Purinergic proliferation of coronary smooth muscle : receptor cloning, up-regulation and signaling /

Shen, Jianzhong,

January 2005

Thesis (Ph. D.)--University of Missouri--Columbia, 2005. / "July 2005." Typescript. Vita. Includes bibliographical references (leaves 152-167). Also issued on the Internet.

Human dermal fibroblasts in tissue engineering /

Junker, Johan P. E.,

January 2009

Diss. (sammanfattning) Linköping : Linköpings universitet, 2009.

Μοριακός έλεγχος τού λείου μυϊκού φαινότυπου

Μυρίσσα, Αναστασία

07 June 2013

Ο Λείος Μυϊκός Φαινότυπος (ΛΜΦ) χαρακτηρίζεται από σημαντική πλαστικότητα και παίζει κομβικό λειτουργικό ρόλο τόσο σε φυσιολογικές όσο και σε παθολογικές καταστάσεις. Στις αρτηρίες, η μεταβολή του ΛΜΦ στο φάσμα από φυσιολογικός-συσταλτός μέχρι συνθετικός-παθολογικός εμπλέκεται αιτιολογικά σε διάφορες ανθρώπινες ασθένειες όπως στην αθηροσκλήρωση, στην υπέρταση και στην επαναστένωση των αγγείων μετά από εγχείρηση. Η έκφραση γονιδίων ΛΜΦ έιναι επίσης μεγάλης σημασίας σε ασθένειες άλλων οργάνων, όπως η ίνωση των νεφρών και του ήπατος και η μετάσταση του καρκίνου. Συνεπώς, η μελέτη των μοριακών μηχανισμών μέσω των οποίων επηρεάζεται ο ΛΜΦ είναι πολύ σημαντική για την ανάπτυξη νέων τεχνικών περιορισμού της εξέλιξης αυτών των νόσων. Η λειτουργία πολλών ιστών όπως είναι τα αγγεία ελέγχεται σε σημαντικό βαθμό από το συμπαθητικό νευρικό σύστημα. Σκοπός λοιπόν της παρούσας εργασίας ήταν πρώτα-πρώτα να εξετάσουμε εάν in vitro η διέγερση των α και β αδρενεργικών υποδοχέων πιθανώς ρυθμίζει την έκφραση γονιδίων ΛΜΦ και προκαταρκτικά να διακριβώσουμε μέσω ποιών μοριακών μηχανισμών οι α1 (υπότυποι α1Α και α1Β) και οι β-ΑΥς επηρεάζουν και ελέγχουν το ΛΜΦ. Κατά δεύτερο λόγο θελήσαμε να εξετάσουμε εάν η εξωγενής έκφραση του μεταγραφικού παράγοντα Μυοκαρδίνη προκαλεί επιθηλιο-μεσεγχυματική μετάβαση (ΕΜΤ-Epithelial to Mesenchymal Transition) σε ενδοθηλιακά κύτταρα in vitro. Για τα πρώτα πειράματά μας χρησιμοποιήσαμε δύο διαφορετικούς κυτταρικούς πληθυσμούς: α) διαφοροποιημένα λεία μυϊκά κύτταρα αορτής αρουραίου της κυτταρικής σειράς A7r5, και β) κύτταρα ινοβλαστών της κυτταρικής σειράς ΝΙΗ3Τ3 προερχόμενα απο ποντικό, προκειμένου να δούμε αντίστοιχα πως η δράση των ΑΥ ελέγχει την έκφραση των γονιδίων αυτών σε διαφοροποιημένα ΛΜΚ (A7r5) και σε αδιαφοροποίητα κύτταρα που όμως μπορούν να μετατραπούν σε «ΛΜΚ» (ΝΙΗ3Τ3). Ως δείκτη για την έκφραση του ΛΜΦ, εξετάσαμε την έκφραση κυτταροσκελετικών, δομικών πρωτεϊνών-δεικτών, όπως η λείου μυϊκού τύπου α-Ακτίνη (SM-α-Αctin),, η λείου μυϊκού τύπου βαριά αλυσίδα της Μυοσίνης (SM-MHC), η λείου μυϊκού τύπου Καλπονίνη (SM-Calponin) και η λείου μυϊκού τύπου πρωτεΐνη 22α (τρανσγελίνη) (SM22α), σε δύο επίπεδα: α) είτε χρησιμοποιώντας αντισώματα, είτε β) με την χρήση πλασμιδίων αναφοράς όπου minimal υποκινητές των παραπάνω γονιδίων ελέγχουν την προσμετρούμενη έκφραση λουσιφεράσης. Η ενεργοποίηση της μεταγραφής αυτών των γονιδίων ρυθμίζεται, σε μεγάλο μέρος, από τις αλληλουχίες CArG (CArG boxes) στους υποκινητές τους, στις οποίες προσδένεται ο παράγοντας Serum Response Factor (SRF). Στα ΛΜΚ, ο μεταγραφικός παράγοντας SRF ενεργοποιεί τη μεταγραφή των γονιδίων-δεικτών μέσω δημιουργίας ενός απαραίτητου συμπλόκου με έναν μεταγραφικό παράγοντα της οικογένειας των Μυοκαρδινών, η οποία αποτελείται από 3 μέλη : τη Μυοκαρδίνη και τις συγγενείς πρωτεΐνες MRTF-A και MRTF-B. Στη μελέτη που πραγματοποιήσαμε, αρχικά παρατηρήσαμε ότι οι δύο αυτοί κυτταρικοί πληθυσμοί δεν εκφράζουν τους α1-ΑΥς (α1Α και α1Β υπότυποι) ενδογενώς, αλλά, με εισαγωγή του αντίστοιχου πλασμιδίου των α1Α ή α1Β ΑΥς, το σύστημα καθίσταται λειτουργικό. Επιπλέον ανακαλύψαμε ότι τα κύτταρα A7r5 εκφράζουν ενδογενώς τους β-ΑΥς. Από τα πειράματα που πραγματοποιήσαμε, καταλήξαμε στο συμπέρασμα ότι οι υποδοχείς αυτοί επηρεάζουν και καθορίζουν με διαφορετικό τρόπο το ΛΜΦ, ανάλογα με τον υπότυπο των ΑΥς και ανάλογα με τον τύπο των κυττάρων. Πιο αναλυτικά, όσον αφορά στα κύτταρα A7r5 παρατηρήσαμε ότι: α) η ενεργοποίηση των α1Α-ΑΥ επάγει την έκφραση και των τεσσάρων γονιδίων-δεικτών που καθορίζουν το ΛΜΦ τόσο σε μεταγραφικό όσο και σε πρωτεϊνικό επίπεδο, β) η ενεργοποίηση του υποκινητή της SM22α από τους α1Α-ΑΥς εξαρτάται από τα στοιχεία CΑrG ενώ η ενεργοποίηση του υποκινητή της SM-Calponin δεν εξαρτάται από τα στοιχεία αυτά, γ) η ενεργοποίηση των α1Β-ΑΥ επάγει τη μεταγραφική ενεργότητα των υποκινητών των γονιδίων SM22α και SM-Calponin ενώ δεν επηρεάζει την μεταγραφική ενεργότητα των υποκινητών των γονιδίων SM-α-Αctin και της SM-MHC, δ) η ενεργοποίηση των υποκινητών της SM22α και της SM-Calponin από τους α1Β-ΑΥς εξαρτάται από τα στοιχεία CΑrG, ε) οι β-ΑΥς, σε αντίθεση με τους α1-ΑΥς, επηρεάζουν με διαφορετικό τρόπο τη μεταγραφή των γονιδίων-δεικτών που καθορίζουν το ΛΜΦ, κυρίως ελαττώνοντας τη μεταγραφική ενεργότητα των υποκινητών των γονιδίων SM-Calponin, SM-α-Αctin και SM-MHC ενώ δεν επηρεάζουν τη μεταγραφική ενεργότητα του SM22α. Επίσης, όταν παρόμοια πειράματα έγιναν στα κύτταρα ΝΙΗ3Τ3 παρατηρήσαμε ότι: α) οι α1Α-ΑΥs επάγουν τη μεταγραφή των υποκινητών και των τεσσάρων γονιδίων-δεικτών που καθορίζουν το ΛΜΦ, β) στα κύτταρα αυτά η ενεργοποίηση των υποκινητών της SM22α και της SM-Calponin από τους α1Α-ΑΥς δεν εξαρτάται από τα στοιχεία CΑrG, γ) η ενεργοποίηση των α1Β-ΑΥs επάγει τη μεταγραφική ενεργότητα των υποκινητών των γονιδίων SM22α, SM-Calponin και SM-MHC ενώ δεν επηρεάζει την ενεργότητα του υποκινητή της SM-α-Αctin. Από τα παραπάνω λοιπόν, καταλήξαμε στα εξής συμπεράσματα: 1) Η διέγερση των α1-ΑΥ οδηγεί σε άυξηση της έκφρασης των γονιδίων-δεικτών του ΛΜΦ, και άρα οι α1-ΑΥς λειτουργούν, τουλάχιστον in vitro, ως παράγοντες προώθησης του ΛΜΦ. 2) Η δράση των α1-ΑΥ εξαρτάται μόνο μερικώς απο την ύπαρξη στοιχείων CArG (SRE), και διαφέρει ανάλογα με τον υποκινητή, άρα οι διάφοροι υποκινητές χρησιμοποιούν διαφορετικά τα στοιχεία CArG που περιέχουν, πράγμα που ενισχύει την υπόθεση συνδυαστικής χρήσης μεταφραφικών παραγόντων για την «πλαστική» έκφραση του λειτουργικού ΛΜΦ. 3) Οι δύο υπότυποι των α1-ΑΥ που εξετάστηκαν, α1Α-ΑΥς και α1Β-ΑΥς, έχουν προφανείς διαφορές ως πρός την διέγερση της έκφρασης των ΛΜ γονιδίων, και άρα πιθανώς θα παίζουν διαφορετικό λειτουργικό ρόλο στα αγγεία και στους άλλους ιστούς όπου εκφράζονται. 4) Αντίθετα με τους α1-ΑΥς, οι β-ΑΥς λειτουργούν ανασταλτικά στην έκφραση των γονιδίων του ΛΜΦ, και άρα το τελικό προϊόν της συμπαθητικής διέγερσης στα αγγεία θα είναι η συνισταμένη των δράσεων α και β ΑΥ, που θα διαφέρει στα διάφορα αγγεία ανάλογα με την σχετική έκφραση των υποδοχέων αυτών. Παράλληλα, εξετάζοντας ενδοθηλιακά κύτταρα φλέβας ανθρώπινου ομφάλιου λώρου (HUVEC), είδαμε ότι η εξωγενής έκφραση της Μυοκαρδίνης προκαλεί αλλαγές στο φαινότυπό τους, τόσο σε μορφολογικό επίπεδο όσο και μέσω de novo έκφρασης της SM-α-Ακτίνης και της SM-Καλπονίνης σε πρωτεϊνικό επίπεδο. Παρατηρήσαμε δηλαδή αλλαγές που είναι συμβατές με την επιθηλιο-μεσεγχυματική μετάβαση (ΕΜΤ-Epithelial to Mesenchymal Transition), διαδικασία με πολύ σπουδαίο ρόλο στην εμβρυογένεση, στη διαμόρφωση ιστών και οργάνων, αλλά επίσης και στην ίνωση, στη μετάσταση του καρκίνου και στην παθολογική αγγειογένεση. Συμπερασματικά, τα ενδοθηλιακά κύτταρα των αγγείων συμμετέχουν στη μετάβαση αυτή και μπορεί να συμβάλλουν σε διεργασίες κυτταρικής διαφοροποίησης και ιστικής δόμησης. Συμπεραίνουμε ότι η έκφραση της Μυοκαρδίνης επαρκεί για να προκαλέσει ΕΜΤ σε ανθρώπινα ενδοθηλιακά κύτταρα, με πιθανές συνέπειες για τη δυνατότητα trans-διαφοροποίησης και συνεισφοράς αυτών των κυττάρων, σε ανακατασκευή και αναδιοργάνωση ιστών, όπως πχ. στην αθηροσκλήρωση και την καρδιακή ανεπάρκεια. / The Smooth Muscle Cell (SMC) Phenotype is characterized by important plasticity and it plays crucial functional role in physiological and pathological conditions. Modulation of SMC Phenotype in arteries is a key etiological feature of some major human pathologies, including atherosclerosis, hypertension and vessel restenosis. Expression of SMCs marker-genes is also important in chronic diseases of other organs, such as in kidney or hepatic fibrosis and in cancer metastasis. So, study of the molecular mechanisms which affect SMC phenotype is necessary in order to develop new therapeutic approaches to combat to these diseases. Function of many tissues such as the vasculature is regulated by the sympathetic nervous system. The aim of this study was first, to examine in vitro whether the stimulation of alpha (α) and beta (β) adrenergic receptors (ARs) can control the expression of SMCs marker-genes in vitro and in case it did, to probe the molecular mechanisms via which α1-ARs (subtypes α1A and α1B) and β-ARs affect and regulate SMC Phenotype. Secondly, we wanted to investigate if the exogenous expression of Myocardin can cause Epithelial to Mesenchymal Transition (ΕΜΤ)-like changes in endothelial cells in vitro. For our experiments, we used two different cell populations : a) A7r5, which are differentiated Smooth Muscle Cells isolated from rat embryonic aorta, and b) ΝΙΗ3Τ3, mouse fibroblasts, in order to examine how stimulation of ARs modulates the expression of these marker-genes in differentiated SMCs (A7r5) and in mesenchymal cells which can convert to SMCs (ΝΙΗ3Τ3), respectively. As a marker for the expression of SMC Phenotype, we monitored the expression of cytoskeletal, structural protein-markers, such as Smooth Muscle-α-Actin (SM-α-Actin), SM-Myosin Heavy Chain (SM-MHC), h1-Calponin (SM-Calponin) and SM22α (transgelin) at two levels: a) using specific antibodies or b) using reporter plasmids in which the minimal promoters of the above genes drive luciferase gene transcription and hence activity. The coordinate transcriptional activation of these genes is, in major part, regulated by the function of CArG boxes in their promoters, which bind Serum Response Factor (SRF). In SMCs, SRF mediates its transcriptional effects via essential complex formation with members of the Myocardin family, which includes Myocardin (Myocd), Myocardin-Related Transcription Factor-A (MRTF-A) and MRTF-B. In our study, we initially noticed that these two cell populations do not express α1-ARs (subtypes α1Α and α1Β) endogenously, but when we transfect them with the plasmids expressing α1Α and α1Β ARs, the cells respond to α1-ARs agonist stimulation. In addition, we discovered that A7r5 cells express endogenous β-ARs. From our experiments, we concluded that these receptors can modulate SMC Phenotype in distinct way. This depends on both the specific subtype of receptor as well as on the cellular background (cell type). More specific, we observed that in A7r5 cells: a) activation of α1A-ARs by phenylephrine induces the expression of all four marker-genes at a transcriptional and at a protein level, b) activation of the SM22α minimal promoter by α1A-ARs depends on CΑrG boxes, while activation of the SM-Calponin minimal promoter does not depend on the presence of CΑrG boxes, c) activation of α1B-ARs induces the transcriptional activity of the minimal promoters of SM22α and SM-Calponin but does not affect the transcriptional activity of the minimal promoter of SM-α-Αctin and SM-MHC, d) activation of both the SM22α and the SM-Calponin minimal promoters by α1B-ARs depends on the presence of CΑrG boxes, e) on the contrary, β-ARs affect the transcription of SMCs marker-genes in an opposite way to α1-ARs reducing the transcriptional activity of the minimal promoters of SM-Calponin, SM-α-Αctin and SM-MHC genes, without affecting the transcriptional activity of the SM22α promoter. Additionally, we noticed that in ΝΙΗ3Τ3 cells: a) α1Α-ARs induce transcriptional activity of minimal promoters of SMC marker-genes, b) activation of minimal promoters of SM22α and SM-Calponin by α1A-ARs does not depend on CΑrG boxes, c) activation of α1B-ARs induce the transcriptional activity of the minimal promoters of SM22α, SM-Calponin και SM-MHC but does not affect the transcriptional activity of the minimal promoter of SM-α-Αctin. Based on the above findings, we conclude that: 1) Stimulation of α1-ARs drives an increased expression of SMC marker genes and consequently α1-ARs function, at least in vitro, as factors which have the ability to induce/maintain the SMC Phenotype. 2) The activity of α1-ARs depends variably on the presence of CArG boxes (SREs) and differs between these minimal promoters. In essence, different promoters use their CArG boxes in a different way. This is in support of the hypothesis that combinational use of transcriptional factors is essential for «plastic» expression of the SMC Phenotype. 3) The two subtypes of α1-ARs examined, α1Α and α1Β, display obvious differences in stimulating SM-specific gene expression and consequently these subtypes may play different functional role in vessels and in other tissues in which they are expressed. 4) On the contrary, β-ARs inhibit the expression of SMC marker-genes. Therefore, the final result of vascular sympathetic stimulation would depend on the combined action of α και β ARs. This action will differ in different vessels, depending on the relative expression of these receptors and their subtypes. In addition, adenoviral expression of Myocardin in human umbilical vein endothelial Cells (HUVECs) induced phenotypic alterations, evidenced by morphological changes and by de novo expression of SM-α-Αctin and SM-Calponin at the protein level. These observations are compatible with an Epithelial to Mesenchymal Transition (EMT), a process which plays an important role in embryogenesis, tissue and organs formation and angiogenesis, but also participates, in fibrosis and cancer metastasis. Consequently, vascular endothelial cells can undergo in EMT and may contribute in cellular differentiation and in tissue formation. We conclude that the expression of Myocardin is sufficient to cause EMT-like changes in human endothelial cells. This may lead to cellular trans-differentiation and contribution of these cells in active tissue remodeling such as in atherosclerosis and in cardiac failure.

612.740 45

Smooth muscle phenotype

Adrenergic receptors

Efeitos da castração e reposição hormonal tardia no tecido erétil do pênis de ratos Sprague-Dawley / Effects of castration and late hormonal replacement in the structure of rat corpora cavernosa

Alexandre de Freitas Miranda

25 March 2009

Estudos em animais e humanos sugerem que níveis adequados de testosterona são necessários para preservar a integridade do tecido eretor peniano. Nenhum estudo prévio confirmou se as mudanças estruturais são reversíveis após longo período de deprivação hormonal. Foi proposto a avaliação, através de métodos quantitativos, as alterações estruturais no corpo cavernoso de ratos submetidos à castração cirúrgica; bem como o papel da reposição hormonal tardia na reversão das possíveis alterações estruturais. Foram usados 25 ratos Sprague-Dawley machos com aproximadamente 12 semanas de idade. Os animais foram divididos em 5 grupos compostos por 5 animais em cada grupo e tratados da seguinte forma: ORQ1 = Grupo submetido à orquiectomia e sacrificado após 1 mês. C1- Grupo controle morto após 1 mês. ORQ2 - Grupo orquiectomizado e morto após 2 meses. C2 - Grupo controle morto após 2 meses. T Grupo orquiectomizado que recebeu, após 1 mês, suplementação com undecanoato de testosterona na dose de 100mg/ Kg subcutâneo. Após 1 mês de reposição hormonal os animais foram mortos.No Resultado Houve uma redução significativa no valor absoluto do colágeno, músculo liso, espaço sinusoidal e área total do corpo cavernoso após 2 meses no grupo castrado, quando comparado ao controle. Em termos gerais a densidade não apresentou nenhuma diferença significativa entre os grupos. A reposição hormonal com testosterona foi capaz de reverter as alterações observadas, demonstrando um aumento dos elementos estudados. A metodologia utilizada permitiu mostrar que valores absolutos demonstram melhor o que de fato ocorre com os elementos observados, eliminando um víeis de análise, quando se consideram os valores relativos. Esses resultados sugerem que a reposição, mesmo quando realizada tardiamente, foi eficaz na reversibilidade das alterações geradas pela castração / Introduction. Studies in animals and humans have suggested that adequate levels of testosterone are necessary to preserve the integrity of penile erectile tissue. No previously reported studies have confirmed if these structural changes are reversible following long-term hormonal deprivation. To evaluate, through quantitative methods, the structural alterations in the corpora cavernosa of rats submitted to surgical castration as well as the role of late hormone replacement in reversing the possible structural alterations. We used 25 male Sprague-Dawley rats who were approximately 12 weeks of age. The animals were divided into 5 groups composed of 5 animals each and treated as follows. ORCHIEC-1 = group that underwent orchiectomy and were sacrificed after 1 month, C-1 = control group sacrificed after 1 month, ORCHIEC-2 = group that underwent orchiectomy and were sacrificed after 2 months, C-2 = control group sacrificed after 2 months, T = group that underwent orchiectomy, and after 1 month underwent testosterone replacement with a subcutaneous single dose of testosterone undecanoate at 100 mg/kg (T); after 1 month of hormonal replacement, the animals were sacrificed. Quantification of smooth muscle, collagen and elastic system fibers in controls and rats submitted to orchiectomy alone and with late hormonal replacement. There were a significant decrease in the absolute values of collagen, smooth muscle, sinusoidal space and total area of corpora cavernosa after 2 months in the castrated group when compared with controls. Overall, as regards density, no significant differences were observed among the groups. The hormonal replacement with testosterone was able to reverse the alterations observed, demonstrating an increase in the elements studied. The method used for this research allowed demonstrating that absolute values are reliable to quantify the structural alterations of corpora cavernosa structures. The results suggest that hormonal replacement, even when instituted at a late stage, is effective in reversing the corpora cavernosa alterations produced by castration

Pênis

Testosterona

Andropausa

Colágeno

Músculo liso

Rato

Penis

Testosterone

Andropause

Collagen

Smooth muscle

Rat

CIRURGIA UROLOGICA

Gene regulation in embryonic development

Losa Llabata, Marta

January 2016

Branchial arches (BAs) are a series of transient structures that develop on the ventro-lateral surface of the head in vertebrate embryos. BAs initially appear as a series of similar segments; as development proceeds each BA will contribute to different structures. Here, it was investigated the transcriptional mechanisms that instruct the different fates of the BAs in development. Initially, each BA contains a blood vessel, known as aortic arch (AA) artery, that connects the dorsal aorta with the heart. Remodelling of the AAs is crucial to form the adult heart circulation. This process leads to regression of the anterior AAs, running though the first and second BAs (BA1 and BA2), and persistence of the AAs contained in more posterior BAs (PBA). To identify the mechanisms that control remodelling of the AAs, we compared the transcriptomes and epigenomic landscapes of different BAs. Using RNA-seq and H3K27Ac ChIP-seq, we uncovered the activation of a vascular smooth muscle cell (VSMC) differentiation transcriptional program exclusively in the PBAs (and not in BA1/BA2). In support of this finding, we show that VSMC differentiation occurs specifically in the PBAs, but not BA1-2 in mouse embryonic development. Despite the absence of VSMC differentiation in developing BA1-2, cells harvested from these tissues reveal a spontaneous tendency to differentiate towards VSMC fate when grown in vitro, and activate several VSMC-specific genes (Myocd, Acta2, Tagln, Jag1). Together, our results suggest that forming VSMCs is a key process for the persistence of AAs. We also showed that cells derived from all BAs have the potential to differentiate to VSMCs in vitro. However, only cells in the PBAs differentiate to VSMCs in vivo, resulting in the maintenance of posterior AAs. In this study, we also uncovered a novel transcriptional principle that specifies the fate of BA2. Using ChIP-seq, we found that binding of Meis transcription factors establish a ground pattern in the BAs. Hoxa2, which specifies BA2 identity, selects a subset of Meis-bound sites. Meis binding is strongly increased at these sites, which coincide with active enhancers, linked to genes highly expressed in the BA2 and regulated by Hoxa2. Thus, Hoxa2 modifies a ground state binding of Meis to instruct segment-specific transcriptional programs.

612.6

The role of pulmonary mast cells in neurotrophin 4 mediated cholinergic neuroplasticity in neonatal asthma

Patel, Kruti Rajan

15 June 2016

Asthma is a chronic inflammatory lung disease characterized by recurrent wheezing, coughing and difficulties in breathing. Asthma affects 25.7 million people in the USA including 8 million children. Asthma is often associated with early-life exposure to environmental insults. However, mechanisms that link early-life insults to persistent airway dysfunction are unknown. Our previous studies in mice showed that early-life allergen exposure increases the levels of neurotrophin 4 (NT4) causing airway smooth muscle (ASM) hyper innervation and persistent airway hyper reactivity (AHR). I show that early-life allergen exposure selectively increases cholinergic innervation. Notably, cholinergic nerves release acetylcholine, a potent airway constrictor that signals through the M3 receptor in ASM. Building upon these findings, my thesis encompasses two components. Firstly, how is NT4 expression aberrantly up regulated following early-life allergen exposure? Secondly, what is the effect of enhanced cholinergic innervation on the neonatal ASM? I find that NT4 is selectively expressed by ASM and mast cells in mice, nonhuman primates and humans. We show in mice that while NT4 expression in ASM remains unchanged upon allergen exposure, mast cells expand in number and degranulate to release NT4 thereby increasing NT4 levels in the lung. Adoptive transfer of wild-type mast cells, but not NT4-/- mast cells restores ASM innervation and AHR in KitW-sh/W-sh mice following early-life insults. In an infant primate model of asthma, the increased ASM innervation is also associated with the expansion and degranulation of mast cells. Therefore, pulmonary mast cells are a key source of aberrant NT4 expression following early-life insults in both mice and possibly primates. Next, I speculated that an increased cholinergic output in the neonatal lung might lead to persistent AHR. Using recurrent methacholine exposure and M3 receptor blocker, 4-DAMP, I show that enhanced cholinergic signaling in neonatal mice leads to persistent AHR without inflammation. In contrast, methacholine exposure in adult mice has no prolonged effects on airway reactivity. Together, my findings support a model in which deregulated neural activities following early-life insults cause persistent ASM hyper contractility. Thus, early-life interventions to block mast cell degranulation and the cholinergic pathway may benefit children with recurrent wheezing. / 2016-12-15T00:00:00Z

Immunology

NT4

Airway smooth muscle

Childhood asthma

Cholinergic innervation

Mast cells

Efeitos da castração e reposição hormonal tardia no tecido erétil do pênis de ratos Sprague-Dawley / Effects of castration and late hormonal replacement in the structure of rat corpora cavernosa

Alexandre de Freitas Miranda

25 March 2009

Estudos em animais e humanos sugerem que níveis adequados de testosterona são necessários para preservar a integridade do tecido eretor peniano. Nenhum estudo prévio confirmou se as mudanças estruturais são reversíveis após longo período de deprivação hormonal. Foi proposto a avaliação, através de métodos quantitativos, as alterações estruturais no corpo cavernoso de ratos submetidos à castração cirúrgica; bem como o papel da reposição hormonal tardia na reversão das possíveis alterações estruturais. Foram usados 25 ratos Sprague-Dawley machos com aproximadamente 12 semanas de idade. Os animais foram divididos em 5 grupos compostos por 5 animais em cada grupo e tratados da seguinte forma: ORQ1 = Grupo submetido à orquiectomia e sacrificado após 1 mês. C1- Grupo controle morto após 1 mês. ORQ2 - Grupo orquiectomizado e morto após 2 meses. C2 - Grupo controle morto após 2 meses. T Grupo orquiectomizado que recebeu, após 1 mês, suplementação com undecanoato de testosterona na dose de 100mg/ Kg subcutâneo. Após 1 mês de reposição hormonal os animais foram mortos.No Resultado Houve uma redução significativa no valor absoluto do colágeno, músculo liso, espaço sinusoidal e área total do corpo cavernoso após 2 meses no grupo castrado, quando comparado ao controle. Em termos gerais a densidade não apresentou nenhuma diferença significativa entre os grupos. A reposição hormonal com testosterona foi capaz de reverter as alterações observadas, demonstrando um aumento dos elementos estudados. A metodologia utilizada permitiu mostrar que valores absolutos demonstram melhor o que de fato ocorre com os elementos observados, eliminando um víeis de análise, quando se consideram os valores relativos. Esses resultados sugerem que a reposição, mesmo quando realizada tardiamente, foi eficaz na reversibilidade das alterações geradas pela castração / Introduction. Studies in animals and humans have suggested that adequate levels of testosterone are necessary to preserve the integrity of penile erectile tissue. No previously reported studies have confirmed if these structural changes are reversible following long-term hormonal deprivation. To evaluate, through quantitative methods, the structural alterations in the corpora cavernosa of rats submitted to surgical castration as well as the role of late hormone replacement in reversing the possible structural alterations. We used 25 male Sprague-Dawley rats who were approximately 12 weeks of age. The animals were divided into 5 groups composed of 5 animals each and treated as follows. ORCHIEC-1 = group that underwent orchiectomy and were sacrificed after 1 month, C-1 = control group sacrificed after 1 month, ORCHIEC-2 = group that underwent orchiectomy and were sacrificed after 2 months, C-2 = control group sacrificed after 2 months, T = group that underwent orchiectomy, and after 1 month underwent testosterone replacement with a subcutaneous single dose of testosterone undecanoate at 100 mg/kg (T); after 1 month of hormonal replacement, the animals were sacrificed. Quantification of smooth muscle, collagen and elastic system fibers in controls and rats submitted to orchiectomy alone and with late hormonal replacement. There were a significant decrease in the absolute values of collagen, smooth muscle, sinusoidal space and total area of corpora cavernosa after 2 months in the castrated group when compared with controls. Overall, as regards density, no significant differences were observed among the groups. The hormonal replacement with testosterone was able to reverse the alterations observed, demonstrating an increase in the elements studied. The method used for this research allowed demonstrating that absolute values are reliable to quantify the structural alterations of corpora cavernosa structures. The results suggest that hormonal replacement, even when instituted at a late stage, is effective in reversing the corpora cavernosa alterations produced by castration

Pênis

Testosterona

Andropausa

Colágeno

Músculo liso

Rato

Penis

Testosterone

Andropause

Collagen

Smooth muscle

Rat

CIRURGIA UROLOGICA

Expressão de citoceratinas de padrão basal (CK5/6), luminal (CK8/18) e actina de músculo liso (1A4) em carcinoma de mama

Delgallo, William Davila [UNESP]

31 August 2007

Made available in DSpace on 2014-06-11T19:32:50Z (GMT). No. of bitstreams: 0 Previous issue date: 2007-08-31Bitstream added on 2014-06-13T21:04:58Z : No. of bitstreams: 1 delgallo_wd_dr_botfm.pdf: 223230 bytes, checksum: 254dbff0ba8e45f49db67178b8a1ae49 (MD5) / Estudos de expressão gênica têm identificado vários grupos moleculares de carcinoma de mama, com diferentes comportamentos clínico e biológico. A correlação entre “cDNA microarray” e imunoistoquímica(IQ) com marcadores para citoceratinas, Her2/neu, receptor de estrógeno(RE) e de células basais mioepiteliais (1A4, S-100 e p63), identificaram cinco grupos: (1) luminal A (RE+; Her2/neu-), (2) luminal B (RE+; Her2/neu+), (3) superexpressão de Her2/neu (RE-; Her2/neu+), (4) tipo basal (RE-; Her2/neu-; Ck 5/6 +) e (5) nenhum destes (“null”). Os de tipo luminal expressam citoceratinas de padrão luminal (Ck8/18) e os de tipo basal expressam citoceratinas 5/6 e 14 ou marcadores de células basais mioepiteliais. Avaliamos a expressão de Ck5/6, Ck8/18 e 1A4 em material de citoinclusão, comparando-a ao espécime cirúrgico. Material e Métodos: Foram selecionados 62 casos, seqüenciais, de carcinoma de mama diagnosticados por PAAF, com citoinclusão e espécime cirúrgico. Cortes de citoinclusão e do espécime cirúrgico foram imunocorados para Ck 5/6, Ck 8/18 e 1A4. Resultados e Conclusão: Os valores, em porcentagem, de sensibilidade, especificidade, valor preditivo positivo(VPP), valor preditivo negativo(VPN) e acurácia foram, respectivamente: Ck5/6 (77, 100, 100, 92 e 94); Ck8/18 ( 98, 66, 96, 80 e 95) e 1A4 ( 92, 96, 85, 98 e 95). Portanto, a identificação de Ck5/6, Ck8/18 e 1A4 por IQ em material de citoinclusão é método confiável, com resultados muito próximos aos obtidos no espécime cirúrgico e pode contribuir para a classificação dos carcinomas mamários de expressão luminal e basal, fornecendo informações importantes que possam orientar na escolha do tratamento, bem como na avaliação de fatores prognósticos e preditivos. A importância da obtenção de dados morfológicos e imunoistoquímicos sobre os carcinomas mamários através do material... (Rewsumo completo, clicar acesso eletrônico abaixo) / Genetic expression studies have identified many molecular groups of breast carcinoma, with different clinical and biological behavior. The correlation between cDNA microarray and immunohistochemistry (IHC) with markers for cytokeratin, Her2/neu, estrogen receptor (ER) and of basal myoepithelial cells (1A4, S-100 e p63), identified five groups: (1) luminal A (ER+; Her2/neu-), (2) luminal B (ER+; Her2/neu+), (3) overexpression of Her2/neu (ER- ; Her2/neu+), (4) basal-like (ER- ; Her2/neu-; Ck 5/6 +) and (5) none of them (null). The luminal-like express cytokeratines of luminal pattern (Ck8/18) and the basal-like express cytokeratines 5/6 and 14 or markers of myoepithelial basal cells. We have evaluated the expression of Ck5/6, Ck8/18 and 1A4 in cell block comparing it to the surgical specimen. Material and Methods: 43 62 cases have been selected, sequencial, of breast carcinoma diagnosed through fine needle aspiration (FNA), with cell block and surgical specimen. Cuts of cell block and from the surgical specimen were immunostained for Ck 5/6, Ck 8/18 and 1A4. The value, in percentage, of sensibility, specificity, positive predictive value, negative predictive value, and accuracy were respectively: Ck5/6 (77, 100, 100, 92 e 94); Ck8/18 (98, 66, 96, 80 e 95) e 1A4 ( 92, 96, 85, 98 e 95). Therefore, the identification of CK5/6, 8/18 and 1A4 for IHC in cell block is a reliable method, with results very close to the ones obtained in the surgical specimen, and it can contribute to the sub classification of the breast carcinomas of luminal and basal expression, providing important information, which can orientate the treatment... (Complete abstract click electronic access below)

Mamas - Cancer - Cirurgia

Actina de músculo liso

Caracinoma de mama

Citologia de inclusão

Citoceratinas

Breast carcinoma

Smooth muscle actin

Caracterização da crotamina e seu efeito sobre a contratilidade da musculatura lisa do ducto deferente de rato / Characterization of crotamine and its effect in the smooth muscle contraction of rat vas deferens

Mariana Dangelo Martins Kmaid El-corab

27 November 2015

A crotamina, um peptídeo catiônico que possui 42 aminoácidos e 4,88 kDa, é proveniente do veneno de Crotalus durissus terrificus. Ela apresenta características que permitem sua forte interação com alvos moleculares e membranas biológicas e assim foi o primeiro peptídeo de veneno a ser classificado como um CPP (cell penetrating peptide), justificando seus importantes efeitos biológicos e suas diversas atividades farmacológicas. A crotamina é descrita por sua atividade miotóxica, tendo como efeito a paralisia e espasmos das patas traseiras de ratos e camundongos. Esse fenômeno é descrito por ações em canais de Na+ e/ou K+ e consequente aumento do influxo intracelular dos níveis do íon Ca2+. Estudos a descrevem como um agente despolarizante utilizando a musculatura esquelética como modelo experimental. Outra atividade descrita da crotamina é um aumento na liberação basal de acetilcolina (ACh) e dopamina no sistema nervoso central de ratos. Até o momento, pouco ou nenhum estudo foi realizado em musculatura lisa. A junção neuromuscular autônoma difere em vários aspectos importantes da já conhecida junção neuromuscular esquelética. O ducto deferente de rato (DDR), um órgão par e tubular pertencente à genitália acessória masculina, foi utilizado como modelo experimental por ser um dos órgãos periféricos mais densamente inervados pelo sistema nervoso autônomo simpático. Esse fato, o torna uma importante ferramenta para estudos que envolvam a neurotransmissão e a ação de drogas adrenérgicas. O objetivo do presente trabalho é investigar o efeito da crotamina na contração da musculatura lisa. A crotamina foi isolada a partir do veneno de C. d. terrificus por cromatografia de exclusão molecular seguida de troca iônica. Os estudos em modelos animais foram realizados utilizando o DD (porção prostática) de ratos Wistar com 5 meses de idade entre 350 g (protocolo CEUA 1261/14). O estudo de neurotransmissão foi feito em sistema de órgão isolado (n=6) por estimulação elétrica transmural com tensão de 70V, 3ms de duração em frequências de 0,05 (30 min) e 1; 5 10 e 20Hz (30 seg). A contração isométrica foi registrada em gramas de tensão. Em todos os experimentos a crotamina (0,1;0,5 e 1g/ml) incubada 30 min antes da estimulação. O efeito máximo de contração (Emax) do componente fásico e tônico foi usado como medida. O componente pós-sináptico foi avaliado por meio de curvas dose-resposta de noradrenalina e dose única de ATP (10-3M) na presença ou ausência da crotamina. A diferença estatística foi avaliada pelo teste-t de student (P0,05). Os ensaios de estimulação elétrica de baixa frequência (0,05Hz) revelaram que a crotamina (0,1 e 0,5g/ml) promoveu uma diminuição da contração do DDR (95,7±4,6% e 85,4±5,9%, respectivamente) enquanto que na dose de 1 g/mL de crotamina este efeito não foi significativo. Na curva de freqüência observamos também com as mesmas concentrações de crotamina uma tendência à diminuição da contração fásica e tônica enquanto que a dose de 1 g/mL promoveu um aumento na contração fásica na freqüência de 20,0Hz ((3,2±0,3) em relação ao controle (2,2±0,2). O componente pós-sináptico não foi alterado pela crotamina conforme evidenciado pela curva concentração-resposta de noradrenalina e concentração única de ATP. Com base nos resultados obtidos, concluímos que a crotamina atua apenas no componente pré-sináptico da contração do DDR, provavelmente interferindo na neuroliberação de ATP e noradrenalina. Ela apresenta um efeito bifásico, dependendo da dose utilizada, inibindo ou potencializando a resposta, efeito semelhante ao da -defensinas, uma proteína cuja estrutura se assemelha bastante com a da crotamina. / Crotamin, a 4.88 kDa polypeptide composed of 42 amino acids, is derived from the venom of Crotalus durissus terrificus. It presents features that allow its strong interaction with molecular targets and biological membranes and was the first venom peptide to be classified as a CPP (cell penetrating peptide), justifying the important biological effects and different pharmacological activities of crotamine. It is described by its myotoxic activity, having the effect of paralysis and spasms of the hind legs of mice and rats. This phenomenon is described by actions on Na+ channels and / or K+ and the resulting increase in intracellular influx of Ca2+ ion levels. Studies describe crotamine as a depolarizing agent and neurotransmitter release inductor using the skeletal muscle as an experimental model. Another activity of crotamine described is an increase in the basal release of acetylcholine (ACh) and dopamine in the central nervous system of rats. To date, few or no study has been performed in smooth muscle. The autonomous neuromuscular junction differs in several important aspects of already known skeletal neuromuscular junction. The vas deferens, a pair and tubular organ belonging to the male accessory genitalia, was used as experimental model because it is one of the most densely peripheral organs innervated by the sympathetic nervous system. This fact makes it an important tool for studies involving the neurotransmission and the action of adrenergic drugs. A better understanding of crotamine mechanism of action is fundamental to the development of a pharmacological agent or a possible drug. In this context, we aim to investigate the crotamine behaviour in the contraction of the smooth muscle vas deferens through neurogenic stimulation and exogenous drugs.

contração

crotamina

ducto deferente

musculatura lisa

contraction

crotamine

smooth muscle

vas deferens

Difusão anômala de micropartículas em células no regime de altas frequências / Anomalous diffusion of microbeads in cells at a high frequency regime

Adriana Valerio

07 November 2017

Este trabalho tem como objetivo caracterizar experimentalmente a difusão anômala de microesferas em células com alta resolução temporal. As microesferas são cobertas com um peptídeo para que elas fiquem aderidas ao citoesqueleto celular (CSK), de forma que quando o CSK se movimenta, as microesferas se movimentam junto. A grande parte dos trabalhos na literatura usa técnicas ativas, que consistem em aplicar uma perturbação na célula, para estudar a movimentação das microesferas, diferente da técnica usada neste trabalho, que é passiva. A vantagem de usar a técnica passiva é que é possível olhar a difusão das microesferas, sem haver fatores externos ativos atuando, porque o CSK já é um ambiente sujeito a forças dos próprios motores celulares, o que está relacionado com o comportamento anômalo. Ao calcular o deslocamento quadrático médio (MSD) das microesferas, os regimes aos quais as microesferas estão sujeitas, são o subdifusivo e o superdifusivo, e ambos possuem características que podem ser consideradas comportamento anômalo. Neste trabalho focamos em estudar a difusão anômala a altas frequências, usando uma câmera que pode chegar a 1000 frames por segundo (fps) para observações curtas, ou em torno de 200 fps, sustentável por longos tempos, a fim de evidenciar o comportamento anômalo. Conseguimos mostrar que a movimentação das microesferas segue uma lei de potência para deslocamentos normalizados |Z| > 3, o que indica que o fenômeno é livre de escala, corroborando com a hipótese de o citoplasma celular ter um comportamento do tipo mole. Além disso, como a análise do movimento é baseada na análise de imagem da posição das microesferas, propusemos um estudo para estimar o erro na posição das microesferas. / The aim of this master\'s thesis is to characterize experimentally anomalous diffusion of microbeads in cells with high temporal resolution. The microbeads are coated with a peptide, such that they can bound to integrins, which is a specific cell surface receptor, thus when the cytoskeleton moves the microbeads move together. The majority of works in scientific literature deals with active techniques, that consists of applying a disturbance on the cell, in order to investigate the movement of the beads, differently from the passive technique used in this work. The advantage of using the passive technique is that it makes possible to look to diffusion without having external active factors, because the cell cytoskeleton itself is an environment subjected to forces, provided by cell motors, which has been related to the anomalous behavior in the mean squared displacement. When calculating the microbeads mean squared displacement (MSD), they are subjected to the subdiffusive and supperdifusive regimes, and both have characteristics that can be considered anomalous behavior. Our goal was to study anomalous diffusion at high frequencies by using a camera that reaches up to 1000 frames per second (fps), for shorter observation times, or around 200 fps, sustainable for longer observation times, having the purpose of evidencing the anomalous behavior. We were able to show that the microbeads movement follows a power law for normalized displacements |Z| > 3, indicating that the phenomenon is scale-free, agreeing with the hypothesis that the cellular cytoplasm has a soft glassy behavior. Besides, since the movement analysis is based on the microbeads position image analysis, we have proposed a way to estimate the error in the microbeads position.

lei de potência

músculo liso

reologia

viscoelasticidade

power law

rheology

smooth muscle

viscoelasticity