O fluido folicular de mulheres inférteis com endometriose leve pode comprometer o fuso meiótico de oócitos em metáfase II / Follicular fluid from infertile women with mild endometriosis may compromise the meiotic spindle of methaphase II oocytes

Broi, Michele Gomes da

01 November 2011

Os mecanismos envolvidos na etiopatogênese da infertilidade em pacientes com endometriose não foram totalmente elucidados. A infertilidade apresentada por pacientes com as formas moderada e grave (estadios III e IV, respectivamente) seria, parcialmente, decorrente de alterações anatômicas pélvicas associadas à endometriose. Entretanto, há evidências de que lesões sutis ou implantes endometrióticos em estágios iniciais (estágio mínimo e leve) também poderiam contribuir com a etiopatogênese da infertilidade. Uma pior qualidade oocitária pode estar envolvida nas menores taxas de implantação após fertilização in vitro encontradas nessas pacientes. Questionamos a possibilidade de haver alterações no microambiente folicular de pacientes inférteis com endometriose, as quais poderiam afetar a aquisição de competência oocitária e, consequentemente, comprometer a fertilidade natural e os resultados dos tratamentos de reprodução assistida em mulheres com esta doença. Sabe-se que, para ser competente e poder ser fertilizado, o oócito precisa estar maduro e ter um fuso morfologicamente funcional, que garanta a fidelidade da segregação cromossômica durante a meiose. Dessa forma, o objetivo deste estudo foi avaliar o potencial impacto de diferentes concentrações de fluido folicular (FF) de mulheres inférteis com e sem endometriose leve sobre a integridade do fuso, alinhamento cromossômico e organização dos microfilamentos de actina de oócitos bovinos maturados in vitro. Realizou-se um estudo experimental, onde amostras de fluido follicular foram consecutivamente obtidas de 22 pacientes inférteis (11 com endometriose leve e 11 com infertilidade por fator tubário e/ou masculino) submetidas à estimulação ovariana para injeção intracitoplasmática de espermatozóide. Oócitos bovinos imaturos foram submetidos à maturação in vitro (MIV) sem adição de fluido follicular (sem fluido) e com 4 concentrações (1%, 5%, 10%, e 15%) de duas amostras de fluido folicular (uma de paciente com endometriose e outra de paciente sem endometriose). Foram realizadas 11 MIVs e cada amostra de fluido follicular foi usada apenas uma vez. Os oócitos foram fixados, marcados por imunofluorescência para visualização morfológica de microtúbulos, cromatina e microfilamentos de actina e, então, analisados por microscopia confocal. A porcentagem de anormalidade de oócitos em MII (fuso normal e cromossomos desalinhados, fuso anormal e cromossomos desalinhados, fuso anormal e cromossomos alinhados) foi significativamente maior naqueles maturados com FF de pacientes com endometriose (1%: 55,56%, 5%: 63,26%, 10%: 54,54%, 15%: 48,84%) quando comparados com oócitos maturados com FF de pacientes controles (1%: 19,15%, 5%: 23,44%, 10%: 25%, 15%: 23,81%) e oócitos maturados sem fluido (23,53%), sem haver diferença entre as concentrações testadas em cada grupo. Pode-se concluir que oócitos bovinos maturados in vitro na presença de FF de mulheres inférteis com endometriose leve têm maior freqüência de anormalidade meiótica. Estes dados sugerem que o FF de mulheres com endometriose pode comprometer a qualidade oocitária por promover danos ao fuso e/ou cromossomos / The mechanisms involved in the etiopathogenesis of infertility in patients with endometriosis have not been fully elucidated. The infertility presented by patients with moderate and severe disease (stages III and IV, respectively) would be partly due to anatomical pelvic changes associated with endometriosis. However, there are evidences that subtle lesions or endometriosis implants in the early stages (stages I and II) might also contribute to the etiophatogenesis of infertility. Impaired oocyte quality may be involved in lower implantation rates after in vitro fertilization in these patients. We question if alterations in the follicular microenvironment of infertile patients with endometriosis might affect oocyte competence acquisition and compromise the natural fertility and assisted reproduction treatment outcomes in women with this disease. It is known that to be competent and capable of fertilizing, the oocyte must be mature and have a morphologically functional spindle, which ensure the fidelity of chromosome segregation during meiosis. Thus, the aim of this study was to evaluate the potential impact of different concentrations of follicular fluid (FF) of infertile women with and without mild endometriosis on spindle integrity, chromosomes alignment and actin microfilaments organization of bovine oocytes in vitro matured. We performed an experimental study, where FF samples were consecutively obtained from 22 infertile patients (11 with mild endometriosis and 11 with tubal or male factors of infertility) submitted to ovarian stimulation for intracytoplasmic sperm injection. Immature bovine oocytes were submitted to in vitro maturation (IVM) without FF and with 4 concentrations (1%, 5%, 10%, and 15%) of 2 samples of FF (1 from a woman with endometriosis and one from a woman without endometriosis). We performed 11 IVM and each FF sample was used only once. The oocytes were then fixed, stained by immunofluorescence for morphological visualization of microtubules, chromatin and actin microfilaments, and then, analyzed by confocal microscopy. The percentage of abnormal MII oocytes was significantly higher for those matured with FF from patients with endometriosis (1%: 55.56%, 5%: 63.26%, 10%: 54.54%, 15%: 48.84%) when compared with oocytes matured with FF from patients without endometriosis (1%: 19.15%, 5%: 23.44%, 10%: 25%, 15%: 23.81%) and those matured without FF (23.53%), with no differences among the tested concentrations in each group. We can conclude that bovine oocytes matured in vitro in the presence of FF from infertile women with mild endometriosis have higher frequency of meiotic abnormalities. These data suggest that FF from women with endometriosis may compromise oocyte quality by promoting spindle and/or chromosomal damage

Endometriose leve

Female infertility

Fluido folicular

Follicular fluid

Fuso meiótico

In vitro maturation

Infertilidade feminina

Maturação in itro

Meiotic spindle

Mild endometriosis

Oocyte quality

Qualidade oocitária

Avaliação do fuso meiótico e distribuição cromossômica de oócitos maturados in vitro de portadoras da Síndrome dos Ovários Policísticos submetidas à estimulação ovariana: estudo piloto / Avaliação do fuso meiótico e distribuição cromossômica de oócitos maturados in vitro de portadoras da Síndrome dos Ovários Policísticos submetidas à estimulação ovariana: estudo piloto

Vieira, Rodolpho Cruz

17 April 2008

Objetivos: Avaliar o fuso meiótico e a distribuição cromossômica de oócitos maturados in vitro obtidos de ciclos estimulados de mulheres inférteis com Síndrome dos Ovários Policísticos (SOP) e fatores masculino e/ou tubário de infertilidade. Métodos: Vinte e seis pacientes inférteis com SOP e 48 pacientes com fator tubário e/ou masculino de infertilidade, submetidas a ciclos estimulados para captação oocitária para injeção intracitoplasmática de espermatozóide, foram selecionadas prospectiva e consecutivamente e divididas em grupos de estudo e controle, respectivamente. Oócitos imaturos (34 e 56 oócitos) foram obtidos de 13 e 27 pacientes, respectivamente, dos grupos SOP e controle, sendo submetidos à maturação in vitro (MIV), respectivamente, por 19 horas ± 1 hora (VG) e 4 horas ± 30 minutos (MI), conforme curva de MIV previamente realizada no presente serviço. Oócitos em metáfase II (MII) após MIV, foram fixados, submetidos a imunocoloração e microscopia de fluorescência para avaliação morfológica do fuso e da distribuição cromossômica. Resultados: Não observamos diferença significativa nas taxas de MIV entre os dois grupos avaliados (50% e 42,8%, respectivamente, para os grupos SOP e controle). Na análise por microscopia de imunofluorescência, detectaram-se 3 e 2 oócitos, respectivamente, no grupo de estudo e no grupo controle, em estágio de Telófase I e 3 oócitos ativados partenogeneticamente no grupo controle. Ocorreu a impossibilidade de análise de 4 oócitos do grupo controle em virtude de dificuldades técnicas durante o processo de imunocoloração. Não houve diferença significativa nas proporções de anomalias meióticas entre os grupos SOP e controle (57,1 e 46,7%, respectivamente). Conclusões: Os dados preliminares do presente estudo, apesar de não demonstrarem aumento significativo na incidência de anomalias meióticas nas portadoras de SOP, sugerem uma tendência a maior ocorrência de anomalias meióticas nos oócitos deste grupo de pacientes, quando comparados aos de portadoras de fator masculino e/ou tubário de infertilidade, o que deverá ser mais bem avaliado em estudos com maiores casuísticas. Estes achados têm potencial clínico para apontar uma possível explicação para as controversas menores taxas de fertilização observadas em pacientes com SOP submetidas às Técnicas de Reprodução Assistida. / Objectives: To evaluate the meiotic spindle and the chromosome distribution of in vitro matured oocytes obtained during stimulated cycles from infertile women with Polycystic Ovary Syndrome (PCOS) and with male factor and/or tubal infertility. Methods: Twenty six infertile patients with PCOS and 48 patients with infertility due to tubal and/or male factor, submitted to stimulated cycles for oocyte retrieval for intracytoplasmic sperm injection, were selected prospectively and consecutively and respectively assigned to the study group and the control group. Imature oocytes (34 and 56 oocytes) were obtained from 13 and 27 patients, respectively, of PCOS and control groups, and submitted to in vitro maturation (IVM) for 19 hours ± 1 hour (GV) and 4 hours ± 30 minutes (MI) according to the IVM curve previously constructed in the present service. After IVM, oocytes in metaphase II (MII) were fixed and submitted to immunostaining and fluorescence microscopy for morphological evaluation of the spindle and of chromosome distribution. Results: IVM rates were similar between the two analyzed groups (50% e 42.8%, respectively, in PCOS e control groups). By immunofluorescence analysis, there were 3 and 2 oocytes, respectively, in PCOS e control groups, in telophase I stage, and 3 parthenogenetic activated oocytes in control group. Because of technical difficulties during the execution of the immunofluorescence protocol, 4 oocytes from the control group could not be analyzed. The difference in the proportions of meiotic anomalies between the two groups was not statistically significant (57.1 e 46.7%, respectively, in PCOS e control groups). Conclusions: The present preliminary data, although not showing a significant increase in the incidence of meiotic anomalies in women with PCOS, suggest a tendency to a higher occurrence of meiotic anomalies in the oocytes of this group of patients compared to women with male and/or tubal infertility, a fact to be better evaluated in studies on larger patient series. The present findings have the clinical potential to provide a possible explanation for the controversial lower fertilization rates observed in patients with PCOS submitted to Assisted Reproduction Techniques

ciclos estimulados

fuso meiótico

human oocyte quality

ICSI

ICSI

In Vitro Maturation

Maturação In Vitro

meiotic spindle

Polycystic Ovary Syndrome

qualidade oocitária

Síndrome dos Ovários Policísticos

stimulated cycles

O fluido peritoneal de mulheres inférteis com endometriose mínima/leve compromete o fuso meiótico de oócitos bovinos em metáfase II / Peritoneal fluid from infertile women with minimal/mild endometriosis compromises the meiotic spindle of metaphase II bovine oocytes

Jianini, Bruna Talita Gazeto Melo

30 November 2015

Os mecanismos etiopatogênicos da infertilidade relacionada à endometriose não estão bem elucidados, especialmente em mulheres com estágios iniciais da doença (mínima e leve), em que não são observadas alterações anatômicas expressivas na cavidade pélvica. Questionamos a possibilidade de haver alterações no microambiente peritoneal de mulheres inférteis com endometriose que poderiam afetar a aquisição da competência oocitária e dessa forma, comprometer a fertilidade natural dessas mulheres. Para ser competente, o oócito precisa estar maduro e ter um fuso meiótico morfologicamente normal e funcional, garantindo a fidelidade da segregação cromossômica durante as divisões da meiose. Nesse sentido, o objetivo do presente estudo foi comparar o potencial impacto de diferentes concentrações (1% e 10%) de fluido peritoneal (FP) de mulheres férteis sem endometriose e mulheres inférteis com endometriose mínima e leve (EI/II) sobre a integridade do fuso celular e alinhamento cromossômico de oócitos bovinos maturados in vitro. Realizou-se um estudo experimental, onde amostras de FP foram obtidas de 12 mulheres (6 mulheres férteis sem endometriose e 6 mulheres inférteis com endometriose mínima e leve) submetidas a videolaparoscopia, respectivamente, para realização de laqueadura tubária e investigação de infertilidade. Oócitos bovinos imaturos foram submetidos a maturação in vitro (MIV) na ausência de FP, na presença de 1% e 10% de FP de mulheres férteis sem endometriose e na presença de 1% e 10% de FP de mulheres inférteis com EI/II. Foram realizados 6 experimentos de MIV e cada amostra de FP foi utilizada em apenas um experimento. Os oócitos foram fixados, marcados por imunofluorescência e então analisados por microscopia confocal. A porcentagem de oócitos meioticamente normais foi significantemente maior nos oócitos submetidos a MIV na ausência de FP (88.46%) e na presença de 1% (78.57%) e 10% (84.62%) de FP de mulheres férteis sem endometriose do que aqueles oócitos submetidos a MIV na presença de 1% (62.50%) e 10% (56.25%) de FP de mulheres inférteis com EI/II. Além disso, no grupo endometriose, a porcentagem de oócitos meioticamente normais foi significantemente maior nos oócitos submetidos a MIV na presença de 1% (62.50%) do que na presença de 10% (56.25%) de FP, sugerindo um efeito dose-dependente do FP de mulheres com endometriose na ocorrência de danos meióticos oocitários. Demonstrou-se que o FP de mulheres inférteis com EI/II comprometeu a maturação nuclear oocitária durante a MIV, de modo dosedependente, promovendo anormalidades meióticas em oócitos em metáfase II. Nossos resultados contribuem para a compreensão dos mecanismos etiopatogênicos da infertilidade relacionada à EI/II e abrem perspectivas para o estudo de novas abordagens terapêuticas visando melhorar a fertilidade natural destas pacientes. / The etiopathogenic mechanisms of endometriosis-related infertility are not well elucidated, especially in women with early stages of the disease (minimal and mild endometriosis), where significant anatomical abnormalities in the pelvic cavity are not observed. We question if alterations in the peritoneal microenvironment of infertile women with endometriosis might affect oocyte competence acquisition and in this way, compromise the natural fertility in these women. To be competent, the oocyte must be mature and have a morphologically normal and functional meiotic spindle, which ensure the fidelity of chromosome segregation during the divisions of meiosis. Thus, the aim of the present study was to compare the potencial impact of different concentrations (1% and 10%) of peritoneal fluid (PF) from fertile women without endometriosis and infertile women with minimal and mild endometriosis (EI/II) on spindle integrity and chromosomes alignment of bovine oocytes in vitro matured (IVM). We performed an experimental study, where PF samples were obtained from 12 women (six fertile women without endometriosis and six infertile women with minimal and mild endometriosis) submitted to laparoscopy, respectively for tubal ligation and investigation of infertility. Immature bovine oocytes were submitted to IVM in the absence of PF, in the presence of 1% and 10% PF from fertile women without endometriosis and in the presence of 1% and 10% PF from infertile women with EI/II. We performed 6 experiments of IVM and each PF sample was used in only one experiment. The oocytes were fixed, immunofluorescence staining and then, analyzed by confocal microscopy. The percentage of meiotically normal oocytes was significantly higher for oocytes that underwent IVM in the absence of PF (88.46%) and in the presence of 1% (78.57%) and 10% (84.62%) PF from fertile women without endometriosis than for oocytes that underwent IVM in the presence of 1% (62.50%) and 10% (56.25%) PF from infertile women with EI/II. Furthermore, in the endometriosis group, the percentage of meiotically normal oocytes was significantly higher for oocytes that underwent IVM in the presence of 1% (62.50%) than in the presence of 10% (56.25%) PF, suggesting a dose-dependent effect of PF from women with endometriosis on the occurrence of meiotic oocyte damage. The study have demonstrated that PF from infertile women with EI/II compromised the oocyte nuclear maturation during the IVM, in a dosedependent manner, promoting meiotic abnormalities in metaphase II oocytes. Our results contribute to a better understanding of the etiopathogenic mechanisms of infertility related to EI/II and open perspectives in the design of new therapeutic approaches to improve the natural fertility of these infertile women

Endometriose mínima e leve

Female infertility

Fluido peritoneal

Fuso meiótico

Infertilidade feminina

Meiotic spindle

Minimal and mild endometriosis

Oocyte quality

Peritoneal fluid

Qualidade oocitária

Avaliação do fuso meiótico e distribuição cromossômica de oócitos maturados in vitro de portadoras da Síndrome dos Ovários Policísticos submetidas à estimulação ovariana: estudo piloto / Avaliação do fuso meiótico e distribuição cromossômica de oócitos maturados in vitro de portadoras da Síndrome dos Ovários Policísticos submetidas à estimulação ovariana: estudo piloto

Rodolpho Cruz Vieira

17 April 2008

Objetivos: Avaliar o fuso meiótico e a distribuição cromossômica de oócitos maturados in vitro obtidos de ciclos estimulados de mulheres inférteis com Síndrome dos Ovários Policísticos (SOP) e fatores masculino e/ou tubário de infertilidade. Métodos: Vinte e seis pacientes inférteis com SOP e 48 pacientes com fator tubário e/ou masculino de infertilidade, submetidas a ciclos estimulados para captação oocitária para injeção intracitoplasmática de espermatozóide, foram selecionadas prospectiva e consecutivamente e divididas em grupos de estudo e controle, respectivamente. Oócitos imaturos (34 e 56 oócitos) foram obtidos de 13 e 27 pacientes, respectivamente, dos grupos SOP e controle, sendo submetidos à maturação in vitro (MIV), respectivamente, por 19 horas ± 1 hora (VG) e 4 horas ± 30 minutos (MI), conforme curva de MIV previamente realizada no presente serviço. Oócitos em metáfase II (MII) após MIV, foram fixados, submetidos a imunocoloração e microscopia de fluorescência para avaliação morfológica do fuso e da distribuição cromossômica. Resultados: Não observamos diferença significativa nas taxas de MIV entre os dois grupos avaliados (50% e 42,8%, respectivamente, para os grupos SOP e controle). Na análise por microscopia de imunofluorescência, detectaram-se 3 e 2 oócitos, respectivamente, no grupo de estudo e no grupo controle, em estágio de Telófase I e 3 oócitos ativados partenogeneticamente no grupo controle. Ocorreu a impossibilidade de análise de 4 oócitos do grupo controle em virtude de dificuldades técnicas durante o processo de imunocoloração. Não houve diferença significativa nas proporções de anomalias meióticas entre os grupos SOP e controle (57,1 e 46,7%, respectivamente). Conclusões: Os dados preliminares do presente estudo, apesar de não demonstrarem aumento significativo na incidência de anomalias meióticas nas portadoras de SOP, sugerem uma tendência a maior ocorrência de anomalias meióticas nos oócitos deste grupo de pacientes, quando comparados aos de portadoras de fator masculino e/ou tubário de infertilidade, o que deverá ser mais bem avaliado em estudos com maiores casuísticas. Estes achados têm potencial clínico para apontar uma possível explicação para as controversas menores taxas de fertilização observadas em pacientes com SOP submetidas às Técnicas de Reprodução Assistida. / Objectives: To evaluate the meiotic spindle and the chromosome distribution of in vitro matured oocytes obtained during stimulated cycles from infertile women with Polycystic Ovary Syndrome (PCOS) and with male factor and/or tubal infertility. Methods: Twenty six infertile patients with PCOS and 48 patients with infertility due to tubal and/or male factor, submitted to stimulated cycles for oocyte retrieval for intracytoplasmic sperm injection, were selected prospectively and consecutively and respectively assigned to the study group and the control group. Imature oocytes (34 and 56 oocytes) were obtained from 13 and 27 patients, respectively, of PCOS and control groups, and submitted to in vitro maturation (IVM) for 19 hours ± 1 hour (GV) and 4 hours ± 30 minutes (MI) according to the IVM curve previously constructed in the present service. After IVM, oocytes in metaphase II (MII) were fixed and submitted to immunostaining and fluorescence microscopy for morphological evaluation of the spindle and of chromosome distribution. Results: IVM rates were similar between the two analyzed groups (50% e 42.8%, respectively, in PCOS e control groups). By immunofluorescence analysis, there were 3 and 2 oocytes, respectively, in PCOS e control groups, in telophase I stage, and 3 parthenogenetic activated oocytes in control group. Because of technical difficulties during the execution of the immunofluorescence protocol, 4 oocytes from the control group could not be analyzed. The difference in the proportions of meiotic anomalies between the two groups was not statistically significant (57.1 e 46.7%, respectively, in PCOS e control groups). Conclusions: The present preliminary data, although not showing a significant increase in the incidence of meiotic anomalies in women with PCOS, suggest a tendency to a higher occurrence of meiotic anomalies in the oocytes of this group of patients compared to women with male and/or tubal infertility, a fact to be better evaluated in studies on larger patient series. The present findings have the clinical potential to provide a possible explanation for the controversial lower fertilization rates observed in patients with PCOS submitted to Assisted Reproduction Techniques

ciclos estimulados

fuso meiótico

ICSI

Maturação In Vitro

qualidade oocitária

Síndrome dos Ovários Policísticos

human oocyte quality

ICSI

In Vitro Maturation

meiotic spindle

Polycystic Ovary Syndrome

stimulated cycles

Neural circuits engaged in mastication and orofacial nociception

Athanassiadis, Tuija

January 2009

A deeper understanding of both movement control and the effects of nociceptor inputs on our motor systems is critical for proper clinical diagnosis of musculo-skeletal dysfunctions and for development of novel rehabilitation schemes. In the jaw system, masticatory movements are produced by a central pattern generator (CPG) located in the brainstem. Considerable efforts have been made in deciphering this neuronal network. The present thesis contributes towards an increasingly detailed understanding of its essential elements, and presents a hypothesis of how deep somatic pain (i.e. muscle pain) may be evoked and interferes with the masticatory CPG circuitry. In Paper I, the expression of c-Fos-like protein was used as a molecular marker to visualize brainstem neurons that were active during induced fictive mastication in the anesthetized and paralyzed rabbit. Our findings provide a previously lacking detailed record of the neuronal populations that form the masticatory motor pattern. Certain cells were located in brainstem areas previously suggested to be involved in the masticatory CPG. However, it was a new finding that neurons in the dorsal part of the trigeminal main sensory nucleus (NVsnpr-d) may belong to this circuitry. Paper II focused on the discovered neurons in NVsnpr in an in vitro slice preparation from young rats.  Intracellular recordings allowed us to define two cell types based on their response to depolarizing current. Microstimulation applied to the trigeminal motor nucleus, its reticular border, the parvocellular reticular formation and the nucleus reticularis pontis caudalis, elicited postsynaptic potentials in 81% of the neurons tested. Responses obtained were predominately excitatory and sensitive to gluta-matergic antagonists DNQX or/and APV. Some inhibitory and biphasic responses were also evoked. Bicuculline methiodide or strychnine blocked the IPSPs indicating that they were mediated by GABAA or glycinergic receptors. About one third of the stimulations activated both types of neurons antidromically. Neurons in NVsnpr-d seem to gather all the conditions that can theoretically account for a role in masticatory rhythm generation. In Paper III, the masticatory model system was used to investigate the possible role of muscle spindle primary afferents in development of persistent musculoskeletal pain. Following intramuscular acidic (pH 4.0) saline injections of rat masseter muscles, in vitro whole cell recordings were done from jaw closing muscle spindle somata located in the trigeminal mesencephalic nucleus (NVmes). Compared to control neurons, the somata of afferents exposed to acid had more hyperpolarized membrane potentials, more hyperpolarized thresholds for firing, high frequency membrane oscillations and ectopic bursting of action potentials. These changes in membrane properties lasted for up to 35 days. Within the same time frame experi-mental animals showed hypersensitivity to touch on the skin covering the injected muscle. Similar saline injections also resulted in a significant increase of activity dependent c-Fos expression in NVmes neurons compared to controls. Immuno-fluorescence and lectin binding studies indicated that small-caliber muscle afferents containing known nociceptor markers (CGRP, SP, P2X3, TRPV1 and IB4) and expressing glutamate receptors are found close to the annulo-spiral endings of the NVmes afferents. Combined, our new observations support the hypothesis that excessive release of glutamate, within muscle spindles due to ectopically evoked antidromic action potentials, could lead to development of persistent musculoskeletal pain by activation and/ or sensitization of adjacent muscle afferent nociceptors.

Neurophysiology

Neurofysiologi

Design and Construction Modifications of Switched Reluctance Machines / Entwurf und konstruktive Modifikationen von Geschalteten Reluktanzmaschinen

Wichert, Torsten

25 February 2009

Although the design principles of the Switched Reluctance Machines (SRMs) are available in different fragments in numerous bibliography positions, there no exists the complex design procedure of whole drive system taking into account the SR Machine, control system and supply device as well. The hybrid design method for SRM drives with application of new analytical calculation methods, finite element method and simulation models is proposed in this thesis. The calculation/design system is characterised by important effectivity and reliability. The new possibilities in analytical determination of saturation effects and core losses under various modes of control, including sensorless method, are also taken into account. The correctness of the proposed design algorithms are verified by laboratory tests made on three motor prototypes manufactured in industry for concrete application. This dissertation provides the elements indispensable for more accurate and complex analysis and design of drives with switch reluctance motors. The elements of electrical motor and control system design as well as the considerations on the choice of supply device and controller subsystems are jointed in the thesis for final receiving of the design tool for considered industrial drive system.

SRM

Switched Reluctance Machine

design

drive system

spindle

gear

iron losses

Reluktanzmaschine

Antrieb

Elektronik

Getriebe

Spinnmaschine

Analytik

Berechnung

Eisenverluste

ddc:620

rvk:ZN 8210

Regulation of Mitotic Spindle Assembly in Caenorhabditis elegans Embryos / Regulation der Bildung der mitotischen Spindel in Caenorhabditis elegans embryos

Schlaitz, Anne-Lore

10 June 2007

The mitotic spindle is a bipolar microtubule-based structure that mediates proper cell division by segregating the genetic material and by positioning the cytokinesis cleavage plane. Spindle assembly is a complex process, involving the modulation of microtubule dynamics, microtubule focusing at spindle poles and the formation of stable microtubule attachments to chromosomes. The cellular events leading to spindle formation are highly regulated, and mitotic kinases have been implicated in many aspects of this process. However, little is known about their counteracting phosphatases. A screen for genes required for early embryonic cell divisions in C. elegans identified rsa-1 (for regulator of spindle assembly 1), a putative Protein Phosphatase 2A (PP2A) regulatory subunit whose silencing causes defects in spindle formation. Upon rsa-1(RNAi), spindle poles collapse onto each other and microtubule amounts are strongly reduced. My thesis work demonstrates that RSA-1 indeed functions as a PP2A regulatory subunit. RSA-1 associates with the PP2A enzyme and recruits it to centrosomes. The centrosome binding of PP2A furthermore requires the new protein RSA-2 as well as the core centrosomal protein SPD-5 and is based on a hierarchical protein-protein interaction pathway. When PP2A is lacking at centrosomes after rsa-1(RNAi), the centrosomal amounts of two critical mitotic effectors, the microtubule destabilizer KLP-7 and the kinetochore microtubule stabilizer TPXL-1, are altered. KLP-7 is increased, which may account for the reduction of microtubule outgrowth from centrosomes in rsa-1(RNAi) embryos. TPXL-1 is lost from centrosomes, which may explain why spindle poles collapse in the absence of RSA-1. TPXL-1 physically associates with RSA-1 and RSA-2, suggesting that it is a direct target of PP2A. In summary, this work defines the role of a novel PP2A complex in mitotic spindle assembly and suggests a model for how different microtubule re-organization steps might be coordinated during spindle formation.

mitosis

spindle assembly

protein phosphatase 2A

centrosome

microtubule

Caenorhabditis elegans embryo

Mitose

mitotische Spindel

Protein Phosphatase 2A

Centrosom

Mikrotubulus

Caenorhabditis elegans Embryo

ddc:570

rvk:WG 2100

THE ROLE OF RAPID EYE MOVEMENT AND SLOW WAVE SLEEP FOR THE CONSOLIDATION OF MEMORY IN RATS

Fogel, STUART

26 October 2009

The functions of sleep remain enigmatic. One of the dominant, yet more contentious hypotheses is that sleep is involved in memory consolidation. A large body of evidence supports the role of rapid eye movement (REM) sleep in memory consolidation, especially in rodents. In humans, the role of REM sleep in memory consolidation has also been investigated, however it is unclear if it supports only one type of memory, or consolidation for several memory systems. Recent evidence suggests that non-REM is also involved in memory consolidation. The role of theta activity during REM and sleep spindles during non-REM may provide electrophysiological signatures reflecting memory consolidation processes. The studies presented here attempt to further investigate the electrophysiological characteristics of the learning-dependent changes in REM and slow wave sleep (SWS) in rats. A 2-stage model of memory consolidation is outlined here, and both steps of the model were investigated. Consistent with previous studies, REM increases were observed following avoidance training. During this period, theta power during REM sleep was increased compared to non-learning rats. Increased sleep spindle density during SWS was observed following REM increases. When REM sleep was suppressed by infusing the GABAB agonist baclofen into the pedunculopontine nucleus, avoidance performance acquisition was impaired. Baseline sleep spindles predicted whether rats were able to learn to make avoidance responses. Results suggest that both REM and SWS may be sequentially involved in memory consolidation processes. Discrete periods (windows) exist for REM and SWS when memory consolidation processes appear to take place. Theta activity during REM sleep from 17- 20 h on the first post-training day and sleep spindles during SWS from 21-24 h on the first post- training day are increased in learning rats and are related to memory performance. / Thesis (Ph.D, Neuroscience Studies) -- Queen's University, 2009-10-26 12:07:47.515

sleep

memory

electroencephalogram (EEG)

rat

spindle

rapid eye movement (REM)

slow wave sleep (SWS)

theta

pedunculopontine nucleus

deep mesencephalic reticular nucleus

baclofen

GABA

learning

Bcl-xL regulation and function in cell cycle checkpoints and progression

Wang, Jianfang

06 1900

Quelques évidences suggèrent que Bcl-xL, un membre anti-apoptotique de la famille Bcl-2, possède également des fonctions au niveau du cycle cellulaire et de ses points-contrôle. Pour étudier la régulation et fonction de Bcl-xL au cours du cycle cellulaire, nous avons généré et exprimé dans des cellules humaines une série de mutants de phosphorylation incluant Thr41Ala, Ser43Ala, Thr47Ala, Ser49Ala, Ser56Ala, Ser62Ala et Thr115Ala. L'analyse de cette série de mutants révèle que les cellules exprimant Bcl-xL(Ser62Ala) sont moins stables au point-contrôle G2 du cycle cellulaire comparées aux cellules exprimant le type sauvage ou les autres mutants de phosphorylation incluant Thr41Ala, Ser43Ala, Thr47Ala, Ser56Ala et Thr115Ala. Les études de cinétiques de phosphorylation et de localisation de phospho-Bcl-xL(Ser62) dans des cellules synchronisées et suite à l'activation du point-contrôle en G2 médié par l'étoposide (VP16), nous indiquent que phospho-Bcl-xL(Ser62) migre dans les corps nucléolaires durant l'arrêt en G2 dans les cellules exposées au VP16. Une série d'expériences incluant des essais kinase in vitro, l'utilisation d'inhibiteurs pharmacologiques et d'ARN interférant, nous révèlent que Polo kinase 1 (PLK1) et MAPK9/JNK2 sont les protéines kinase impliquées dans la phosphorylation de Bcl-xL(Ser62), et pour son accumulation dans les corps nucléolaires pendant le point-contrôle en G2. Nos résultats indiquent que durant le point-contrôle en G2, phospho-Bcl-xL(Ser62) se lie et se co-localise avec CDK1(CDC2), le complexe cycline-kinase qui contrôle l'entrée en mitose. Nos résultats suggèrent que dans les corps nucléolaires, phospho-Bcl-xL(Ser62) stabilise l'arrêt en G2 en séquestrant CDK1(CDC2) pour retarder l'entrée en mitose. Ces résultats soulignent également que les dommages à l'ADN influencent la composition des corps nucléolaires, structure nucléaire qui émerge maintenant comme une composante importante de la réponse aux dommages à l'ADN. Dans une deuxième étude, nous décrivons que les cellules exprimant le mutant de phosphorylation Bcl-xL(Ser62Ala) sont également plus stables au point-contrôle de l'assemblage du fuseau de la chromatine (SAC) suite à une exposition au taxol, comparées aux cellules exprimant le type sauvage ou d'autres mutants de phosphorylation de Bcl-xL, incluant Thr41Ala, Ser43Ala, Thr47Ala, Ser56Ala. Cet effet est indépendent de la fonction anti-apoptotique de Bcl-xL. Bcl-xL(Ser62) est fortement phosphorylé par PLK1 et MAPK14/SAPKp38α à la prométaphase, la métaphase et à la frontière de l'anaphase, et déphosphorylé à la télophase et la cytokinèse. Phospho-Bcl-xL(Ser62) se trouve dans les centrosomes avec γ-tubuline, le long du fuseau mitotique avec la protéine moteure dynéine et dans le cytosol mitotique avec des composantes du SAC. Dans des cellules exposées au taxol, phospho-Bcl-xL(Ser62) se lie au complexe inhibiteur CDC20/MAD2/BUBR1/BUB3, alors que le mutant Bcl-xL(Ser62Ala) ne se lie pas à ce complexe. Ces résultats indiquent que durant le SAC, la phosphorylation de Bcl-xL(Ser62) accélère la résolution du SAC et l'entrée des cellules en anaphase. Des expériences bloquant l'expression de Bcl-xL révèlent ègalement un taux très élevé de cellules tétraploïdes et binuclées après un traitement au nocodazole, consistant avec une fonction de Bcl-xL durant la mitose et dans la stabilité génomique. Dans la troisième étude, l'analyse fonctionnelle de cette série de mutants de phosphorylation indique également que les cellules exprimant Bcl-xL(Ser49Ala) sont moins stables durant le point-contrôle G2 et entre en cytokinèse plus lentement dans des cellules exposées aux inhibiteurs de la polymérisation/dépolymérisation des tubulines, composantes des microtubules. Ces effets de Bcl-xL(Ser49Ala) sont indépendents de sa fonction anti-apoptotique. La phosphorylation de Bcl-xL(Ser49) est dynamique au cours du cycle cellulaire. Dans des cellules synchronisées, Bcl-xL(Ser49) est phosphorylé en phase S et G2, déphosphorylé à la prométaphase, la métaphase et à la frontière de l'anaphase, et re-phosphorylé durant la télophase et la cytokinèse. Au cours du point-contrôle G2 induit par les dommages à l'ADN, un pool important de phospho-Bcl-xL(Ser49) se trouve aux centrosomes, un site important pour la régulation de l'entrée en mitose. Durant la télophase et la cytokinèse, phospho-Bcl-xL(Ser49) se trouve le long des microtubules avec la protéine moteure dynéine et dans le cytosol mitotique. Finalement, nos résultats suggèrent que PLK3 est responsable de la phosphorylation de Bcl-xL(Ser49), une protéine kinase impliquée pour l'entrée des cellules en mitose et pour la progression de la mitose jusqu'à la division cellulaire. / Accumulating evidence suggest that Bcl-xL, an anti-apoptotic member of the Bcl-2 family, also functions in cell cycle progression and cell cycle checkpoints. To further understand Bcl-xL regulation and function in cell cycle progression, we first expressed a series of single-point Bcl-xL cDNA phospho-mutants, including Thr41Ala, Ser43Ala, Thr47Ala, Ser49Ala, Ser56Ala, Ser62Ala and Thr115Ala in human cancer cell lines and investigated their impact on cell cycle progression. Analysis of this series of phosphorylation mutants reveals that cells expressing Bcl-xL(Ser62Ala) mutant are less stable at the G2 checkpoint and enter mitosis more rapidly than cells expressing wild type Bcl-xL or Bcl-xL phosphorylation mutants, including Thr41Ala, Ser43Ala, Thr47Ala, Ser56Ala and Thr115Ala. Dynamic phosphorylation and location studies on phospho-Bcl-xL(Ser62) in unperturbed, synchronized cells and during DNA damage-induced G2 arrest revealed that phospho-Bcl-xL(Ser62) translocates into nucleolar structures in VP16-exposed cells during G2 arrest. Using in vitro kinase assays, pharmacological inhibitors and specific siRNAs experiments, we found that Polo kinase 1 and MAPK9/JNK2 are major protein kinases involved in Bcl-xL(Ser62) phosphorylation and accumulation into nucleolar structures during the G2 checkpoint. In nucleoli, phospho-Bcl-xL(Ser62) binds to and co-localizes with CDK1(CDC2), the key cyclin-dependent kinase required for entry into mitosis. These data indicate that, during G2 checkpoint, phospho-Bcl-xL(Ser62) stabilizes G2 arrest by timely trapping CDK1(CDC2) in nucleolar structures to slow mitotic entry. It also highlights that DNA damage affects the dynamic composition of the nucleolus, which now emerges as a key event in the DNA damage response. In a second study, we describe that cells expressing Bcl-xL(Ser62Ala) are also more stable at a sustained spindle-assembly checkpoint (SAC) after exposure to taxol than cells expressing wild-type Bcl-xL or other mutants, an effect that appears to be independent of its anti-apoptotic activity. Bcl-xL(Ser62) is strongly phosphorylated by PLK1 and MAPK14/SAPKp38α at prometaphase, metaphase and the anaphase boundary, while it is dephosphorylated at telophase and cytokinesis. Phospho-Bcl-xL(Ser62) localizes in centrosomes with γ-tubulin, along the mitotic spindle with dynein motor protein and in cytosol with SAC signaling components. In taxol-exposed cells, phospho-Bcl-xL(Ser62) binds to the CDC20/MAD2/BUBR1/BUB3 complex, while Bcl-xL(Ser62Ala) does not. The data indicate that during SAC, Bcl-xL(Ser62) phosphorylation accelerates SAC resolution and cell entry into anaphase, even in the presence of unattached or misaligned chromosomes. Silencing Bcl-xL expression also leads nocodazole-exposed cells to tetraploidy and binucleation, consistent with a Bcl-xL function in SAC and genomic stability. In the third study, the functional analysis of a Bcl-xL phosphorylation mutant series has revealed that cells expressing Bcl-xL(Ser49Ala) mutant are less stable at G2 checkpoint after DNA damage and enter cytokinesis much more slowly after microtubule poisoning than cells expressing wild-type Bcl-xL. These effects of Bcl-xL(Ser49Ala) mutant seem to be distinct from Bcl-xL function in apoptosis. Bcl-xL(Ser49) phosphorylation is cell cycle-dependent. In synchronized cells, phospho-Bcl-xL(Ser49) appears during the S phase and G2, whereas it disappears rapidly in early mitosis during prometaphase, metaphase and early anaphase, and re-appears during telophase and cytokinesis. During DNA damage-induced G2 arrest, an important pool of phospho-Bcl-xL(Ser49) accumulates in centrosomes which act as essential decision centers for progression from G2 to mitosis. During telophase/cytokinesis, phospho-Bcl-xL(Ser49) is found along microtubules and at midbody with dynein motor protein. In a series of in vitro kinase assays, specific small interfering RNA and pharmacological inhibition experiments, polo kinase 3 (PLK3) was implicated in Bcl-xL(Ser49) phosphorylation. These data indicate that during G2 checkpoint phospho-Bcl-xL(Ser49) is another downstream target of PLK3, acting to stabilize G2 arrest. Bcl-xL phosphorylation at Ser49 also correlates with essential PLK3 activity and function, enabling cytokinesis and mitotic exit.

Bcl-xL

Bcl-xL

phosphorylation

phosphorylation

cycle cellulaire

cell cycle

point-contrôle G2

G2 checkpoint

mitose

spindle-assembly checkpoint

Dynamic Modeling Of Spindle-tool Assemblies In Machining Centers

Erturk, Alper

01 May 2006

Regenerative chatter is a well-known machining problem that results in unstable cutting process, poor surface quality, reduced material removal rate and damage on the machine tool itself. Stability lobe diagrams supply stable depth of cut &amp / #8211 / spindle speed combinations and they can be used to avoid chatter. The main requirement for generating the stability lobe diagrams is the system dynamics information at the tool tip in the form of point frequency response function (FRF). In this work, an analytical model that uses structural coupling and modification methods for modeling the dynamics of spindle-holder-tool assemblies in order to obtain the tool point FRF is presented. The resulting FRF obtained by the model can be used in the existing analytical and numerical models for constructing the stability lobe diagrams. Timoshenko beam theory is used in the model for improved accuracy and the results are compared with those of Euler-Bernoulli beam theory. The importance of using Timoshenko beam theory in the model is pointed out, and the circumstances, under which the theory being used in the model becomes more important, are explained. The model is verified by comparing the results obtained by the model with those of a reliable finite element software for a case study. The computational superiority in using the model developed against the finite element software is also demonstrated. Then, the model is used for studying the effects of bearing and contact dynamics at the spindle-holder and holder-tool interfaces on the tool point FRF. Based on the results of the effect analysis, a new approach is suggested for the identification of bearing and interface parameters from experimental measurements, which is demonstrated on a spindle-holder-tool assembly. The model is also employed for studying the effects of design and operational parameters on the tool point FRF, from the results of which, suggestions are made regarding the design of spindles and selection of operational parameters. Finally, it is experimentally demonstrated that the stability lobe diagram of an assembly can be predicted pretty accurately by using the model proposed, and furthermore the stability lobe diagram can be modified in a predictable manner for improving chatter stability.