• Refine Query
  • Source
  • Publication year
  • to
  • Language
  • 39
  • 35
  • 30
  • 13
  • 5
  • 4
  • 4
  • 3
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • 1
  • Tagged with
  • 152
  • 80
  • 40
  • 36
  • 35
  • 33
  • 23
  • 22
  • 22
  • 21
  • 20
  • 17
  • 16
  • 15
  • 15
  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
131

Crosswind assessment of trains on different ground configurations

Venkatasalam, Nachiyappan January 2013 (has links)
Cross wind analysis is one of the important safety measures for rail vehicle certification. The objective of this study is to identify which vehicle certification ground setup, true flat ground (TFG) or single track ballast and rail (STBR) represents a more realistic ground setup with atmospheric boundary layer (ABL) wind inlet and also to represent an embankment scenario. A streamlined high speed train ICE3 and a conventional Regional train are taken for the analysis to represent both categories. CFD is used as a tool for calculations. The best practice recommended by the AeroTRAIN project is used for the CFD approach. The analysis is done for various configurations including STBR, TFG, embankments, ground roughness, moving ground, non-moving ground, block profile inlet, ABL inlet, model scale and full scale setups. The Regional train shows higher roll moment coefficient about lee rail (Cmx,lee) compared to the ICE3 train, whereas the ICE3 train has a higher lift force coefficient than the Regional train. STBR setup shows a higher force and moment coefficient compared to TFG. The STBR setup represents the more realistic setup of moving rough ground with ABL wind inlet and also the realistic embankment scenario.
132

Critical Molecular Pathways in Cancer Stem Cells of Chronic Myeloid Leukemia: A Dissertation

Chen, Yaoyu 11 May 2011 (has links)
Chronic myeloid leukemia (CML) is a disease characterized by the expansion of granulocytic cells. The BCR-ABL tyrosine kinase inhibitor imatinib, the frontline treatment for Ph+ leukemias, can induce complete hematologic and cytogenetic response in most chronic phase CML patients. Despite the remarkable initial clinic effects, it is now recognized that imatinib will unlikely cure patients because a small cell population containing leukemic stem cells (LSCs) with self-renewal capacity is insensitive to tyrosine kinase inhibitors. In Chapter I, I briefly review the BCR-ABL kinase and its related signaling pathways. BCR-ABL kinase activates several signaling pathways including MAPK, STAT, and JNK/SAPK. BCR-ABL also mediates kinase-independent pathways through SRC family kinases. I will also discuss pathways involving β-catenin, hedgehog, FoxO and Alox5 are critical to the regulation of self-renewal and differentiation in LSC of CML. As detailed in Chapter II, I describe our work evaluating the effects of omacetaxine, a novel CML drug inducing cell apoptosis by inhibition of protein synthesis, on self-renewal and differentiation of LSCs and BCR-ABL-induced CML and acute lymphoblastic leukemia (B-ALL) in mice. We found that treatment with omacetaxine decreased the number of LSCs and prolonged the survival of mice with CML or B-ALL. In chapter III, I describe that Alox5 is an essential gene in the function of LSCs and CML development. We show evidence that Alox5 affects differentiation, cell division, and survival of long-term LSCs. Treatment of CML mice with a 5-LO inhibitor also impaired the function of LSCs similarly and prolonged survival. In chapter IV, I present evidence of our work showing a further dissection the Alox5 pathway by comparing the gene expression profiles of wild type and Alox5-/- LSCs. We show that Msr1 deletion causes acceleration of CML development. We also show that Msr1 affects CML development by regulating the PI3K-AKT pathway and β-catenin. Taken together, these results demonstrate that some pathways including Alox5 and Msr1 play an important role in regulating the self-renewal and differentiation of LSC. More efforts should be put into developing the novel strategies that may effectively target LSCs and thus cure CML.
133

The Role of Collateral in Asset Based Lending / 動産・売掛金担保融資(ABL)における担保の役割

Kinjo, Aki 23 March 2015 (has links)
京都大学 / 0048 / 新制・課程博士 / 博士(経済学) / 甲第18755号 / 経博第506号 / 新制||経||272(附属図書館) / 31706 / 京都大学大学院経済学研究科経済学専攻 / (主査)教授 川北 英隆, 教授 徳賀 芳弘, 教授 澤邉 紀生 / 学位規則第4条第1項該当 / Doctor of Economics / Kyoto University / DGAM
134

Acompanhamento molecular de pacientes com leucemia mielóide crônica tratados com mesilato de imatinibe e avaliação dos mecanismos de resistência ao tratamento: mutação do gene BCR-ABL e expressão dos genes MDR1 e BCRP / Molecular monitoring of patients with chronic myeloid leukemia treated with imatinib mesylate and evaluation of treatment resistance mechanisms: mutation of BCR-ABL and expression of MDR1 and BCRP genes

Nardinelli, Luciana 25 March 2009 (has links)
A leucemia mielóide crônica (LMC) é caracterizada pela translocação (9;22) que dá origem ao gene quimérico BCR-ABL. Este gene codifica uma proteína com atividade tirosina quinase, p210, constitutivamente ativa. O três mecanismos envolvidos na patogênese da LMC são o aumento da proliferação celular, alteração da adesão celular ao estroma e matriz medular e inibição da apoptose. A introdução do mesilato de imatinibe (MI), um inibidor de tirosina quinase, revolucionou o tratamento da LMC levando pacientes em fase crônica a remissões duráveis, porém uma parcela destes não responde ou perde a resposta ao longo do tratamento. Os mecanismos de resistência ao MI podem ser classificados como independentes de BCR-ABL (a1- glicoproteína ácida e genes de resistência a múltiplas drogas) ou dependentes de BCR-ABL (superexpressão de BCR-ABL e mutações do domínio quinase do gene ABL). Objetivo: avaliar a presença de mutações no domínio quinase do gene ABL e a expressão dos genes de resistência a múltiplas drogas MDR1 e BCRP em amostras pré-tratamento com MI, acompanhar estes pacientes mensalmente através da quantificação de transcritos BCR-ABL e quando ocorrer resistência reavaliar a presença de mutações do domínio quinase do ABL e a expressão dos genes de resistência a múltiplas drogas. Material e Métodos: Foram avaliados 61 pacientes com LMC em fase crônica. A pesquisa de mutações do domínio quinase foi realizada pela técnica de seqüenciamento direto e a expressão relativa dos genes de resistência a múltiplas drogas foi avaliada por PCR em tempo real. A quantificação absoluta do número de transcritos BCR-ABL foi realizada pela técnica de PCR em tempo real utilizando-se o sistema Taqman de sondas de hibridização. Resultados: Nas amostras pré-tratamento dos 61 pacientes estudados não foram detectadas mutações. Quando relacionamos o aumento da expressão dos genes MDR1 e BCRP à resposta citogenética completa aos 12 meses de tratamento não houve diferença estatística significativa (p>0,05). Quanto ao número de transcritos BCR-ABL, observamos que os pacientes que apresentaram menos de 1% pela escala internacional aos 3 meses de tratamento atingiram a RMM em período menor (7 meses) do que os que apresentaram mais de 1% (12 meses) com diferença estatística significativa (p = 0,03). Conclusões: As mutações do domínio quinase do gene BCR-ABL nas amostras pré-tratamento não foram detectadas ou pela sensibilidade da técnica de seqüenciamento direto (10%) ou porque tais mutações são mais freqüentes nas fases acelerada e blástica. A expressão dos genes de resistência a múltiplas drogas (MDR1) e BCRP) em pacientes com LMC-FC ao diagnóstico não apresentou correlação com o aparecimento de resistência secundária ao MI. Além disso a quantificação mensal dos transcritos BCR-ABL aos 3 meses pode ser considerada um marcador com valor prognóstico. / Chronic myeloid leukemia is characterized by t(9;22) translocation. The chimeric gene BCR-ABL encodes a p210BCRABL protein with constitutive tyrosine kinase activity which is directly related to CML pathogenesis. The imatinib mesylate, a tyrosine kinase inhibitor, is the first-choice treatment for patients in chronic phase but some patients show primary resistance or relapse after initial response. The mechanisms of resistance to the imatinib mesylate treatment are BCR-ABL dependent (amplification of BCR-ABL and mutation of kinase domain of BCR-ABL) or independent of BCR-ABL (1-acid glycoprotein and expression of multidrug resistance genes). Objective: The objective of this work was to evaluate the mechanisms of resistance (kinase domain mutation and MDR1 and BCRP genes expression) to imatinib mesylate in pretreatment samples, quantify of BCR-ABL transcript on a monthly follow up plan, and to re-evaluate the mechanisms of resistance in the absence or loss of treatment response. Patients and Methods: We have evaluated 61 pretreatment samples derived from chronic phase CML patients. The number of BCR-ABL transcripts was quantified by RTQ-PCR with taqman probes and MDR1 and BCRP expression were evaluated by RTQ-PCR with Syber Green. Mutations within the BCR-ABL kinase domain were screened by direct sequencing and we also have screened the T315I mutation in pretreatment samples by allele-specific PCR. Results:We detected no mutations in the 61 pretreatment samples. The correlation analysis between the expression of MDR1/BCRP genes and the cytogenetic response at 12 months of treatment revealed no significant statistical difference (p = > 0.05). The results of BCR-ABL quantification in the follow up of our cohort indicated that patients who had transcripts <1% by the international scale at 3 months of therapy are more likely to achieve rapid MMR (median of 7 months) than those who had >1% (median of 12 months) (p = 0,03). Conclusions: As expected, the kinase domain mutations of BCR-ABL in pretreatment samples of CML chronic phase patients are not detectable by direct sequencing because of the sensitivity of the assay (10%) and also because these mutations are more common in accelerated phase and blast crisis. About the expression of multidrug resistance genes MDR1 and BCRP, they showed no correlation with secondary resistance to imatinib mesylate. And finally the number of BCR-ABL transcripts at 3 months of treatment can be considered a marker with prognostic value.
135

Acompanhamento molecular de pacientes com leucemia mielóide crônica tratados com mesilato de imatinibe e avaliação dos mecanismos de resistência ao tratamento: mutação do gene BCR-ABL e expressão dos genes MDR1 e BCRP / Molecular monitoring of patients with chronic myeloid leukemia treated with imatinib mesylate and evaluation of treatment resistance mechanisms: mutation of BCR-ABL and expression of MDR1 and BCRP genes

Luciana Nardinelli 25 March 2009 (has links)
A leucemia mielóide crônica (LMC) é caracterizada pela translocação (9;22) que dá origem ao gene quimérico BCR-ABL. Este gene codifica uma proteína com atividade tirosina quinase, p210, constitutivamente ativa. O três mecanismos envolvidos na patogênese da LMC são o aumento da proliferação celular, alteração da adesão celular ao estroma e matriz medular e inibição da apoptose. A introdução do mesilato de imatinibe (MI), um inibidor de tirosina quinase, revolucionou o tratamento da LMC levando pacientes em fase crônica a remissões duráveis, porém uma parcela destes não responde ou perde a resposta ao longo do tratamento. Os mecanismos de resistência ao MI podem ser classificados como independentes de BCR-ABL (a1- glicoproteína ácida e genes de resistência a múltiplas drogas) ou dependentes de BCR-ABL (superexpressão de BCR-ABL e mutações do domínio quinase do gene ABL). Objetivo: avaliar a presença de mutações no domínio quinase do gene ABL e a expressão dos genes de resistência a múltiplas drogas MDR1 e BCRP em amostras pré-tratamento com MI, acompanhar estes pacientes mensalmente através da quantificação de transcritos BCR-ABL e quando ocorrer resistência reavaliar a presença de mutações do domínio quinase do ABL e a expressão dos genes de resistência a múltiplas drogas. Material e Métodos: Foram avaliados 61 pacientes com LMC em fase crônica. A pesquisa de mutações do domínio quinase foi realizada pela técnica de seqüenciamento direto e a expressão relativa dos genes de resistência a múltiplas drogas foi avaliada por PCR em tempo real. A quantificação absoluta do número de transcritos BCR-ABL foi realizada pela técnica de PCR em tempo real utilizando-se o sistema Taqman de sondas de hibridização. Resultados: Nas amostras pré-tratamento dos 61 pacientes estudados não foram detectadas mutações. Quando relacionamos o aumento da expressão dos genes MDR1 e BCRP à resposta citogenética completa aos 12 meses de tratamento não houve diferença estatística significativa (p>0,05). Quanto ao número de transcritos BCR-ABL, observamos que os pacientes que apresentaram menos de 1% pela escala internacional aos 3 meses de tratamento atingiram a RMM em período menor (7 meses) do que os que apresentaram mais de 1% (12 meses) com diferença estatística significativa (p = 0,03). Conclusões: As mutações do domínio quinase do gene BCR-ABL nas amostras pré-tratamento não foram detectadas ou pela sensibilidade da técnica de seqüenciamento direto (10%) ou porque tais mutações são mais freqüentes nas fases acelerada e blástica. A expressão dos genes de resistência a múltiplas drogas (MDR1) e BCRP) em pacientes com LMC-FC ao diagnóstico não apresentou correlação com o aparecimento de resistência secundária ao MI. Além disso a quantificação mensal dos transcritos BCR-ABL aos 3 meses pode ser considerada um marcador com valor prognóstico. / Chronic myeloid leukemia is characterized by t(9;22) translocation. The chimeric gene BCR-ABL encodes a p210BCRABL protein with constitutive tyrosine kinase activity which is directly related to CML pathogenesis. The imatinib mesylate, a tyrosine kinase inhibitor, is the first-choice treatment for patients in chronic phase but some patients show primary resistance or relapse after initial response. The mechanisms of resistance to the imatinib mesylate treatment are BCR-ABL dependent (amplification of BCR-ABL and mutation of kinase domain of BCR-ABL) or independent of BCR-ABL (1-acid glycoprotein and expression of multidrug resistance genes). Objective: The objective of this work was to evaluate the mechanisms of resistance (kinase domain mutation and MDR1 and BCRP genes expression) to imatinib mesylate in pretreatment samples, quantify of BCR-ABL transcript on a monthly follow up plan, and to re-evaluate the mechanisms of resistance in the absence or loss of treatment response. Patients and Methods: We have evaluated 61 pretreatment samples derived from chronic phase CML patients. The number of BCR-ABL transcripts was quantified by RTQ-PCR with taqman probes and MDR1 and BCRP expression were evaluated by RTQ-PCR with Syber Green. Mutations within the BCR-ABL kinase domain were screened by direct sequencing and we also have screened the T315I mutation in pretreatment samples by allele-specific PCR. Results:We detected no mutations in the 61 pretreatment samples. The correlation analysis between the expression of MDR1/BCRP genes and the cytogenetic response at 12 months of treatment revealed no significant statistical difference (p = > 0.05). The results of BCR-ABL quantification in the follow up of our cohort indicated that patients who had transcripts <1% by the international scale at 3 months of therapy are more likely to achieve rapid MMR (median of 7 months) than those who had >1% (median of 12 months) (p = 0,03). Conclusions: As expected, the kinase domain mutations of BCR-ABL in pretreatment samples of CML chronic phase patients are not detectable by direct sequencing because of the sensitivity of the assay (10%) and also because these mutations are more common in accelerated phase and blast crisis. About the expression of multidrug resistance genes MDR1 and BCRP, they showed no correlation with secondary resistance to imatinib mesylate. And finally the number of BCR-ABL transcripts at 3 months of treatment can be considered a marker with prognostic value.
136

La voie Rho/ROCK, un nouveau mécanisme d'échappement des cellules leucémiques au contrôle de l'immunité T innée / The Rho/ROCK pathway as a new pathological mechanism of innate T cell immune subversion in chronic myeloid leukemia

Basbous, Sara 13 July 2016 (has links)
Les cellules iNKT et T CDS innées sont présumées contribuer à l'irnmunosurveillance (IS) des cancers et sont fonctionnellement déficientes dans la leucémie myéloïde chronique (LMC). Notre hypothèse était que ces défauts résultent de l'incapacité des cellules dendritiques myéloïdes (mDC) à les activer. Des analyses par cytométrie en flux et microscopie confocale ont révélé une baisse de l'expression membranaire de CD 1 d, qui présente les antigènes aux cellules iNKT, à la surface des mDC des patients LMC, par comparaison aux sujets sains. Ce défaut n'est associé ni à un défaut de maturation des mDC, comme le montre l'expression normale de HLA-DR et de CDS6, ni à une baisse d'expression intracellulaire de CDld ou de son transcrit. Ces résultats sont conciliables avec une rétention intracellulaire. Le traitement in vitro des mDC des patients LMC avec un inhibiteur de la protéine ROCK restaure partiellement l'expression de surface de CD 1 d et la présentation antigénique par CD Id, alors qu'il n'a eu aucun effet sur les mDC des sujets sains. Nous proposons que la protéine ROCK, qui est activée par le domaine DH-PH de BCR-ABL, interfere avec la réponse immunitaire dépendant des lymphocytes iNKT au cours de la LMC par régulation négative de l'expression membranaire de CDld des mDC. Le fait que les cellules iNKT et T CDS innées retrouvent des fonctions normales après rémission complète de la LMC est en faveur d'une génération de cellules T CD8 innées dépendante des cellules iNKT, comme décrit chez la souris. Notre travail suggère une implication des cellules iNKT et T CD8 innées dans l'IS de la LMC et révèle l'axe ROCK/mDC comme une nouvelle cible thérapeutique dans la maladie. / CDld-restricted iNKT cells and innate CD8 T cells are believed to play a key role in cancer immune surveillance and are functionally deficient in chronic myeloid leukemia (CML). Herein, we have hypothesized that this defect might originate from BCR-ABL-dependent dysfunctions in myeloid dendritic cells (mDC). Indeed, flow cytometry and confocal microscopy revealed that cell-surface expression of CDld was downregulated in CML mDC, relative to healthy donor (HD) controls. The decreased cell-surface display of CDld could not be ascribed to defective mDC differentiation, as attested by normal expression of HLA-DR and the CD86 maturation marker. On the other hand, reduced membrane expression was not associated with decreased intracytoplasmic levels of CDld or its mRNA transcripts, consistent with intracellular retention. ln vitro treatrnent of CML mDC with the Rho-associated protein Kinase (ROCK) inhibitor Y-27632 partially restored both cell-surface CDld expression and CDld-mediated antigen presentation, while it had no effect on HD mDC. We propose that ROCK, which is most likely activated by the DH-PH domain of BCR-ABL, mediates iNKT-cell immune subversion in CML patients by downregulating CDld expression on CML mDC. Remarkably, both iNKT cells and innate CD8 T cells retumed to nonnal after complete CML remission, a finding consistent with a iN KT cell-dependent generation of innate CD8 T cells, similarly to the observations in mice. Ali in ali, our study supports the possible contribution of iNKT/innate CD8 T cells to tumor surveillance in CML, and reveals the ROCK/mDC axis as a new potential target to restore immune surveillance in CML.
137

Influence du microenvironnement inflammatoire sur la sénescence contrôlée par la réponse aux dommages à l'ADN, et sa régulation par l’induction du stress à la chromatine

Carrier-Leclerc, Audrey 01 1900 (has links)
La sénescence cellulaire, ou l’arrêt irréversible de la prolifération, influence des processus physiologiques et pathologiques, comme le cancer. Parmi les caractéristiques de la sénescence, se retrouve le PSAS ou phénotype sécrétoire associé à la sénescence. Le PSAS est composé d’une variété de cytokines, facteurs de croissance et protéases. Ses actions pro- et anti-tumorale sont connues, mais l’on ignore laquelle prédomine. Mes travaux s’attardent aux effets du PSAS sur l’induction de la sénescence dans les cellules environnantes et à sa régulation. Nous avons démontré que le PSAS ne synergise pas avec la dysfonction télomérique chronique ou aigue, afin de causer un arrêt de croissance. Également, l’étude du mécanisme responsable de l’induction de la sénescence par stress à la chromatine, suggère que la kinase c-Abl n’est pas requise pour cette voie, contrairement à des publications antérieures. Mes travaux éclairent les mécanismes d’action et la régulation du PSAS dans la sénescence induite par dysfonction télomérique et par stress à la chromatine. / Cellular senescence, or irreversible proliferation arrest, is known for its influence on physiological and pathological processes, such as cancer. Among the features found in the senescent phenotype is the inflammatory secretome, also known as the senescence associated secretory phenotype (SASP). The SASP consists of a variety of factors such as cytokines, growth factors and proteases. It is widely recognized that SASP can have either a pro- or anti-tumor effect, but it is not clear which one predominates. My work focused on the SASP effects on the induction of senescence in surrounding cells and its regulation mechanisms. We demonstrated that the SASP does not synergize with chronic or induced telomere dysfunction to cause cellular proliferation arrest. Also, study of chromatin stress-induced senescence mechanism suggests that kinase c-Abl is not required for this pathway, contrary to what had been previously published. My work helps understand the regulatory and working mechanisms of the SASP in chromatin stress-induced and telomere dysfunction-induced senescence models.
138

Leukemie s fusním genem BCR/ABL. / Leukaemias with BCR/ABL fusion gene.

Hovorková, Lenka January 2013 (has links)
Philadelphia (Ph) chromosome, as a result of reciprocal translocation, is in majority of cases connected to two types of leukaemia - chronic myelogenous (CML) and acute lymphoblastic (ALL). The translocation occurs within large intronic sequences of BCR and ABL genes. The breakpoints are specific for individual patient and may be used as a target for monitoring of leukemic burden (MRD, minimal residual disease) during the treatment. In general, MRD is an important prognostic factor, which influences the treatment intensity. Two standardized methods are currently used for its monitoring. The first one is based on the detection of clonal specific Immunoglobulin and/or T-cell receptor genes rearrangements (and thus cannot be used for CML cases) at the DNA level, the second one utilizes detection of the BCR/ABL fusion gene at the mRNA level. Our aim was to optimize and standardize the process to find individual patient breakpoints on Ph chromosome and to use it for MRD quantification. We found the breakpoint in 80 % cases. The MRD data from 15 patients obtained by our method were compared to the levels obtained by standard methods (Ig/TCR and BCR/ABL transcript quantification). In all but 1 patient we found significant discrepancies, raising the questions about leukemic origin and the most accurate method for...
139

Målbolagsstyrelsens roll vid offentliga uppköpserbjudanden : De nya takeover-reglernas inverkan

Lundquist, Dennis, Nilsson, Fredrik January 2012 (has links)
Ett offentligt uppköpserbjudande skiljer sig från andra typer av företagsförvärv på så sätt att det riktar sig till en större ägandekrets. Eftersom köparen av praktiska skäl inte kan förhandla enskilt med aktieägarna riktar sig köparen istället, i ett offentligt erbjudande, till alla aktieägare i bolaget. Aktieägarna har sedan att förkasta eller acceptera erbjudandet. Förfarandet kring ett offentligt uppköpserbjudande kräver en aktiv målbolagsstyrelse för att tillvarata aktieägarnas intresse. Takeover-reglernas koppling till LUA har i och med revideringen tydliggjorts och de två regelverken utgör tillsammans stommen i regleringen av offentliga uppköpserbjudanden. Målbolagsstyrelsens roll vid ett offentligt uppköpserbjudande kommer främst till uttryck i punkterna II.17, II.19 och II.20 i takeover-reglerna. Takeover-reglerna har reviderats ett antal gånger sedan de första reglerna, då benämnda rekommendationer, utkom 1971 och målbolagsstyrelsens roll har vid varje revidering utvecklats till att bli mer omfattande. De nya takeover-reglerna träder i kraft den 1 juli 2012. Förutom frågan om hur de nya reglerna kommer att påverka målbolagsstyrelsens roll framträder frågan om vilka intressen som målbolagsstyrelsen ska tillvarata och hur dessa förhåller sig till varandra. Intressebegreppen, aktieägarnas intresse och bolagets intresse, kommer till uttryck såväl aktiemarknadsrättsligt som aktiebolagsrättsligt. Märkbart vid analys av ändringarna är att de till viss del har skett genom kodifiering av AMN:s uttalanden och doktrin på området. Reglerna har även anpassats, om än inte fullt ut, till brittiska Takeover Code. Ett tydligt exempel är ändringen avseende avtal om deal protection-arrangemang. För att utröna de konkreta konsekvenserna av regeländringarna krävs, i vissa fall, uttalanden från AMN eller komplettering och uppdatering av doktrin på området. Målbolagsstyrelsens roll har, i och med de nya takeover-reglerna, blivit än mer omfattande samtidigt som dess position, gentemot budgivaren, har stärkts genom tydligare reglering för hur styrelsen ska agera.
140

A Src-Abl kinase inhibitor, SKI-606, blocks breast cancer invasion, growth and metastasis in vitro and in vivo /

Jallal, Houda. January 2007 (has links)
The central role of Src in the development of several malignancies including breast cancer and the accumulating evidence of its interaction with receptor tyrosine kinases (RTK), integrins and steroid receptors have identified it as an attractive therapeutic target. In the current study we have evaluated the effect of a Src/Abl kinase inhibitor SKI-606, on breast cancer growth, migration, invasion and metastasis. Treatment of human breast cancer cells MDA-MB-231 with SKI-606 caused a marked inhibition of cell proliferation, invasion and migration by inhibiting MAPK and Akt phosphorylation. For in vivo studies MDA-MB-231 cells transfected with the plasmid encoding green fluorescent protein (GFP) [MDA-MB-231-GFP] were inoculated into mammary fat pad of female BALB/c nu/nu mice. Once tumor volume reached 30-50 mm3, animals were randomized and treated with vehicle alone or 150 mg/kg of SKI-606 by daily oral gavage. Experimental animals receiving SKI-606 developed tumors of significantly smaller volume (45-54%) as compared to control animals receiving vehicle alone. Analysis of lungs, liver and spleen of these animals showed a significant decrease in GFP positive tumor metastasis in animals receiving SKI-606 at a dose that was well tolerated. Western blot analysis and immunohistochemical analysis of primary tumors showed that these effects were due to the ability of SKI-606 to block tumor cell proliferation, angiogenesis, growth factors expression and inhibition of Src mediated signalling pathways in vivo. Together the results from these studies provide compelling evidence for the use of Src inhibitors as therapeutic agents for blocking breast cancer growth and metastasis.

Page generated in 0.0363 seconds