great flexibility of this approach will allow for easy adaptation to many research problematics both preclinical and fundamental.

Immunologie tumorale

Cancer

iPSC

Souris humanisées

Immunothérapie du cancer

Cellules stromales mésenchymateuses

Transformation tumorale

Immuno-oncologie

Tumor immunology

Immuno-oncology

Humanized mice

Cancer immunotherapy

Mesenchymal stromal cells

Tumorigenic transformation

Mezenchymální stromální buňky a biologické scaffoldy pro regeneraci nervové tkáně / Mesenchymal stromal cells and biological scaffolds for neural tissue regeneration

Kočí, Zuzana

January 2018

Despite tremendous progress in medicine, injuries of the adult central neural system remain without satisfactory solution. Regenerative medicine employs tissue engineering, cellular therapies, medical devices, gene therapy, or growth factors with the aim to bridge the lesion, re-establish lost connections and enhance endogenous repair in order to restore neural function. The aim of my thesis was to evaluate therapeutic potential of two approaches, transplantation of human mesenchymal stromal cells (hMSCs) and biological scaffolds derived from extracellular matrix (ECM) for neural regeneration, particularly in models of spinal cord injury (SCI). First, hMSCs from various sources - bone marrow (BM), adipose tissue (AT) and Wharton's jelly (WJ) - were isolated and characterized in vitro. All cell types met the minimal criteria for MSC phenotype and displayed similar properties in terms of their surface marker expression, differentiation potential, migratory capacity, and secretion of cytokines and growth factors. On the other hand, the cell yield from WJ and AT was significantly higher, and MSCs isolated from these tissues proliferated better than from BM. Therapeutic effect of intrathecal application of hWJ-MSCs was then evaluated in SCI compression model in rats. The effect of low (0.5 million) and...

Adheze, růst a diferenciace osteoblastů a kmenových stromálních buněk na povrchu biokompatibilních nanomateriálů / Adhesion, growth and differentiation of osteoblasts and mesenchymal stromal cells on biocompatible nanomaterial surfaces

Brož, Antonín

January 2017

The thesis is based on articles describing the fundamental research of carbon based nanomaterials for their possible utilization in biomedicine. The aim of this thesis was to describe the way how human osteoblasts (SAOS-2 cell line) and primary human mesenchymal stem cells (hMSC) adhere, grow and behave on surfaces made of several carbon allotropes - nanocrystalline diamond (NCD), single walled carbon nanotubes (SWCNTs) films and graphene. The utilization of carbon as the basic material promised good biocompatibility and possibility of useful surface modifications. The NCD had modified surface nanotopography (nanoroughness and nanostructuring prepared by dry ion etching). All the materials had modified surface atomic termination with oxygen and hydrogen which changes the surface electrical conductivity, surface charge and wettability. It was hypothesized that the surface termination can also influence the cell adhesion and growth. It turned out that all the studied materials were suitable as substrates for cultivation of mentioned cell types. Various nanoroughnesses of NCD surface had different effect on the cell adhesion and cell metabolic activity. Nanostructuring of the NCD influenced the formation of focal adhesions. The surface terminations of NCD and the other studied nanomaterials in...

Targeting the leukemic stem cell niche: An opportunity for novel therapeutic treatment options

Fusenig, Maximilian

09 June 2022

Acute myeloid leukemia (AML) presents the deadliest form of blood cancer which leads to abrupt, premature deaths. Current therapeutic treatment options in AML are unspecific, resulting in high relapse rates and poor clinical responses in patients. Therapy-resistant, stem cell-like AML cells are believed to be protected by proximal stromal cells in their microenvironment, the leukemic stem cell niche. In part A of this work, an innovative first-of-its-kind arrayed endoribonuclease-prepared siRNA (esiRNA) screen was established for the targeted identification of stromal-derived, AML-supportive genes. Immortalized bone-marrow derived mesenchymal stromal cells (SCP-1) were subjected to individual esiRNA-mediated target gene knockdowns (KD) and subsequently cocultured with AML cell lines MV4-11, OCI-AML3, MOLM-13 and HL-60. AML proliferation and therapy resistance to cytostatic agents Cytarabine or Daunorubicin and tyrosine kinase inhibitor Midostaurin were assessed in direct cocultures. In SCP-1, several secreted, membrane-associated and intracellular molecules were identified which, upon esiRNA-mediated KD, resulted in proliferation inhibition and enhanced treatment response of cocultured AML cells. Carbonic anhydrase 9 (CA9), a stabilizer of intracellular pH, was identified as a supportive factor in proliferation and resistance of leukemic cells to Daunorubicin treatment whilst CA9-KD exerted only a comparably low toxicity in SCP-1 cells. Excitingly, published data by Chen and colleagues (Blood, 2017, Vol. 130, Suppl. 1, 2521) indicated an upregulation of CA9 in hypoxic ex vivo cultures of leukemic cells, measured an anti-leukemic effect of pharmacological CA9 inhibition and identified a synergistic effect on leukemic cells via combinatorial treatment of CA9-inhibition and Cytarabine under hypoxic culture conditions. Taken together, an arrayed esiRNA screen identified CA9 and other stromal-derived factors which potentially open up new avenues for selective therapeutic treatments targeting the leukemic microenvironment in AML. Currently, preclinical leukemia research relies on artificial suspension cultures of AML cells and highly sophisticated, patient-derived xenograft (PDX) mouse models that are marked by suboptimal translation of findings of PDX experiments into the clinic. Recent developments in complex three-dimensional (3D) hydrogel star-shaped poly(ethylene glycol) (starPEG)-heparin cocultures of leukemic and stromal cells of human origin showed promising results in proliferation and drug response studies. Therefore, in part B of this work, a high throughput screening (HTS)-compatible 3D hydrogel culture setup of human stromal cells was established in 384-well plates. Implementation of design of experiments (DoE) enabled an efficient, cost-effective optimization of hydrogel monocultures of human umbilical vein endothelial cells (HUVECs). Optimized culture conditions favored angiogenic sprouting of hydrogel-embedded HUVECs which responded to angiogenic inhibitors Axitinib, AZD4547 and Bevacizumab in a dose-dependent manner. A coculture with bone marrow derived MSCs altered the angiogenic network formation of endothelial CD31+ vessel-like structures. The hydrogel coculture was further stabilized by extensive hydrogel degradation and ECM deposition of MSCs. Stromal MSC networks were illustrated as highly interconnected and elongated F-Actin filament structures (CD31- F-Actin+) that were closely associating with CD31+ F-Actin+ endothelial vessel-like structures. Excitingly, the established 3D hydrogel HTS platform of primary human stromal cells enables future addition of patient-derived leukemic cells for targeted leukemic vulnerability screens in an ex vivo cell culture model of the perivascular stem cell niche. / Akute myeloische Leukämie (AML) gilt als die tödlichste Form der Blutkrebserkrankungen, welche untherapiert zum abrupten, vorzeitigen Tod führt. Etablierte therapeutische Verfahren der AML sind unspezifisch, welche durch heterogene Behandlungseffekte gekennzeichnet sind und zu hohen Rückfallquoten führen. Man vermutet, dass therapie-resistente, stammzellähnliche leukämische Zellen von proximal residierenden Stromazellen in ihrem Mikromilieu, in der sogenannten leukämischen Stammzellnische, vor therapeutischen Behandlungen geschützt werden. In Teil A dieser Arbeit wurde ein innovativer, neuartiger Screen basierend auf Endoribonuklease-generierten kleinen, interferierenden Ribonukleinsäuren (esiRNAs) für eine gezielte Identifikation von AML-supportiven, stromalen Faktoren etabliert. Immortalisierte, mesenchymale Stromazellen aus dem Knochenmark (SCP-1) wurden in einem Array mit spezifischen esiRNAs transfiziert, um esiRNA-basierende inhibierende Effekte (Knockdown) auf die Genexpression von Zielgenen in SCP-1 zu studieren und indirekte Auswirkungen auf Proliferationsrate und Therapieresistenz von kokultivierten leukämischen Zelllinien, MV4-11, OCI-AML3, MOLM-13 und HL-60, bei Behandlung mit Cytarabin, Daunorubicin und Midostaurin, zu studieren. Mehrere sezernierte, membranständige und intrazelluläre Faktoren wurden in SCP-1 identifiziert, deren esiRNA-vermittelter Knockdown zu einer Proliferationsminderung sowie verstärkten Toxizitätseffekten von applizierten Therapeutika in Leukämiezellen führten. Beispielhaft wurde Carboanhydrase (CA9), ein Enzym welches den intrazellularen pH einer Zelle stabilisert, als Target identifiziert. Ein Knockdown von CA9 in SCP-1 resultierte in einer Proliferationsminderung von kokultivierten Leukämiezellen, welche des Weiteren in einer Behandlung mit Daunorubicin verstärkt abgetötet wurden. Publizierte Daten von Chen et al. (Blood, 2017, Vol. 130, Suppl. 1, 2521) zeigten, dass CA9 in hypoxischen ex vivo Kulturen in leukämischen Zellen hochreguliert war und, dass dessen pharmakologische Inhibition einen anti-leukämischen Effekt aufwies. Zudem wurde ein synergistischer Therapieffekt, bei einer Kombinationstherapie mit einem CA9-Inhibitor und Cytarabin, auf AML Zellen in hypoxischer Zellkultur festgestellt. Zusammenfassend wurden in einem esiRNA-Screen CA9 und weitere stromal-exprimierte Faktoren identifiziert, die das Potential besitzen neuartige Therapiestrategien zu ermöglichen, welche auf die leukämische Stammzellnische als Zielstruktur ausgerichtet sind. In der präklinischen Forschung von hämatologischen Erkrankungen werden vorrangig artifizielle zweidimensionale Suspensionskulturen von Leukämiezellen verwendet oder ausgefeilte, patienten-derivierende Xenograft (PDX) Mausmodelle eingesetzt. Bedauerlicherweise weisen Erkenntnisse aus Mausmodellen eine geringe Translationseffizienz in die klinische Forschung auf. Neuste Entwicklungen mit komplexen, dreidimensionalen Hydrogelkulturen, bestehend aus sternförmigem Polyethylenglykol (starPEG) und Heparin, von stromalen und leukämischen Zellen humanen Ursprungs zeigten vielversprechende Ergebnisse in präklinischen Proliferations- und Vulnerabilitätsstudien. Daher wurde in Teil B dieser Arbeit ein hochdurchsatzfähiges dreidimensionales Kultursystem von humanen Stromazellen in Hydrogelen entwickelt. Per statistischer Versuchsplanung wurde eine effiziente, kostengünstige Optimierung von etablierten Hydrogelkulturen für die Hochdurchsatz-kompatible Kultur von humanen venösen Endothelzellen aus Nabelschnuren (HUVECs) durchgeführt. Optimierte Kulturbedingungen führten zur Angiogenese von Hydrogel-eingebetteten HUVECs, welche des Weiteren auf die Angiogenese-Inhibitoren Axitinib, AZD4547 und Bevacizumab in einer konzentrationsabhängigen Weise mit verminderter Bildung von gefäßähnlichen Strukturen reagierten. Eine Kokultur von HUVECs mit primären, mesenchymalen Stromazellen aus dem Knochenmark (MSCs) beeinflusste die Bildung von CD31+ gefäßähnlichen Strukturen. Die Hydrogel-Kokultur wurde des Weiteren durch verstärkte Degradation des Hydrogels und Deposition von Komponenten der extrazellulären Matrix via MSCs verändert und dadurch zusätzlich stabilisiert. Geformte Netzwerkstrukturen von MSCs und HUVECs wurden mittels F-Actin Färbung identifiziert, wodurch ersichtlich wurde, dass Strukturen von MSCs (CD31- F-Actin+) in enger räumlicher Distanz zu HUVEC Strukturen (CD31+ F-Actin+) gebildet wurden. Spannenderweise ermöglicht die, in dieser Arbeit etablierte, Hochdurchsatz-kompatible Kokultur von humanen Stromazellen die Möglichkeit auch leukämische Zellen in die Hydrogelmatrix einzubetten. Eine humane AML-Stroma Kokultur in Hydrogelen wird gezielte Vulnerabilitätsscreens von AML Zellen in einem komplexen ex vivo Zellkulturmodel der perivaskulären Stammzellnische ermöglichen.

info:eu-repo/classification/ddc/610

ddc:610

Altered interactions between mesenchymal stromal cells and hematopoietic stem cells from MDS and AML through expression of FAK / Interactions modifiées entre les cellules stromales mésenchymateuses et les cellules souches hématopoïétiques du SMD et de la LAM par l’expression du FAK

Wu, Yuenv

16 September 2019

La FAK est une tyrosine kinase cytoplasmique qui régule divers processus cellulaires, dont la survie, la prolifération, la différenciation et la motilité. Bien que diverses études aient démontré l'importance du FAK dans la pathogenèse du SMD et de la LAM, le rôle de cette molécule dans le microenvironnement des tumeurs du SMD et de la LAM reste à déterminer davantage. En examinant les CSM de la moelle osseuse qui dérivent de patients atteints de SMD et de LAM, nous avons observé une augmentation continue de l'expression et de l'activation de la FAK pendant la progression du SMD vers de la LAM, semblable à celle observée chez les patients hémopoïétiques. Dans le SMD à faible risque, on a constaté que les CSM se caractérisaient par une faible expression et une faible activation du FAK. Ils présentaient une morphologie modifiée, un immunophénotype, une différenciation et l'expression de facteurs favorables à l'hématopoïèse. Il convient de noter que ces caractéristiques pourraient être largement reproduites dans les CSM saines par inhibition FAK. De plus, l'appauvrissement en FAK dans la lignée cellulaire stromale pourrait induire une expansion massive et l'apoptose des CSH normaux. Nos résultats mettent en évidence le rôle crucial du FAK dans le maintien des fonctions des CSM et fournissent la preuve que la dysrégulation du FAK dans les CSM contribue à la perturbation de l'hématopoïèse et éventuellement à la progression des tumeurs malignes myéloïdes. Une meilleure compréhension du rôle que joue le microenvironnement du SMD et de la LAM permettra de mieux reconnaître les patients à faible risque et de mettre au point des traitements ciblant les CSM défectueuses, améliorant ainsi le résultat clinique / FAK is a cytoplasmic tyrosine kinase that regulates diverse cellular processes, including survival, proliferation, differentiation, and motility. Though various studies have demonstrated the importance of FAK in MDS and AML pathogenesis, the role of this molecule in MDS and AML tumor microenvironment remained to be further determined. By examining BM MSCs derived from MDS and AML patients, we have observed a continues increase of FAK expression and activation during MDS progression to AML, similar to those detected in hemopoietic counterparts. In LR-MDS, MSCs were found to be characterized by low FAK expression and activation. They exhibited altered morphology, immunophenotype, differentiation, and expression of hematopoiesis-supporting factors. Of note, these features could be largely reproduced in normal MSCs by FAK inhibition. Furthermore, FAK depletion in BM stromal cell line could induce massive expansion and apoptosis of normal HSPCs. Our results highlight a critical role of FAK in maintaining the functions of BM MSCs and provide evidence that dysregulation of FAK in MSCs contribute to the disturbed hematopoiesis and possibly the progression of myeloid malignancies. A greater understanding of the role that BM microenvironment plays in MDS and AML will enable an increased recognition of poor-risk patients and the development of therapies that target the defected MSCs, thereby improving the clinical outcome

Cellules stromales mésenchymateuses

Propriété cellulaire

Support d'hématopoïèse

Microenvironnement de la moelle osseuse

Syndromes myélodysplasiques

Leucémie myéloïde aiguë

Focal adhesion kinase

Mesenchymal stromal cells

Cellular property

Hematopoiesis-support

Bone marrow microenvironment

Myelodysplastic syndromes

Acute myeloid leukemia

Focal adhesion kinase

570

Assessment of High Purity Mesenchymal Stromal Cells Derived Extracellular Vesicles Presenting NRP1 Show Functional Suppression of Activated Immune Cells

Gobin, Jonathan

04 January 2022

Background: The focus of this study was to investigate how producing human bone marrow (hBM) derived mesenchymal stromal cell (MSC) extracellular vehicles (EVs) in a high purity isolation system would affect their established characterization criteria and address the validity of these methods of EV production. Additionally, we set out to functionally characterize the hBM-MSC-EVs for their identified immunomodulatory ability while also assessing the presence of novel MSC-EV marker NRP1 identified by our group to further affirm its validity as a functional MSC-EV identity marker. Methods: Each hBM-MSC-EV donor was cultured in a hollow-fiber bioreactor system in non-stimulating serum/xeno-free conditions for 25 days to produce EVs persistently under quiescent conditions to characterize the hBM-MSC-EVs in their native form. EVs were isolated by traditional PEG-based precipitation for preliminary characterization to monitor bioreactor production wherein they were characterized using multimodal tangential flow filtration coupled with fast protein liquid chromatograph (FPLC) size exclusion/high-affinity purifications to obtain the final highly purified EV sample. Additionally, functional analysis of their immunomodulatory ability, EVs and MSCs were incubated with activated peripheral blood mononuclear cells (PBMCs) as an in-vitro model to evaluate their potency. Results: The hBM-MSC-EVs produced from the bioreactor system showed consistent characterization in accordance with the MISEV2018 establish criteria. We were also able to demonstrate their functional ability by observing statistically significantly immunomodulatory ability of activated PBMCs equivalent to native MSC ability. We were also able to validate the present of NRP1 on all hBM-MSC-EV samples produced confirming its validity as a MSC-EV marker. Conclusion: The significance of the results obtained from this study confirms the production of MSC-EV using a bioreactor and high purity isolation for obtaining consistent MSC-EVs for downstream investigation. Additionally, we were able to demonstrate the significance of MSC-EVs on MSC signaling for immunomodulation by showing equivalent functional potency when tested in-vitro. These results contribute to further understanding the biological attributes of MSC-EVs and contribute to the validation of currently established characterization guidelines.

Extracellular Vesicles (EVs)

NRP1

Mesenchymal Stromal Cells (MSCs)

Bioreactor

Tangential Flow Filtration (TFF)

Nanoparticle Trackning Analysis (NTA)

Immune Suppression

Characterization

Isolation

ISEV

ISCT

cGMP

Pre-clinical

Cell based therapy

Tenogenic Properties of Mesenchymal Progenitor Cells Are Compromised in an Inflammatory Environment

Brandt, Luisa, Schubert, Susanna, Scheibe, Patrick, Brehm, Walter, Franzen, Jan, Gross, Claudia, Burk, Janina

22 December 2023

Transplantation of multipotent mesenchymal progenitor cells is a valuable option for treating tendon disease. Tenogenic differentiation leading to cell replacement and subsequent matrix modulation may contribute to the regenerative effects of these cells, but it is unclear whether this occurs in the inflammatory environment of acute tendon disease. Equine adipose-derived stromal cells (ASC) were cultured as monolayers or on decellularized tendon scaffolds in static or dynamic conditions, the latter represented by cyclic stretching. The impact of different inflammatory conditions, as represented by supplementation with interleukin-1β and/or tumor necrosis factor-α or by co-culture with allogeneic peripheral blood leukocytes, on ASC functional properties was investigated. High cytokine concentrations increased ASC proliferation and osteogenic differentiation, but decreased chondrogenic differentiation and ASC viability in scaffold culture, as well as tendon scaffold repopulation, and strongly influenced musculoskeletal gene expression. Effects regarding the latter differed between the monolayer and scaffold cultures. Leukocytes rather decreased ASC proliferation, but had similar effects on viability and musculoskeletal gene expression. This included decreased expression of the tenogenic transcription factor scleraxis by an inflammatory environment throughout culture conditions. The data demonstrate that ASC tenogenic properties are compromised in an inflammatory environment, with relevance to their possible mechanisms of action in acute tendon disease.

info:eu-repo/classification/ddc/570

ddc:570