Embryonic stem cells alter cardiomyocyte electrophysiological properties

Karan, Priyanka

15 July 2008

Embryonic stem cells (ESCs) are being considered as a cell source for cardiac regeneration because of their potency and availability. We studied the electrophysiological implications using co-cultures of ESCs and neonatal rat ventricular myocytes (NRVM) grown on a multi-electrode array (MEA). To mimic expected engraftment rates 5% mouse ESCs were co-cultured with NRVMs. Comparing cultures without and with 5% ESCs at 4 days, the mean bipolar field potential duration (FPD) of NRVMs increased from 26.3 ± 2.2 ms (n=10) to 44.3 ± 6.2 ms (n=9; p < 0.05), the interspike interval (ISI) increased from 358.3 ± 62.8 ms (n=10) to 947.8 ± 214.6 ms (n=7; p < 0.01), and conduction velocity (CV) decreased from 14.2 ± 1.3 cm/s (n=8) to 4.6 ± 1.2 cm/s (n=5; p < 0.01). To evaluate whether ESC were having direct or paracrine effects on NRVMs, media conditioned by 3x106 ESCs for 24 hr was diluted 1:1 with fresh media and then introduced to NRVM cultures on the day of plating. Conditioned media was changed daily and altered mean FPD, ISI, and CV to 46.1 ± 7.8 ms, ISI to 682.0 ± 128.5 ms, and 4.2 ± 0.4 cm/s (n=8; p < 0.01 for each measure), respectively at 4 days. However, changes were not seen in media that was incubated for 24hrs and diluted 1:1 with fresh media and introduced to NRVM cultures in a similar fashion (n=7; p > 0.05). Slowed CV is associated with increased arrhythmic risk and reports demonstrate an inverse relationship between CV and nonphosphorylated Cx43(NP-Cx43). Western blots for total Cx43 expression revealed a decrease in ratio of P-Cx43/NP-Cx43 in the 5% mouse ESCs and ESC conditioned media cultures as compared to controls (n=8; p < 0.01 for each). There was not significant increase in the total Cx43 expression (n=6; p > 0.05). Culturing ESCs with NRVMs resulted in a decreased ISI, prolonged FPD, and slowed CV of the co-cultures as compared to controls leading to pro-arrhythmic conditions. Similar effects on NRVMs were observed when applying media conditioned by ESCs, suggesting that the electrophysiological changes were mediated by soluble factors. The increase in NP-Cx43 leads to gap junction uncoupling being a potential mechanism for these arrhythmogenic substrates. Further research into preventing NP-Cx43 in cultures is currently underway.

Paracrine factors

Microelectrode arrays

Arrhythmias

Embryonic stem cells

Cardiomyoplasty

Embryonic stem cells

Electrophysiology

Estratégias para indução de competência de oócitos bovinos com atividade da enzima glicose 6-fosfato desidrogenase

Salviano, Mauricio Barbosa

January 2014

O objetivo deste trabalho foi modificar os procedimentos da maturação in vitro (MIV) para induzir a competência de oócitos bovinos com intensa atividade da enzima glicose 6-fosfato desidrogenase (G6PDH), determinada pelo emprego do corante vital Azul de Cresil Brilhante (BCB). Foram realizados dois experimentos; no primeiro trabalho foi realizada a MIV de oócitos após a identificação da atividade da G6PDH, empregando-se a seguinte proporção: competentes (sem atividade enzimática)/não competentes - 10:01, respectivamente. Os resultados revelaram um efeito negativo dos oócitos não competentes sobre a capacidade dos competentes em realizarem a MIV, a FIV e a CIV. Os resultados sugerem que para aumentar a produção de embriões deve-se realizar a MIV de oócitos competentes e não competentes, separadamente. O objetivo do segundo experimento foi verificar se a prolongação do tempo de MIV (30h) afetaria as taxas de MIV, FIV e CIV obtidas a partir de oócitos não competentes. Os oócitos não competentes não foram afetados, positiva ou negativamente, pelo prolongamento do tempo de MIV, no entanto, os oócitos competentes sofreram decréscimo na capacidade de serem fecundados e desenvolverem-se até o estágio de blastocistos. Podemos concluir que as modificações realizadas no procedimento da MIV não foram capazes de induzir competência em oócitos com intensa atividade da enzima G6PDH. / The present work aimed modify the in vitro maturation (IVM) procedure to induce competence of bovine oocytes with high glucose 6-phosphate dehydrogenase (G6PDH) activity. Two experiments were carried out; the first non-competent oocytes (with high enzymatic activity) were matured with competent oocyte (lower G6PDH activity) on proportion of 1:10, respectively. The second experiment aimed observe the effect of prolonged IVM (from 24 to 30h) on the cleavage and development rates in oocytes with higher enzymatic activity. Our data showed that oocytes with lower enzymatic activity did not induce competence of higher G6PDH activity oocyte. However, we observed a negatively effect on the cleavage and development rates on oocytes competent, then, to increase the number of embryos in vitro produced we need to mature oocytes competent and non-competent separately. In the second experiment, the non-competent gametes submitted to prolonged IVM were not affected, however, competent oocytes were negatively affect by prolonged IVM. We can concluded that the IVM modifications did not able to induce the competence in the oocytes with high G6PDH activity.

Reprodução animal

Biotécnicas de reprodução

Maturação in vitro

Oócitos

BCB test

Complex cumulus-oocyte

In vitro maturation

Paracrine effect

Estratégias para indução de competência de oócitos bovinos com atividade da enzima glicose 6-fosfato desidrogenase

Salviano, Mauricio Barbosa

January 2014

O objetivo deste trabalho foi modificar os procedimentos da maturação in vitro (MIV) para induzir a competência de oócitos bovinos com intensa atividade da enzima glicose 6-fosfato desidrogenase (G6PDH), determinada pelo emprego do corante vital Azul de Cresil Brilhante (BCB). Foram realizados dois experimentos; no primeiro trabalho foi realizada a MIV de oócitos após a identificação da atividade da G6PDH, empregando-se a seguinte proporção: competentes (sem atividade enzimática)/não competentes - 10:01, respectivamente. Os resultados revelaram um efeito negativo dos oócitos não competentes sobre a capacidade dos competentes em realizarem a MIV, a FIV e a CIV. Os resultados sugerem que para aumentar a produção de embriões deve-se realizar a MIV de oócitos competentes e não competentes, separadamente. O objetivo do segundo experimento foi verificar se a prolongação do tempo de MIV (30h) afetaria as taxas de MIV, FIV e CIV obtidas a partir de oócitos não competentes. Os oócitos não competentes não foram afetados, positiva ou negativamente, pelo prolongamento do tempo de MIV, no entanto, os oócitos competentes sofreram decréscimo na capacidade de serem fecundados e desenvolverem-se até o estágio de blastocistos. Podemos concluir que as modificações realizadas no procedimento da MIV não foram capazes de induzir competência em oócitos com intensa atividade da enzima G6PDH. / The present work aimed modify the in vitro maturation (IVM) procedure to induce competence of bovine oocytes with high glucose 6-phosphate dehydrogenase (G6PDH) activity. Two experiments were carried out; the first non-competent oocytes (with high enzymatic activity) were matured with competent oocyte (lower G6PDH activity) on proportion of 1:10, respectively. The second experiment aimed observe the effect of prolonged IVM (from 24 to 30h) on the cleavage and development rates in oocytes with higher enzymatic activity. Our data showed that oocytes with lower enzymatic activity did not induce competence of higher G6PDH activity oocyte. However, we observed a negatively effect on the cleavage and development rates on oocytes competent, then, to increase the number of embryos in vitro produced we need to mature oocytes competent and non-competent separately. In the second experiment, the non-competent gametes submitted to prolonged IVM were not affected, however, competent oocytes were negatively affect by prolonged IVM. We can concluded that the IVM modifications did not able to induce the competence in the oocytes with high G6PDH activity.

Reprodução animal

Biotécnicas de reprodução

Maturação in vitro

Oócitos

BCB test

Complex cumulus-oocyte

In vitro maturation

Paracrine effect

Estratégias para indução de competência de oócitos bovinos com atividade da enzima glicose 6-fosfato desidrogenase

Salviano, Mauricio Barbosa

January 2014

O objetivo deste trabalho foi modificar os procedimentos da maturação in vitro (MIV) para induzir a competência de oócitos bovinos com intensa atividade da enzima glicose 6-fosfato desidrogenase (G6PDH), determinada pelo emprego do corante vital Azul de Cresil Brilhante (BCB). Foram realizados dois experimentos; no primeiro trabalho foi realizada a MIV de oócitos após a identificação da atividade da G6PDH, empregando-se a seguinte proporção: competentes (sem atividade enzimática)/não competentes - 10:01, respectivamente. Os resultados revelaram um efeito negativo dos oócitos não competentes sobre a capacidade dos competentes em realizarem a MIV, a FIV e a CIV. Os resultados sugerem que para aumentar a produção de embriões deve-se realizar a MIV de oócitos competentes e não competentes, separadamente. O objetivo do segundo experimento foi verificar se a prolongação do tempo de MIV (30h) afetaria as taxas de MIV, FIV e CIV obtidas a partir de oócitos não competentes. Os oócitos não competentes não foram afetados, positiva ou negativamente, pelo prolongamento do tempo de MIV, no entanto, os oócitos competentes sofreram decréscimo na capacidade de serem fecundados e desenvolverem-se até o estágio de blastocistos. Podemos concluir que as modificações realizadas no procedimento da MIV não foram capazes de induzir competência em oócitos com intensa atividade da enzima G6PDH. / The present work aimed modify the in vitro maturation (IVM) procedure to induce competence of bovine oocytes with high glucose 6-phosphate dehydrogenase (G6PDH) activity. Two experiments were carried out; the first non-competent oocytes (with high enzymatic activity) were matured with competent oocyte (lower G6PDH activity) on proportion of 1:10, respectively. The second experiment aimed observe the effect of prolonged IVM (from 24 to 30h) on the cleavage and development rates in oocytes with higher enzymatic activity. Our data showed that oocytes with lower enzymatic activity did not induce competence of higher G6PDH activity oocyte. However, we observed a negatively effect on the cleavage and development rates on oocytes competent, then, to increase the number of embryos in vitro produced we need to mature oocytes competent and non-competent separately. In the second experiment, the non-competent gametes submitted to prolonged IVM were not affected, however, competent oocytes were negatively affect by prolonged IVM. We can concluded that the IVM modifications did not able to induce the competence in the oocytes with high G6PDH activity.

Reprodução animal

Biotécnicas de reprodução

Maturação in vitro

Oócitos

BCB test

Complex cumulus-oocyte

In vitro maturation

Paracrine effect

PARACRINE/AUTOCRINE ACTIONS OF INSULIN-LIKE GROWTH FACTOR I (IGF-I) IN TRANSGENIC MICE: EFFECTS OF IGF-I IN BONE AND SMOOTH MUSCLE CELLS IN VIVO

Zhao, Guisheng

11 October 2001

No description available.

Insulin-like growth factor I (IGF-I)

Paracrine/autocrine action

Transgenic mouse

Bone

Smooth Muscle Cells

Traitement de l'insuffisance cardiaque : de la transplantation à la thérapie cellulaire

Nguyen, Anthony

08 1900

La transplantation demeure le traitement de choix de l’insuffisance cardiaque (IC) et ce malgré les récents progrès des techniques de support d’assistance mécanique. Une amélioration considérable de la prévention et du traitement du rejet aigu a été réalisée ces 20 dernières années. Cependant, le succès à long terme des transplantations d’organes a été peu modifié : il est toujours compromis par la survenue d'une dysfonction chronique du greffon. Ainsi, l'avenir des transplantés cardiaques demeure sombre et représente un fardeau médical avec un impact socioéconomique important. Toutefois, la recherche a récemment mis en avant l'énorme potentiel de régénération des cellules souches (CS) et représenterait une nouvelle avenue thérapeutique pour les patients souffrant d’IC. Une meilleure compréhension des processus biologiques des CS et de leur interaction avec le cœur transplanté, permettrait d’exploiter pleinement leur potentiel de réparation cardiaque. Le but de cette thèse est d’explorer les différents aspects du traitement de l’IC en 2020. Les hypothèses proposées dans cette thèse sont les suivantes : (1) les excellents résultats obtenus (>20 ans de survie) chez près d’1/3 des patients greffés lors de la 1ère décade de notre expérience à ICM serait difficile à obtenir de nos jours à la vue de l’évolution d’une population plus malade et plus âgée; (2) le cœur artificiel total (CAT) temporaire Syncardia permet d’amener des patients en insuffisance cardiaque terminale à la greffe de façon satisfaisante; (3) la thérapie cellulaire, plus spécifiquement les CS d’origine adipeuse (ASC) sous forme sphéroïdes, permet de diminuer l’impact de la vasculopathie du greffon cardiaque; et (4) l’effet paracrine des ASC permet une diminution de l’inflammation dans un modèle expérimental de péritonite chez le rat. / Transplantation remains the preferred treatment for heart failure (HF) despite recent advances in mechanical support devices. A considerable improvement in the prevention and treatment of acute rejection has been achieved over the past 20 years. However, the long-term survival of organ transplants has not been changed: it is still compromised by the occurrence of chronic graft dysfunction. Thus, the future of cardiac transplant patients remains bleak and represents a medical burden with a significant socio-economic impact. However, research has recently highlighted the potential for regeneration of stem cells (SC) and would represent a new therapeutic avenue for patients with HF. A better understanding of the biological processes of SC and their interaction with the transplanted heart would allow them to fully exploit their cardiac repair potential. The aim of this thesis is to explore the various aspects of the treatment of HF in 2020. The hypotheses proposed in this thesis are as follows: (1) the excellent results obtained (> 20 years of survival) in almost 1/3 of the patients transplanted during the 1st decade of our experience at ICM would be difficult to obtain from our days at the sight of the evolution of a sicker and older population; (2) the temporary Syncardia total artificial heart (CAT) allows patients with end-stage heart failure to be transplanted satisfactorily; (3) cell therapy, more specifically CS of adipose origin (ASC) cultured as spheroid, reduce the impact of cardiac allograft vasculopathy (CAV); and (4) the paracrine effect of ASCs reduces inflammation in a rat experimental model of peritonitis.

Insuffisance cardiaque

Rejet chronique

Thérapie cellulaire

Régénération myocardite

Effet paracrine

Cellules souches mésenchymateuses

Heart failure

Chronic rejection

Cellular therapy

Myocardial regeneration

Paracrine effect

Mesenchymal stem cells

The small GTPases Ras and Rap1 bind to and control TORC2 activity

Khanna, Ankita, Lotfi, Pouya, Chavan, Anita J., Montaño, Nieves M., Bolourani, Parvin, Weeks, Gerald, Shen, Zhouxin, Briggs, Steven P., Pots, Henderikus, Van Haastert, Peter J. M., Kortholt, Arjan, Charest, Pascale G.

13 May 2016

Target of Rapamycin Complex 2 (TORC2) has conserved roles in regulating cytoskeleton dynamics and cell migration and has been linked to cancer metastasis. However, little is known about the mechanisms regulating TORC2 activity and function in any system. In Dictyostelium, TORC2 functions at the front of migrating cells downstream of the Ras protein RasC, controlling F-actin dynamics and cAMP production. Here, we report the identification of the small GTPase Rap1 as a conserved binding partner of the TORC2 component RIP3/SIN1, and that Rap1 positively regulates the RasC-mediated activation of TORC2 in Dictyostelium. Moreover, we show that active RasC binds to the catalytic domain of TOR, suggesting a mechanism of TORC2 activation that is similar to Rheb activation of TOR complex 1. Dual Ras/Rap1 regulation of TORC2 may allow for integration of Ras and Rap1 signaling pathways in directed cell migration.

CONTROLS CELL-ADHESION

DICTYOSTELIUM-DISCOIDEUM

SIGNAL RELAY

MACROPHAGES PROMOTE

MEDIATED ACTIVATION

ACTIN CYTOSKELETON

PARACRINE LOOP

G-PROTEINS

CHEMOTAXIS

MIGRATION

La protéine apparentée à l'hormone parathyroïdienne (PTHrP) dans la biologie de la cellule mésangiale : rôles dans l'inflammation, la croissance et la survie

Hochane, Mazène

28 September 2012

La glomérulonéphrite mésangioproliférative (GNMP) se caractérise par une inflammation locale et la prolifération et l'apoptose des cellules mésangiales (CM). La protéine apparentée à l'hormone parathyroïdienne (PTHrP) a été impliquée dans ces processus dans divers types cellulaires. Nous avons analysé les effets de la PTHrP sur ces processus dans les CM. Nous montrons que la PTHrP majore la prolifération des CM par voie intracrine et diminue leur apoptose par voie paracrine. La PTHrP stimule les voies de l'AMPc/PKA et PI3-K/Akt conduisant à l'activation du NFkB et à la majoration de la cyclooxygénase-2 (Cox-2). La Cox-2 était responsable de la survie des CM par la PTHrP. Par ailleurs, l'IL-1beta et le TNF-alpha majorent l'expression de la PTHrP dans les CM, et la PTHrP elle-même induisait l'expression de cytokines et chimiokines. L'expression des cytokines (IL-17, IL-16), était brève (pic à 2h). L'expression des chimiokine (RANTES, MIP-2, TARC et I-TAC) était plus prolongée (4h). Dans un modèle murin de GNMP, la PTHrP était surexprimée à J1 dans les glomérules malades. Elle pourrait contribuer à l'inflammation locale, à la prolifération et à la survie des CM.

Cellule mésangiale

PTHrP

Prolifération

Apoptose

Inflammation

Intracrine

Paracrine

Papel da interação parácrina entre astrócitos e pinealócitos na mediação do efeito potenciador da angiotensina II sobre a síntese de melatonina induzida pela estimulação noradrenérgica na glândula pineal de ratos. / Paracrine interaction between glial cells and pinealocytes determines the potentiating effects of angiotensin II on noradrenaline-stimulated melatonin synthesis on the rat pineal gland.

Moriconi, Sabrina Heloisa José dos Santos

15 April 2008

Estudos anteriores de literatura indicavam que o sistema renina-angiotensina II local pineal era de fundamental importância para a expressão plena da capacidade de síntese de melatonina induzida pela estimulação noradrenérgica pelos pinealócitos. Essa relação funcional estava na dependência de uma interação parácrina entre pinealócitos e astrócitos onde os astrócitos seriam os responsáveis pela síntese de angiotensina II que, liberada pela ação da noradrenalina, agiria em receptores do tipo AT1 existentes na membrana dos pinealócitos. O objetivo desse trabalho foi o de, uma vez estabelecida a metodologia de dissociação e cultivo dos tipos celulares, estudar a hipótese acima, além das possíveis vias de transdução intrapinealocitárias que levassem ao efeito potenciador da angiotensina II sobre a estimulação noradrenérgica no processo de síntese de melatonina. Os resultados mostraram que, diferentemente do que acontece com glândulas intactas ou com co-cultura (cultura contendo astrócitos e pinealócitos), a estimulação noradrenérgica de pinealócitos isolados não é passível de bloqueio por Losartan, uma droga bloqueadora de receptores AT1. Por outro lado, nas mesmas condições experimentais, a síntese de melatonina induzida pela estimulação noradrenérgica é passível de potenciação pela adição de angiotensina II , efeito esse, que é bloqueado pelo Losartan. Demonstrou-se, ainda, que a estimulação noradrenérgica de astrócitos isolados, provoca a liberação de angiotensina II por esse tipo celular. Demonstrou-se, ainda, que há a mobilização de pelo menos duas vias de transdução nos pinealócitos quando estimulados pela angiotensina II: aumento da concentração de cálcio intracelular e mobilização de processos de fosforilação em tirosina usando as vias das proteínas JAK/ STAT. Dessa forma, pelo presente trabalho pode- se especular que quando a glândula pineal é estimulada pela liberação de noradrenalina dos terminais simpáticos, ao mesmo tempo que esta age nos pinealócitos promovendo a via de síntese de melatonina, age, também, nos 7 astrócitos, liberando angiotensina II que, por sua vez, age nos pinealócitos potenciando a ação estimulatória da noradrenalina, levando a um aumento da síntese de melatonina. / We have previously demonstrated that Angiotensin II (Ang II) potentiates the noradrenaline-stimulated (Nor+) melatonin synthesis in the rat pineal gland [Baltatu et al.,J. Neurochem.(2002)80, 328-334]. The aim of the present paper was to study the possible paracrine interactions between glial cells and pinealocytes in the rat pineal gland. To accomplish this aim, after standard pineal cell dissociation we studied the two cellular types separated in different cell cultures, either of glial pineal cells or pinealocytes. First, we showed, using freshly dissociated pineal cells, that Losartan is able to reduce Nor+ induced melatonin synthesis, similarly to what happens with pineal glands culture. Noradrenaline stimulation is able to induce melatonin synthesis in glial cell-free pinealocytes cell culture, what is not blocked by Losartan. In this condition, Ang II is able to potentiated the Nor+ induced melatonin synthesis, an AngII effect that is blocked by Losartan. Moreover, Ang II stimulated pinealocytes show an increase in Ca2+ current as evaluated by confocal microscopy. On the other hand, pinealocytes-free glial cells cultures when stimulated by noradrenaline release Ang II in the culture medium. Taking into account the above results it is possible to speculate that in the intact pineal gland noradrenaline released by sympathetic terminals stimulated pinealocytes inducing the well know process of melatonin synthesis at the same time that stimulate glial cells that release AngII that acting through AT1 receptors in pinealocytes potentiate melatonin synthesis by the inducing an increase in the intracellular Ca2+ pool and tyrosine phosphorylation of JAK/STAT complex.

Angiotensin II

Angiotensina II

Astrócitos

Astrocytes

Glândula pineal

Interação parácrina

Melatonin

Melatonina

Paracrine interaction

Pineal gland

Pinealócitos

Pinealocytes

Paracrine factors of vascular endothelial cells facilitate cardiomyocyte differentiation of mouse embryonic stem cells

日高, 京子, Hidaka, Kyoko, 三輪, 佳子, Miwa, Keiko, 室原, 豊明, Murohara, Toyoaki, 笠井, 謙次, Kasai, Kenji, 佐賀, 信介, Saga, Shinsuke, 森崎, 隆幸, Morisaki, Takayuki, 上田, 裕一, Ueda, Yuichi, 児玉, 逸雄, Kodama, Itsuo

January 2008

No description available.

Embryonic stem cell

Cardiac cell

Vascular endothelial cell

Paracrine factor

Cardiomyogenesis

Nkx2.5

Bone morphogenic protein

Wnt

Cyclooxygenase

Nitric oxide synthase