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1	Einfluss des transmembranen Hüllproteins des humanen endogenen Retrovirus K (HERV-K) auf die Zytokinproduktion humaner in-vitro kultivierter unreifer und reifer dendritischer Zellen / Influence of the transmembrane envelope protein of human endogenous retrovirus K (HERV-K) on the cytokine production of human in vitro cultured immature and mature dendritic cells Forstner, Maria Elisabeth January 2013 (has links) (PDF) Bei der Implantation des Fetus in den Uterus und während der Schwangerschaft kommt es zu einer Interaktion fetaler Trophoblastzellen mit dem mütterlichen Immunsystem. Trotz vieler verschiedener Studien ist bis heute nicht grundlegend geklärt, welche Mechanismen zur immunologischen Akzeptanz des (semi-)allogenen Fetus durch die Mutter beitragen. Zur wechselseitigen Kommunikation zwischen Kind und Mutter tragen Zytokine bei, die von allen immunkompetenten Zellen sezerniert werden können und regulatorisch auf die Immunantwort wirken. Eine Störung im Gleichgewicht der Zytokine kann zu Aborten, Präeklampsie oder anderen Pathologien führen. Eine wichtige Quelle von Zytokinen stellen u.a. die reifen und unreifen dendritischen Zellen (DC), die in der humanen Dezidua nachgewiesen wurden, dar. DC übernehmen als effiziente Antigen präsentierende Zellen eine entscheidende Funktion im Immunsystem und können inflammatorische Immunantworten induzieren. Jedoch spielen sie auch eine wichtige Rolle bei der Vermittlung immunologischer Toleranz. Die menschliche Plazenta weist eine auffällig starke Expression verschiedener humaner endogener Retroviren (HERV) auf. Immunmodulierende Eigenschaften von HERV wurden bereits beschrieben, jedoch nicht die direkte Wirkung von HERV-Proteinen der Plazenta auf Zellen des Immunsystems. Im Rahmen der Arbeit sollte daher die Wirkung des Hüllproteins des HERV-K, das in den Zytotrophoblastenzellen und in den Zellen des extravillösen Trophoblasten nachgewiesen wurde, auf die Zytokinproduktion unreifer (iDC) und reifer DC (mDC) untersucht werden. Als Modellsystem wurden in-vitro aus Monozyten des peripheren Blutes differenzierte DC gewählt. Die DC wurden in unreifem und reifem Zustand mit unterschiedlichen Konzentrationen von HERV-K-Peptiden (rekombinante Proteine (TM05.04 und TM12.12) bzw. Peptide aus 22 Aminosäuren (K120 und K177)) behandelt. Untersucht wurden die Veränderungen der Zytokinspiegel in den Zellkulturüberständen mittels Cytometric Bead Assay und Durchflusszytometrie. Die Messungen zeigten z.T. signifikante Veränderungen der Zytokinproduktion. So wurde die TNF-α-Sekretion der mDC durch K120 und K177 signifikant vermindert. Dieselben Peptide supprimierten ebenfalls signifikant die IL-8-Sekretion der mDC. Jedoch kam es durch alle vier HERV-Peptide (bei drei Peptiden signifikant) zu einer Steigerung der IL-8-Produktion in den iDC. Auch IL-6 wurde von den iDC durch HERV-K mehrheitlich signifikant vermehrt ausgeschüttet. Bzgl. IL-6 ergaben sich jedoch keine signifikanten Veränderungen in den mDC. In allen Ansätzen kam es zu einer konzentrationsabhängigen Stimulation der Sekretion des immunsuppressiven IL-10 (bei je drei Peptiden signifikante Ergebnisse). Keine signifikanten Veränderungen ergaben sich für IL1-β und IL-4. Die Erkenntnis, dass die HERV-Peptide die Zytokinproduktion der DC z.T. signifikant modulieren und diese Veränderung in den unterschiedlichen Reifestadien der DC variieren, lässt vermuten, dass die in der humanen Plazenta exprimierten Proteine einen Einfluss auf den Verlauf einer Schwangerschaft nehmen. Bei einer Schwangerschaft sind extrem fein abgestimmte, komplexe Vorgänge, bei denen viele verschiedene Faktoren eine Rolle spielen, für einen Erfolg vonnöten. Eine Übertragung der in-vitro-Ergebnisse auf in-vivo-Zustände ist nicht leicht zu vollziehen. Die vorliegenden Ergebnisse sprechen jedoch für einen Einfluss des HERV-K auf die Kommunikation zwischen Fetus und Mutter. Inwiefern genau und wie wichtig bzw. essentiell die Expression der HERV-K-Peptide für einen physiologischen Verlauf der Schwangerschaft ist, ob sie einen Einfluss auf Pathologien während der Gestation hat und ob dem HERV-K eine Bedeutung in der humanen Evolution zukommt, kann mit dieser Arbeit nicht geklärt werden. Jedoch gibt diese Arbeit Anlass dafür, den Einfluss des HERV-K auf die menschliche Fortpflanzung weitergehend zu untersuchen. / During the implantation of the fetus in the uterus and during pregnancy fetal trophoblast cells interact with the maternal immune system. Despite a multitude of studies, so far it is not completely clear, which mechanisms contribute to the immunological acceptance of the (semi)allogeneic fetus by the mother. Cytokines are vital to an intact communication between child and mother. They have a significant regulatory influence on the maternal immune response. A disturbance in the balance of cytokines can lead to miscarriage, preeclampsia or other pathologies. Among others, an important source of cytokines are the mature and immature dendritic cells (DC), which were detected in the human decidua. DC have a crucial function in the immune system: They are efficient antigen presenting cells and are able to induce inflammatory immune responses. However, they also play an important role in the mediation of immunological tolerance. The human placenta shows a remarkably high expression of various human endogenous retroviruses (HERV). Immunomodulating properties of HERV have been described. The direct effect of placental HERV proteins on cells of the immune system, however, has not been analyzed yet. Hence this study examines the effect of the transmembrane envelope protein of HERV-K, which was detected in cytrophoblast and extravillous trophoblast cells, on the cytokine production of human immature (iDC) and mature (mDC) DC. The significant changes in cytokine release suggest that the expression of the HERV-K peptides have an influence on the course of human pregnancy. Fetomaternal Immunologie Endogene Retroviren Dendritische Zelle Cytokine ddc:618
2	Evaluation of a Flow Cytometry Method for Identifying and Quantifying Fetal Red Blood Cells in Maternal Blood Nilsson, Camilla January 2011 (has links) Hemoglobin is an oxygen binding protein in erythrocytes. Hemoglobin is composed of four polypeptide chains. During the fetal stage the type of hemoglobin called fetal hemoglobin (HbF) dominates. After birth HbF is replaced by adult hemoglobin (HbA). HbF persists in concentrations less than 1%. Elevated concentration of HbF in adults exists in different conditions, Talassemi for example. When the uterus is damaged and the fetus doesn’t feel well its blood can pass the placenta barrier and enter the blood stream of the mother. A venous blood sample from the mother is analyzed to determine the status of the fetus. Laboratory Medicine Västernorrland already has two methods for analyzing HbF, one routine and one on call. The routine method needed to be replaced and the possibility to use flow cytometry was investigated. In this study, results from flow cytometry using Fetal Cell Count™ kit was compared to the results from the presently used methods, Kleihauer-Betke and HPLC. Cord blood was diluted with venous blood from an adult with the same blood group in various concentrations. A number of tests were performed and showed a fairly good correlation between the different methods. However more tests will be necessary to draw any clear conclusion. Kleihauer-Betke Fetomaternal hemorrhage Fetal hemoglobin HPLC Cord blood
3	Detection and quantification of fetal hemoglobin in blood using flow cytometry Hedblom, Sofia January 2012 (has links) Analytical methods used clinically in Sweden for detection and quantification of fetal hemoglobin (HbF) in maternal blood are either the microscopic method Kleinhauer Betkes test (KBT) or high performance liquid chromatography. A more modern alternative to detect and quantify HbF+ erythrocytes is flow cytometry. The aim of this project was therefore to evaluate the commercial kit "Fetal Cell Count kit" using flow cytometry. The kit used two antibodies; one directed against the specific γ-chain of HbF protein and the other directed against the intracellular enzyme carbanhydrase (CA), which is found in all erythrocytes in adults. The resulting data showed good precision, sensitivity and linearity. A reference interval based on male blood donors was determined to <0.1 % HbF+ erythrocytes and <1.3 %F-cells. The kit is well suited to detect and quantify F-cells. It could be used as a important tool to follow-up patients withβ-thalassemia and sickle cell anemia. However the kit was not as useful for detection and quantification of HbF+ erytrocytes in fetomaternal hemorrhage induced by Rhimmunization. HbF Rh-immunization Carbanhydrase F-cells Fetomaternal hemorrhage
4	The role of endothelial progenitor cells in the utero-placental vasculature Sipos, Peter January 2013 (has links) Fetal growth in utero depends on nutrient and oxygen reaching the fetus through the uterine and placental microcirculations, both undergoing massive expansion during pregnancy. Aberrations of the placental vasculature are associated with Intrauterine Growth Restriction (IUGR), a common pathological outcome of pregnancy; however, the cellular components responsible for vessel formation in the placenta and the uterus remain unknown. Endothelial Progenitor Cells (EPC) are a group of morphologically and functionally varied bone marrow derived vasculogenic cell types, divided into two major subsets: (i) Circulating Angiogenic Cells (CACs), which promote vessel formation by interfering with the extracellular matrix and (ii) Endothelial Colony Forming Cells (ECFCs), which provide the source for new endothelium. This role has been demonstrated in pathophysiological studies, but not in normal physiological events in vivo. Fetal ECFCs are more proficient than their adult counterparts, but it is unclear in what specific fetal or maternal physiological situations fetal ECFCs are involved. Based upon these considerations, it was hypothesised that: (i) fetal-derived ECFCs play a role in placental vasculogenesis, (ii) these cells transmigrate the placenta and home to loci of vessel formation in the pregnant uterus, and that (iii) intrinsic alterations in their capabilities are associated with fetal growth restriction during intrauterine life. To support these hypotheses the following experiments were performed;(i) EPCs in blood from pairs of human umbilical arteries and veins were counted by flow cytometry. Numbers of EPCs in these samples showed an arterio-venous gradient suggesting their placental sequestration. Furthermore, ECFCs were isolated from human umbilical blood using established culture techniques. Labelled human fetal ECFCs were transplanted into the circulation of murine fetuses using an ultrasound-guided intra-cardiac injection. Using a fluorescent imager and microscopy these cells were shown to home to the murine placenta and participate in vasculogenesis.(ii) Male mice ubiquitously expressing eGFP were crossbred with native females, and fetal (eGFP-positive) endothelial-like cells integrated into the uterine microvasculature. Human fetal ECFCs injected into murine fetuses were shown to migrate to the maternal uterus and became functionally involved with the microvasculature. In humans, microvessels were isolated from uterine biopsies of mothers with male offspring. Copies of the male specific SRY gene (quantified by RT-QPCR) indicated that cells of fetal origin constituted 12% of the endothelium in these vessels. In cross-sections, hybridisation of the Y-chromosome demonstrated the presence of fetal cells in the maternal endothelium of the human uterus. (iii) Using flow cytometry, fewer EPCs were defined within the peripheral circulation of growth-restricted babies. Functional assays showed that ECFCs derived from these growth-restricted cases had intrinsically impaired proliferation, migration, matrix-metalloproteinase (MMP-2) production, and generated fewer blood vessels in a murine vasculogenic bioassay. These results demonstrated the vasculogenic capacity of human fetal ECFCs in vivo and established them as key players in human placental vasculogenesis and uterine vessel expansion. Notably, these results also showed a link between impaired function of fetal ECFCs and IUGR, which is associated with increased cardiovascular risk of both the fetus as an adult, and mother in later life. From these findings it could be speculated, that intrinsic changes in ECFC-biology may be the causative link between IUGR and fetal and maternal cardiovascular susceptibility. Insight into these processes may contribute to early diagnosis, prevention and treatment of IUGR and associated conditions.
5	IPSC-derived trophoblasts: a novel model for infections at the maternal fetal interface Wang, Jennifer 08 June 2020 (has links) BACKGROUND: The placenta is a multifunctional organ whose primary functions are to nourish and protect the fetus throughout gestation. The immune response of the placenta plays an important part in gestational outcome. Microbial infection during pregnancy can be detrimental to both maternal health and fetal development, increasing the risk for miscarriage, preterm birth, and congenital abnormalities. However, evaluating immunological response has been an on-going challenge for scientists and clinicians due to the complexity of the maternal-fetal interface. Research has been done to understand the mechanisms by which pathogens activate placental immune response, but our understanding is still lacking in many areas due to the dynamic changes that occur in immunology over the gestational timeline. The primary challenge faced by researchers is the availability of placental tissue, which is limited by donors and their finite viability in culture once harvested. Additionally, legal restrictions placed on fetal-tissue research have severely limited advancement in the field. Human induced pluripotent stem cells (hiPSCs) present a unique tool to study the differentiation of trophoblasts and maternal-placental immunology without the need of fetal tissue. OBJECTIVE: The goal of this project is to develop an in vitro model for studying placental immunology and pathogenesis using human induced pluripotent stem cell (hiPSC)-derived trophoblasts. Our aim is to report a robust protocol for producing hiPSC-derived trophoblasts and to characterize them against primary trophoblasts using both gene and protein expression detection techniques. Successful modeling of human trophoblasts would allow us the unique opportunity to investigate the cellular interface between the maternal and fetal systems without needing to isolate primary human trophoblasts. Once we produce and fully characterize several hiPSC cell clones from multiple normal individuals, we will demonstrate the use of these cells as a model for infections at the maternal-fetal interface by exposing them to viral pathogens known to target the placenta. METHODS: Earlier publications have reported the differentiation of embryonic stem cells into trophoblasts in culture by using bone morphogenetic protein-4 in conjunction with inhibitors of activin A and FGF2-signaling (BMP4/A83-01/PD173074; BAP-treatment). We applied this approach to hiPSC lines from two different lineage origins and characterized the outcome against known trophoblast markers. We also developed a novel approach to maintain proliferative trophoblast stem cells in culture long term. Two viral pathogens, a recombinant vesicular stomatitis virus strain engineered to express a green fluorescent protein (rVSV-GFP) and a strain of Zika virus (ZIKV-PRVABC59), were used to determine if it is possible to infect hiPSC-derived trophoblasts in culture. RESULTS: Using this approach, hiPSC readily differentiate into trophoblasts by day 8 of culture. These cells demonstrate formation of multinuclear syncytium, invasive capacities, and secretion of placental hormones. Further characterization using quantitative real-time PCR and immunofluorescent staining indicates that these cells express a number of trophoblast markers at levels comparable to those expressed by primary first-trimester trophoblasts. We were also able to maintain a putative CT population which retains the capacity to double and give rise to terminal cell types. HiPSC-derived trophoblasts infected with rVSV-GFP and ZIKV-PRVABC59 tested positive for viral infection by 72 hours post-infection (HPI), demonstrating the use of these cells as an in vitro model for studying placental pathogens at the maternal-fetal interface. / 2022-06-08T00:00:00Z Medicine Cytotrophoblast Fetomaternal organ hiPSC iPSC Placenta Trophoblast
6	Desenvolvimento de imunossensor para detecção de hemorragia feto – materna (HFM) Nishio, Suelen de Souza Assunpção January 2019 (has links) Orientador: Elenice Deffune / Resumo: A Hemorragia feto-materna (HFM) se dá pela transferência do sangue fetal para o compartimento intravascular materno, devido à ruptura na membrana vásculo-sincicial da placenta. A HFM pode ser responsável pela alosensibilização do sistema imune materno, levando a morbidade e mortalidade de gravidez corrente e/ou de futura, assim como também constitui a base da etiopatogenia de várias afecções, como se verifica na doença hemolítica perinatal que expõe a complicações fetais como, hidropsia, danos cerebrais hipóxicos e morte fetal. Detectar e quantificar hemácias fetais ajuda a prevenir as consequências devida a ocorrência da HFM. Entre os testes diagnósticos utilizados na detecção e quantificação têm - se os mais sensíveis o teste quantitativo de Kleihauer e Betke e o de Citometria de fluxo, sendo o primeiro considerado padrão ouro. Tendo em vista a importância do diagnóstico laboratorial da HFM foi desenvolvida a proposta da construção de imunossensor para detecção de amostras de sangue fetal na corrente sanguínea materna. Foi realizada a produção de anticorpo monoclonal com objetivo de produzir anticorpos contra antígenos de superfícies de hemácias fetais humana e também foram realizadas a construção de unidades sensoriais para detecção de sinal biológico de imunoafinidade entre anticorpos que detectam hemácias fetais e a hemoglobina fetal presente nestas células, a fim de se diagnosticar a ocorrência da HFM. Foram obtidos como resultados a produção de anticorpo monoclonal que... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: Fetomaternal hemorrhage (FMH) occurs through the transfer of fetal blood into the maternal intravascular compartment, due to rupture in the placenta-syncytial membrane. FMH may be responsible for the alosensitization of the maternal immune system, leading to morbidity and mortality of current and / or future pregnancies, as well as being the basis of the etiopathogenesis of various conditions, as in perinatal haemolytic disease that exposes to fetal complications such as hydrops, hypoxic brain damage, and fetal death. Detecting and quantifying fetal erythrocytes helps to prevent the consequences due to the occurrence of FMH. Among the diagnostic tests used in the detection and quantification are the most sensitive the quantitative test of Kleihauer and Betke and the one of Flow cytometry, being the first considered gold standard. Considering the importance of the laboratory diagnosis of FMH, the proposal of the construction of immunosensor for the detection of fetal blood samples in the maternal blood was developed. The production of a monoclonal antibody was carried out with the objective of producing antibodies against antigens on human fetal red blood cells and also the construction of sensorial units for the detection of biological signal of immunoaffinity between antibodies that detect fetal red blood cells and the fetal hemoglobin present in these cells, in order to diagnose the occurrence of FMH. The results obtained are the production of monoclonal antibody that detec... (Complete abstract click electronic access below) / Mestre Anticorpo monoclonal Biossensor Hemorragia feto – materna Imunossensor Monoclonal antibody Biosensor Fetomaternal hemorrhage Immunosensor
7	Expressão de VEGF (VEGFR1/VEGFR2) e avaliação estereológica da membrana corioalantóide a termo em éguas Puro Sangue Inglês: influência da pluriparidade sobre o peso dos potros ao nascimento / Expression of VEGF (VEGFR1/VEGFR2) and stereology evaluation of the chorioallantoic membrane at term in Thoroughbred mares: influence of parity in foal birth weight. Carina de Fátima Guimarães 09 December 2013 (has links) A interação materno fetal na espécie equina depende exclusivamente da complexidade anatômica e fisiológica da placenta e este órgão endócrino provisório é a peça chave do presente estudo, onde objetivou-se avaliar a influência do número de partos sob a eficiência placentária. Buscando, por meio da morfometria das macro e microrregiões, além da expressão do VEGF, VEGFR-1/Flt-1 e VEGFR-2/FLK-1 na membrana corioalantóide a termo, dados referentes à inter-relação da pluriparidade, contato materno fetal e peso dos neonatos da raça Puro Sangue Inglês. O delineamento experimental consistiu em um estudo analítico, observacional, transversal, prospectivo. Foram acompanhados cinquenta partos de éguas divididas em três grupos de acordo com a pluriparidade: primíparas (n=18), 2 a 5 partos (n=14) e 6 a 10 partos (n=18). Foram coletados e fixados em formol fragmentos de 3 cm2 das regiões do corpo do útero (Cut), corno uterino gestante (CG) e corno uterino contralateral (CnG) da membrana corioalantóide a termo pós delivramento. Após processamento foram corados pela técnica de Hematoxilina & Eosina e Picro-Sirus-Red. Os estudos imunohistoquímico (método avidina-biotina) e esterológico foram realizados ao microscópio óptico. Foram correlacionados número de partos, altura e perímetro torácico (PT) maternos; idade, altura e PT paternos; composição volumétrica dos compartimentos placentários juntamente com as áreas de superfície de contato materno-fetal e peso, altura e escore de vitalidade neonatal. A paridade, além de diretamente relacionada ao peso do neonato, demonstrou na avaliação morfofuncional ser determinante ao ganho de eficiência placentária. As membranas corioalantóides das éguas pluríparas tenderam a apresentar maior volume total no CG, aumento na porcentagem e volume total de vilos, além de maior densidade microcotiledonária e expressão do VEGF na região do CG. Entre as muitas correlações determinadas no grupo primíparas as mais relevantes foram peso da membrana com variáveis neonatais como peso (r=0,598), PT (r=0,775), tempo para mamar (r=0,553) e tempo de gestação (r=-0,527), além do PT da mãe com o tempo para ruptura do cordão umbilical (r=0,564), reflexo de sucção (r=0,625), para levantar (r=0,756) e decúbito esternal (r=-590). Da mesma forma no grupo 2 a 5 partos, neonatos que nasceram com maior peso, altura, e PT apresentaram menor tempo para levantar (r=-0,546; r=-0,869, r=-0,892), eliminação do mecônio (r=-0,535) e ruptura do cordão umbilical (r=-0,528; r=-0,881). Assim como no grupo 6 a 10 partos, o peso do potro apresentou correlação com o peso (r=0,793), PT (r=0,716) e altura (r=0,667) materna. O volume total do CG correlacionou com volume total do parênquima (r=-0,816) e epitélio nos vilos placentários do CG (r=-0,915), tempo de gestação (r=-0,483), tempo para reflexo de sucção (r=-0,672), para mamar (r=-0,525), e para eliminação do mecônio (r=-0,525). No que diz respeito às variáveis paternas, o peso paterno correlacionou com o volume total do parênquima nos vilos placentários do CnG (r=0,393) , além do PT do garanhão com o peso (r=0,316) e PT (r=0,425) do potro e volume total do CG (r=0,319). Desta forma, acredita-se que estes resultados possam fornecer ferramentas práticas para auxiliar na escolha das fêmeas e machos mais indicados para geração de potros neonatos com desenvolvimento adequado. / Fetomaternal interaction in equine species depends exclusively on the complexity of placental anatomy and physiology. This transient endocrine organ is the key of the present study, which aimed to evaluate the influence of parity on placental efficiency. Morphometric of macro and micro regions, expression of VEGF, VEGFR-1/Flt-1 and VEGFR-2/FLK-1 in term corioallantois were performed and data regarding parity, fetomaternal contact and neonatal weight were evaluated in Thoroughbred. The experimental study consisted of an analytical, observational, cross-sectional, prospective study. Fifty deliveries were monitored in mares divided into three groups according to parity: nulliparous (n=18), 2 to 5 deliveries (n=14) and 6 to 10 deliveries (n=18). Tissue sections measuring 3 cm 2 were collected and fixed in formol saline from term chorioallantois regions: uterine body (UtB), pregnant uterine horn (PH) and contralateral uterine horn (CtH). After processing, samples were stained using Hematoxylineosin and Picro-Sirus-Red. Imunnohistochemistry (avidin-biotin method) and stereology were performed using an optic microscope. Correlations between parity, maternal height and thoracic perimeter; paternal age, height and thoracic perimeter; volume composition of placental compartments, surface area of fetomaternal contact and weight, height and neonatal vitality score were performed. Parity was directly related to weight of the neonate and demonstrated in morphofunctional evaluation to be determinant for placental efficiency. Chorioallantoic membranes from pluriparous mares tended to have greater total PH volume, higher percentage and total villi volume, and greater microcotiledonary density and VEGF expression in PH region. There were several correlations found in nulliparous group, the most relevant were membrane weight and neonatal parameters such as weight (r=0,598), thoracic perimeter (r=0,775), time to nurse (r=0,553) and gestational length (r=-0,527) and also mares thoracic perimeter with time to rupture the umbilical cord (r=0,564), suckle reflex (r=0,625), time to stand (r=0,756) and to achieve sternal recumbency (r=-590). Likewise, for the 2 to 5 deliveries group, neonates that were born heavier, taller and with greater thoracic perimeter took less time to stand (r=-0,546; r=-0,869, r=-0,892), pass meconium (r=-0,535) and rupture the umbilical cord (r=-0,528; r=-0,881). In the group of mares between 6 and 10 deliveries, foals weight was correlated to maternal weight (r=0,793), thoracic perimeter (r=0,716) and height (r=0,667). Total PH volume correlated to total parenchyma (r=-0,816) and epithelium in placental villi in PH (r=-0,915), gestational lenght (r=-0,483), time to suckle reflex (r=- 0,672), to nurse (r=-0,525), and pass meconium (r=-0,525). Regarding Paternal variables, paternal weight correlated to total parenchyma volume in placental villi of the CtH (r=0,393). Also thoracic perimeter of the stallion correlated to neonatal weight (r=0,316) thoracic perimeter (r=0,425) and total volume of the PH (r=0,319). Therefore, these data provides rationale for an adequate choice of mares and stallions to generate well-developed neonates. Angiogênese Equinos Interação materno-fetal Neonato Placenta Equine Fetomaternal interaction Neonate Placenta
8	Expressão de VEGF (VEGFR1/VEGFR2) e avaliação estereológica da membrana corioalantóide a termo em éguas Puro Sangue Inglês: influência da pluriparidade sobre o peso dos potros ao nascimento / Expression of VEGF (VEGFR1/VEGFR2) and stereology evaluation of the chorioallantoic membrane at term in Thoroughbred mares: influence of parity in foal birth weight. Guimarães, Carina de Fátima 09 December 2013 (has links) A interação materno fetal na espécie equina depende exclusivamente da complexidade anatômica e fisiológica da placenta e este órgão endócrino provisório é a peça chave do presente estudo, onde objetivou-se avaliar a influência do número de partos sob a eficiência placentária. Buscando, por meio da morfometria das macro e microrregiões, além da expressão do VEGF, VEGFR-1/Flt-1 e VEGFR-2/FLK-1 na membrana corioalantóide a termo, dados referentes à inter-relação da pluriparidade, contato materno fetal e peso dos neonatos da raça Puro Sangue Inglês. O delineamento experimental consistiu em um estudo analítico, observacional, transversal, prospectivo. Foram acompanhados cinquenta partos de éguas divididas em três grupos de acordo com a pluriparidade: primíparas (n=18), 2 a 5 partos (n=14) e 6 a 10 partos (n=18). Foram coletados e fixados em formol fragmentos de 3 cm2 das regiões do corpo do útero (Cut), corno uterino gestante (CG) e corno uterino contralateral (CnG) da membrana corioalantóide a termo pós delivramento. Após processamento foram corados pela técnica de Hematoxilina & Eosina e Picro-Sirus-Red. Os estudos imunohistoquímico (método avidina-biotina) e esterológico foram realizados ao microscópio óptico. Foram correlacionados número de partos, altura e perímetro torácico (PT) maternos; idade, altura e PT paternos; composição volumétrica dos compartimentos placentários juntamente com as áreas de superfície de contato materno-fetal e peso, altura e escore de vitalidade neonatal. A paridade, além de diretamente relacionada ao peso do neonato, demonstrou na avaliação morfofuncional ser determinante ao ganho de eficiência placentária. As membranas corioalantóides das éguas pluríparas tenderam a apresentar maior volume total no CG, aumento na porcentagem e volume total de vilos, além de maior densidade microcotiledonária e expressão do VEGF na região do CG. Entre as muitas correlações determinadas no grupo primíparas as mais relevantes foram peso da membrana com variáveis neonatais como peso (r=0,598), PT (r=0,775), tempo para mamar (r=0,553) e tempo de gestação (r=-0,527), além do PT da mãe com o tempo para ruptura do cordão umbilical (r=0,564), reflexo de sucção (r=0,625), para levantar (r=0,756) e decúbito esternal (r=-590). Da mesma forma no grupo 2 a 5 partos, neonatos que nasceram com maior peso, altura, e PT apresentaram menor tempo para levantar (r=-0,546; r=-0,869, r=-0,892), eliminação do mecônio (r=-0,535) e ruptura do cordão umbilical (r=-0,528; r=-0,881). Assim como no grupo 6 a 10 partos, o peso do potro apresentou correlação com o peso (r=0,793), PT (r=0,716) e altura (r=0,667) materna. O volume total do CG correlacionou com volume total do parênquima (r=-0,816) e epitélio nos vilos placentários do CG (r=-0,915), tempo de gestação (r=-0,483), tempo para reflexo de sucção (r=-0,672), para mamar (r=-0,525), e para eliminação do mecônio (r=-0,525). No que diz respeito às variáveis paternas, o peso paterno correlacionou com o volume total do parênquima nos vilos placentários do CnG (r=0,393) , além do PT do garanhão com o peso (r=0,316) e PT (r=0,425) do potro e volume total do CG (r=0,319). Desta forma, acredita-se que estes resultados possam fornecer ferramentas práticas para auxiliar na escolha das fêmeas e machos mais indicados para geração de potros neonatos com desenvolvimento adequado. / Fetomaternal interaction in equine species depends exclusively on the complexity of placental anatomy and physiology. This transient endocrine organ is the key of the present study, which aimed to evaluate the influence of parity on placental efficiency. Morphometric of macro and micro regions, expression of VEGF, VEGFR-1/Flt-1 and VEGFR-2/FLK-1 in term corioallantois were performed and data regarding parity, fetomaternal contact and neonatal weight were evaluated in Thoroughbred. The experimental study consisted of an analytical, observational, cross-sectional, prospective study. Fifty deliveries were monitored in mares divided into three groups according to parity: nulliparous (n=18), 2 to 5 deliveries (n=14) and 6 to 10 deliveries (n=18). Tissue sections measuring 3 cm 2 were collected and fixed in formol saline from term chorioallantois regions: uterine body (UtB), pregnant uterine horn (PH) and contralateral uterine horn (CtH). After processing, samples were stained using Hematoxylineosin and Picro-Sirus-Red. Imunnohistochemistry (avidin-biotin method) and stereology were performed using an optic microscope. Correlations between parity, maternal height and thoracic perimeter; paternal age, height and thoracic perimeter; volume composition of placental compartments, surface area of fetomaternal contact and weight, height and neonatal vitality score were performed. Parity was directly related to weight of the neonate and demonstrated in morphofunctional evaluation to be determinant for placental efficiency. Chorioallantoic membranes from pluriparous mares tended to have greater total PH volume, higher percentage and total villi volume, and greater microcotiledonary density and VEGF expression in PH region. There were several correlations found in nulliparous group, the most relevant were membrane weight and neonatal parameters such as weight (r=0,598), thoracic perimeter (r=0,775), time to nurse (r=0,553) and gestational length (r=-0,527) and also mares thoracic perimeter with time to rupture the umbilical cord (r=0,564), suckle reflex (r=0,625), time to stand (r=0,756) and to achieve sternal recumbency (r=-590). Likewise, for the 2 to 5 deliveries group, neonates that were born heavier, taller and with greater thoracic perimeter took less time to stand (r=-0,546; r=-0,869, r=-0,892), pass meconium (r=-0,535) and rupture the umbilical cord (r=-0,528; r=-0,881). In the group of mares between 6 and 10 deliveries, foals weight was correlated to maternal weight (r=0,793), thoracic perimeter (r=0,716) and height (r=0,667). Total PH volume correlated to total parenchyma (r=-0,816) and epithelium in placental villi in PH (r=-0,915), gestational lenght (r=-0,483), time to suckle reflex (r=- 0,672), to nurse (r=-0,525), and pass meconium (r=-0,525). Regarding Paternal variables, paternal weight correlated to total parenchyma volume in placental villi of the CtH (r=0,393). Also thoracic perimeter of the stallion correlated to neonatal weight (r=0,316) thoracic perimeter (r=0,425) and total volume of the PH (r=0,319). Therefore, these data provides rationale for an adequate choice of mares and stallions to generate well-developed neonates. Angiogênese Equine Equinos Fetomaternal interaction Interação materno-fetal Neonate Neonato Placenta Placenta

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