Determining the Physiological Contribution of Adipocyte Subpopulations

Luong, Quyen V.

23 September 2019

No description available.

Biology

Molecular Biology

Adipose Subpopulations

Inflammation

Obesity

Adipose Tissues

Heterogeneity

Crown-like Structures

DISCO

Spatial Distribution

Photo-biomodulation of human skin fibroblast sub-populations: a systematic approach for the optimization of optical treatment parameters

Mignon, Charles

January 2017

The thesis presents a rational path for the optimization of the selection of optical treatment parameters in photobiomodulation of human skin fibroblasts. The project begins with an extensive analysis of 90 bibliographic reports in photobiomodulation published between 1985 and 2015, and revealed major inconsistencies in optical parameters selected for clinical applications. Seeking greater clarity for optimal parameter choice, a systematic approach to disentangle the multiple factors underpinning the response of human dermal fibroblasts in vitro to visible and near-infra red (NIR) light was employed. Light-based devices were constructed to specifically and systematically screen the optical parameter window (i.e. wavelength, irradiance and dose) observed in literature. Additionally, critical culture and treatment conditions that have dramatic impact on the outcome of specific light treatment of these human skin dermal cells were identified. In particular, environmental oxygen concentration, cell confluency and serum concentration were all found to have a great effect on the response of dermal fibroblasts to light. In parallel, the induction of reactive oxygen species (ROS) by short visible wavelengths on two dermal fibroblast sub-populations or lineage, reticular and papillary, was monitored by live-cell imaging. The ROS species were found to be created in or close to mitochondria. Lastly, gene expression studies revealed a strong impact of short visible wavelengths, as compared to long and NIR wavelengths on both subpopulations of human dermal fibroblasts. In particular, blue light (450 nm) specifically down-regulated proliferation, metabolism and protein synthesis molecular pathways. At the protein level, 450-nm light inhibited the production of procollagen I in human reticular and papillary fibroblasts in a dose-dependent manner. Gene expression results were in agreement i.e., the same light parameter down-regulated collagen fiber genes, integrins and up-regulated collagenase MMP1. This thesis concludes with a chapter presenting a characterization of the accuracy of a potential translation tool for the prediction of optical photon density inside human skin. / Marie Skłodowska-Curie Actions.

Photobiomodulation

Skin

Light

Subpopulations

Design of experiment

Monte Carlo method

Human dermal fibroblasts (HDF)

Molecule Analysis in Biological Systems: Plasmids, Nucleotides, and Surface Biomolecules

Wamer, Nathan C.

15 September 2022

No description available.

Analytical Chemistry

Microbiology

Biochemistry

Molecular Biology

Pseudomonas aeruginosa

Study towards the development of broadly reactive live attenuated influenza vaccines with focus on high interferon inducing viral subpopulations

Ghorbani, Amir

15 September 2022

No description available.

Virology

Immunology

Avian Influenza Virus

Live Attenuated Vaccine

Viral Subpopulations

Innate Immunity

Defective Viral Genome

In Ovo Vaccination

Analyse des sous populations lymphocytaires, et plus particulièrement les cellules NK, dans la polyglobulie primitive

Sanchez, Carole

14 December 2012

Caractérisée par la présence de la mutation JAK2 V617F, la polyglobulie primitive voit son développement contenu par des saignées mais est associée à une incidence plus élevée de cancers. Une exploration globale de l'immunité des patients a été réalisée par la quantification des sous populations lymphocytaires de l'immunité innée et adaptative. Ceci a permis la mise en évidence d'une diminution des lymphocytes B et d'une augmentation des cellules NK. Les cellules NK sont réputées pour leurs propriétés antitumorales mais elles ne sont pourtant pas capables d'éradiquer la PV, posant la question de leurs capacités fonctionnelles. Si les cellules NK des patients présentent une activité cytotoxique basale inférieure aux témoins, elles ne présentent pas d'anomalies de l'expression de leurs récepteurs, de la production de molécules cytolytiques ou de prolifération. Par contre, les cellules NK d'un patient ayant développé une érythroleucémie ou des cellules NK de sujets âgés par rapport à des témoins plus jeunes présentent des anomalies d'expression des récepteurs. L'augmentation des cellules NK pourrait être liée à la mutation JAK2 V617F. Si cette mutation est présente dans les lymphocytes de tous les patients, il existe des arguments pour sa présence dans les cellules NK de certains patients. Enfin, une analyse transcriptomique a permis de définir un profil d'expression propre aux cellules NK des patients. / Characterized by the presence of the JAK2 V617F mutation, polycythemia vera's development is content by phlebotomy but is associated with a higher incidence of cancer. A global exploration of the immunity of patients was performed by quantification of lymphocyte subpopulations of innate and adaptive immunity. This allowed the detection of a decrease in B cells and an increase in NK cells. NK cells are known for their antitumor properties but they are not yet able to eradicate PV, raising the question of their functional abilities. If NK cells of patients have a lower basal cytotoxic activity than healthy donors, they do not show abnormal expression of their receptors, the production of cytolytic molecules or proliferation. On the contrary, NK cells from a patient who developed erythroleukemia or NK cells from elderly healthy donors compared with younger healthy donors exhibit abnormalities of receptors expression. The increase in NK cells could be related to the JAK2 V617F mutation. If the mutation is present in cells of all patients, there are arguments for its presence in the NK cells of some patients. Finally, transcriptome analysis has identified an expression profile specific to NK cells of patients.

Polyglobulie primitive

Cellules NK

Sous populations lymphocytaires

Mutation JAK2 V617F

Récepteurs NK

Polycythemia vera

NK cells

Lymphocytes subpopulations

Mutation JAK2 V617F

NK cells receptors

Función y biogénesis mitocondrial. Diferencias entre géneros

Justo López, Roberto

25 July 2005

El objetivo principal de esta tesis se ha centrado en el estudio de las diferencias entre ratas macho y hembra en la morfología, la función y la biogénesis mitocondrial del tejido adiposo marrón (TAM) y del hígado, mediante el análisis de distintas subpoblaciones mitocondriales obtenidas a través del fraccionamiento de la población mitocondrial total. Los resultados han puesto de manifiesto que las diferencias entre géneros a nivel mitocondrial tanto en el TAM y como en el hígado podrían ser atribuidas a la existencia de una subpoblación mitocondrial altamente diferenciada en las hembras, hecho que podría ser indicativo de un proceso de biogénesis mitocondrial distinto entre ambos géneros. Los resultados sugieren la existencia de un factor común a ambos tejidos que influiría en la regulación de dicho proceso. En este sentido, las hormonas sexuales podrían ser uno de los factores candidatos responsables de las diferencias observadas en el presente trabajo. / The main goal of this thesis has been focused on the study of gender differences in the mitochondrial morphology, function and biogenesis both in brown adipose tissue (BAT) and in liver, through the analysis of the several mitochondrial subpopulations isolated by means of the fractionation of the whole mitochondrial population. Results have reflected that the gender dimorphism stated in mitochondrial population both in BAT and in liver could be attributed to the existence to more highly differentiated mitochondria in female rats, which could be the result of a different mitochondrial biogenesis process between genders. Since the existence of a common factor which influences this process in both tissues could be hypothesized, sexual hormones could be one of the main factors responsible for the differences described in the present work

liver

Mitochondrial function

subpoblaciones mitocondriales

tejido adiposo marrón

hígado

Función mitocondrial

brown adipose tissue

mitochondrial subpopulations

Bioquímica i Biologia Molecular

577

Caracterização do perfil de monócitos: comparação da fenotipagem entre adultos e crianças sadias e em crianças portadoras de dermatite atópica

Paiva, Renata da Silveira Rodrigues

15 December 2016

Submitted by Viviane Lima da Cunha (viviane@biblioteca.ufpb.br) on 2017-06-01T14:19:33Z No. of bitstreams: 1 arquivototal.pdf: 3473301 bytes, checksum: 4d22636d8d38c872a66d2aa8bf1d2e3f (MD5) / Made available in DSpace on 2017-06-01T14:19:33Z (GMT). No. of bitstreams: 1 arquivototal.pdf: 3473301 bytes, checksum: 4d22636d8d38c872a66d2aa8bf1d2e3f (MD5) Previous issue date: 2016-12-15 / Monocytes and macrophages represent keys components of the immune response. Based on the expression of LPS co-receptor CD14 and CD16 expression, FCγ III receptor, monocytes are classified into 3 subtypes: classical monocytes, which are CD14hiCD16-; intermediate monocytes, which are CD14hiD16+; and non-classical monocytes, CD14lowCD16+. AD is a chronic inflammatory cutaneous disease, with multifactorial etiology. Our group performed comparative analysis of monocytes subtypes through the study of the frequency and medium fluorescence intensity of surface molecules (HLADR, CCR5, CD80, CD86, PD1L) and cytokine (IL-6, TNF, IL10) in adults and children by using flow cytometry. The study was performed in two stages. First we compared the subtypes of monocytes from healthy adults and children, and then between healthy children and children with atopic dermatitis (AD). The role of monocyte activation and modulation of the inflammatory process is the subject of our investigation. The results of this study showed that: (1) the relative frequency of monocytes subtypes was similar in adults, healthy children and children with AD, with a predominance of classical monocytes; (2) Classical, intermediate and nonclassical monocytes of children with AD have higher HLA-DR expression when compared to those of healthy children, and monocytes of healthy children have higher expression than healthy adults; (3) adults, healthy children and DA children have higher frequency and expression of CCR5 in intermediate and nonclassical that in classical monocytes; (4) the frequency and expression of CD80 was higher in intermediate and nonclassical monocytes both in children and healthy adults and CD86 expression was more pronounced in intermediate monocytes, in these two groups, beyond wich the expression of CD80 and CD86 molecules on classical monocytes of children with AD was higher than in healthy children; (5) PD1L frequency in monocytes subtypes was similar in adults and children, however, there is a higher expression of this molecule in children classical monocytes when compared to healthy adults classical monocytes. In addition, atopic children have higher expression of this molecule on classical monocytes than healthy children; (6) intermediate and nonclassical monocytes of healthy adults and children have greater inflammatory activity than classical monocytes when evaluating the frequency and expression of IL-6 and TNF-α, contrary to what is observed in children with AD who have greater frequency and expression of IL-6 and TNF-α in classical monocytes compared to healthy children; (7) intermediate and nonclassical monocytes have increased IL10 production than classical monocytes in healthy adults and children. Thus, our results revealed that the relative monocytes frequency is constant in the three studied population groups, but the frequency and expression of surface molecules and cytokines presented significant peculiarities. Summarizing, healthy children have greater expression of HLA-DR molecule than healthy adults, and atopic children have greater expression than healthy children. Monocytes subtypes more involved inflammatory response in healthy adults and children are intermediate and nonclassical monocytes, while classical monocytes in atopic children are more involved in inflammatory response than the same subtype in healthy children. These findings revealed changes in the innate immunity of children with atopic dermatitis extremely important for understanding the pathophysiology of disease. / Os monócitos e macrófagos representam componentes fundamentais da resposta imune. Com base na expressão do co-receptor de LPS CD14 e na expressão do CD16, receptor FCγIII, os monócitos são classificados em 3 subtipos: monócitos clássicos, que são CD14hiCD16-; monócitos intermediários, que são CD14hiD16+; e monócitos não-clássicos, ou CD14lowCD16+. A DA é uma doença inflamatória cutânea crônica, de etiologia multifatorial. Nosso grupo realizou análise comparativa entre os subtipos monocitários por meio do estudo da frequência e da média de intensidade de fluorescência (MFI) de moléculas de superfície (HLA-DR, CCR5, CD80, CD86, PD1L) e da produção de citocinas (IL6, TNFα, IL10) em adultos e crianças utilizando a citometria de fluxo. A pesquisa foi executada em duas etapas. Primeiro comparamos os subtipos de monócitos entre adultos e crianças saudáveis e em seguida, entre crianças sadias e crianças portadoras de dermatite atópica (DA). O papel dos monócitos na ativação e modulação do processo inflamatório foi objeto da nossa investigação. Os resultados desse estudo mostraram que: (1) a frequência relativa dos subtipos de monócitos foi similar em adultos, crianças saudáveis e crianças portadoras de DA, com predomínio de monócitos clássicos; (2) monócitos clássicos, intermediários e não-clássicos de crianças atópicas apresentaram maior expressão de HLA-DR que os mesmos subtipos em crianças sadias e essas, que adultos sadios; (3) adultos, crianças saudáveis e crianças doentes apresentaram maior frequência e expressão de CCR5 em monócitos intermediários e monócitos não-clássicos; (4) a frequência e expressão do CD80 foi maior em monócitos intermediários e não clássicos tanto em crianças como em adultos saudáveis e a expressão de CD86 foi maior em monócitos intermediários desses dois grupos. Já a expressão das moléculas de CD80 e CD86 em monócitos clássicos de crianças portadoras de DA foi maior que em crianças saudáveis; (5) a frequência de PD1L nos subtipos de monócitos foi semelhante em adultos e crianças, entretanto, houve maior expressão dessa molécula em monócitos clássicos de crianças que em adultos saudáveis e crianças atópicas apresentaram maior expressão desta molécula em monócitos clássicos que crianças saudáveis; (6) monócitos intermediários e não-clássicos de adultos e crianças saudáveis apresentaram maior atividade inflamatória que monócitos clássicos ao se avaliar a frequência e expressão de IL-6 e TNF-α, ao contrário do que se observou em crianças com DA, que apresentaram maior frequência e expressão de IL-6 e TNF-α em monócitos clássicos que as crianças saudáveis; (7) monócitos intermediários e não-clássicos demonstraram maior produção de IL10 que monócitos clássicos em adultos e crianças saudáveis. Nossos resultados mostraram, portanto que a frequência relativa de monócitos é constante nos três grupos populacionais estudados, mas a frequência e expressão de moléculas de superfície e citocinas apresentam particularidades significativas. Em resumo, crianças atópicas apresentam maior expressão de HLA-DR que crianças saudáveis e essas, que adultos saudáveis. Os subtipos de monócitos mais envolvidos na resposta inflamatória em adultos e crianças sadias são monócitos intermediários e não-clássicos, enquanto monócitos clássicos de crianças atópicas são mais inflamatórios quando comparados ao mesmo subtipo em crianças saudáveis. Essas descobertas revelam alterações na imunidade inata de crianças portadoras de dermatite atópica de extrema importância para a compreensão da fisiopatologia da doença.

Monócitos

Citometria

Subpopulações de Monócitos

Resposta Inflamatória

Citocinas

Marcadores Celulares

Monocytes

Cytometry

Subpopulations of Monocytes

Inflammatory Response

Cytokines

Cell Markers

CIENCIAS BIOLOGICAS::FISIOLOGIA

Změny v distribuci subpopulací B lymfocytů u pacientů s Crohnovou chorobou před a po biologické léčbě / Changes in distribution of B lymphocyte subpopulations in patients with Crohn disease before and after biological therapy

Suchá, Renata

January 2016

B-lymphocytes are lymphoid cells, which are a part of the adaptive/innate immune system and generate antibodies. Recently, many studies have supported hypothesis that different rather minor B-lymphocyte subpopulations may play a direct and indirect role in immunopathogenesis in human pathologies such as Crohn's disease (CD). The aim of current study was therefore to investigate distribution of frequencies of B lymphocyte subpopulations (from transient to mature effector B cell stages) in peripheral blood of healthy subjects (CO), patients with Crohn's disease (CD) and ulcerative colitis (UC). Thus, using 11-colour flow cytometry we have analysed 30 blood samples of individuals, including 14 healthy controls, 11 patients with Crohn's disease and 5 with UC. In 6 patients with CD we have had an opportunity to analyze blood samples collected 2 hours after an administration of anti-TNF therapy. Higher frequencies of memory B-lymphocytes (CD19+ CD27+ , CD19+ CD20+ CD27+ and CD19+ CD20+ CD27+ IgM+) were found in patients with CD as compared to COs. (20.06±13.58%; 17.61±13.48%; 88.60±20.56% vs. 11.75±26.47%; 11.25±26.50%; and 66.82±22.60%), in case of CD19+CD20-CD27-IgM+ B-lymphocytes the difference was statistically significant (57.15±17.21% in CD vs. 19.59±31.79% in CO; p=0.0341), which is in accordance...

Entzündungszelldifferenzierung im Endometrium der Stute

Rudolph (geb. Huth), Nicole

13 November 2019

Subklinische entzündliche Veränderungen des Endometriums können nur durch die histopathologische Untersuchung eines Bioptates diagnostiziert werden und sind von besonderer Bedeutung bei Fertilitätsstörungen. Die nicht-eitrige (NE) Endometritis ist gekennzeichnet durch eine Infiltration des Endometriums mit Lymphozyten, Plasmazellen und/oder Makrophagen. Die genaue Pathogenese ist unklar. Die immunhistologische Phänotypisierung dieser Zell-(sub-)populationen kann möglicherweise pathogenetische Hinweise geben. Der immunhistologische Nachweis equiner Immunzellen ist jedoch fast ausschließlich an Gefrierschnitten etabliert. Dies ist für die Routinediagnostik ungeeignet. Demzufolge ergaben sich die folgenden Ziele: 1. Eine alternative Methode zur Gewebsfixierung zu etablieren, die in der Routinediagnostik praktikabel einsetzbar ist, die einen guten Strukturerhalt, eine geeignete Anfärbbarkeit und ideale Auswertbarkeit gewährleistet sowie umfangreiche immunhistochemische Untersuchungen ermöglicht; 2. Die immunhistochemische Phänotypisierung von Lymphozyten- und Makrophagen-(sub-)populationen an fixierten equinen Gewebeproben zu entwickeln; 3. Eine semiquantitative Bestimmung der endometrialen Entzündungszellen ohne und mit einer NE Endometritis durchzuführen. Tiere, Material & Methoden: Gewebeproben (Lymphknoten als Referenzgewebe und endometriales Gewebe) wurden von 5 Stuten im Rahmen der Sektion entnommen, in Formalin (F), HOPE® (H) oder IHC Zinc Fixative (Z) fixiert und zusätzlich als natives Gefriermaterial aufgearbeitet. Es erfolgte eine vergleichende Beurteilung der Gewebemorphologie, des Färbeverhaltens und der Artefakte am equinen Endometrium in HE gefärbten Gefrierschnitten bzw. im fixierten, Paraffin-eingebetteten Material (F, H und Z). Equine Lymphknoten dienten als Referenzgewebe für die immunhistochemische Etablierung der Lymphozytenmarker (anti-CD3, -CD4, -CD8) an Gefrierschnitten und am fixierten, Paraffin-eingebetteten Material (F, H und Z). F- und Z-fixiertes Referenzgewebe (Leber, Dünndarm, Darmlymphknoten) von 4 Stuten wurde für die Etablierung der Makrophagenmarker (anti-CD172a, -CD14, -CD206) verwendet. Die Immunreaktionen der Primärantikörper wurden verglichen. Als Resultat aus den vergleichenden Analysen wurde die Z-Fixierung als effektivste alternative Fixierungsmethode ausgewählt. Im abschließenden Teil der Untersuchungen wurden 28 Z-fixierte Endometriumbioptate hinsichtlich der Entzündungszellen semiquantitativ ausgewertet. 4 Stuten zeigten keine Entzündungsreaktion und dienten als Kontrolle. 24 Stuten wiesen eine oberflächliche NE Endometritis auf. Die Anzahl CD3+, CD4+, CD8+, CD20+, CD172a+, CD14+ und CD206+ Zellen sowie die Anzahl von Plasmazellen mittels Methylgrün-Pyronin-Färbung wurde an Serienschnitten in 5 zufällig ausgewählten Gesichtsfeldern (400x) jeweils für das Stratum compactum, Stratum spongiosum und das luminale sowie glanduläre Epithel erhoben. Ergebnisse: 1. Die Z-Fixierung zeigt mit der F-Fixierung vergleichbare, exzellente Eigenschaften hinsichtlich des Strukturerhalts, der Anfärbbarkeit und Auswertbarkeit. Sie übersteigt insgesamt die Eigenschaften der H-Fixierung: die Z-Fixierung erweist sich einfacher in der Anwendung und zeigt eine geringere Artefaktbildung. 2. Die immunhistochemische Charakterisierung von T- und B-Lymphozyten, Helfer-T-Lymphozyten sowie zytotoxischen T-Lymphozyten und Makrophagenpopulationen sowie der Nachweis von Plasmazellen mittels Methylgrün-Pyronin-Färbung an Z-fixierten equinen Gewebeproben ist möglich. 3. Im entzündlich veränderten Endometrium sind mehr CD3+, CD4+, CD8+, CD20+, CD172a+, CD206+ Zellen sowie Plasmazellen nachweisbar als in unveränderten Gewebeproben bezogen auf das Stratum compactum und Stratum spongiosum. Die durchschnittliche Anzahl CD3+ Zellen ist im Stratum compactum NE Endometritiden knapp 3x höher als im unveränderten Endometrium. Wenige CD20+ B-Zellen und CD172a+ Makrophagen sowie eine unterschiedliche Anzahl an Plasmazellen sind innerhalb des Stratum compactum entzündlich veränderter Endometrien nachweisbar. Es existieren große individuelle Unterschiede in der Anzahl CD4+ und CD8+ T-Zellen in Endometrien ohne sowie mit einer Entzündung. Schlussfolgerungen: Eine Integration der Z-Fixierung in die Routinediagnostik mit zusätzlichen Anwendungsmöglichkeiten ist problemlos möglich. Die immunhistochemische Entzündungszelldifferenzierung im Endometrium der Stute kann an fixierten equinen Endometriumbioptaten durchgeführt werden und bietet darüber hinaus die Möglichkeit, diese Methode an anderen equinen Organen anzuwenden. Die Ergebnisse der semiquantitiven Auswertung deuten auf das mögliche Vorliegen unterschiedlicher Formen der nicht-eitrigen Entzündung hin. Das etablierte Verfahren gibt möglicherweise nähere Hinweise auf immunologische Konstellationen, die das Auftreten einer nicht-eitrigen Endometritis begünstigen.:INHALTSVERZEICHNIS I ABKÜRZUNGSVERZEICHNIS II 1 EINLEITUNG 1 2 LITERATURÜBERSICHT 2 2.1 Das Endometrium der Stute 2 2.1.1 Endometritiden 4 2.1.1.1 Eitrige Endometritis 4 2.1.1.2 Nicht-eitrige Endometritis 5 2.1.1.3 Sonderformen 6 2.1.2 Resistant und susceptible mares 8 2.1.3 Entzündungszelltypisierung im Endometrium der Stute 10 2.1.4 Diagnostische Bedeutung des Endometriumbioptates 13 2.2 Immunologie 14 2.2.1 T-Lymphozyten 14 2.2.2 B-Lymphozyten 17 2.2.3 Makrophagen 18 2.2.4 Immunhistochemische Charakterisierung von equinen Entzündungszellen 21 2.3 Fixierungsmethoden 24 2.4 Fazit aus der Literatur bezüglich der Fragestellung dieser Arbeit 26 3 PUBLIKATIONEN 28 3.1 Publikation 1 inkl. Stellungnahme zum Eigenanteil 28 3.2 Publikation 2 inkl. Stellungnahme zum Eigenanteil 39 4 DISKUSSION 53 4.1 Etablierung alternativer Methoden zur Gewebefixierung 54 4.2 Immunhistochemische Detektion von Immunzell- (sub-)populationen 59 4.3 Erkenntnisse im Hinblick auf die Pathogenese nicht-eitriger Endometritiden 60 5 ZUSAMMENFASSUNG 63 6 SUMMARY 65 7 LITERATURVERZEICHNIS 67 8 DANKSAGUNG 81 / Clinically unapparent inflammatory alterations of the equine endometrium can only be diagnosed by the histopathological examination of a biopsy and are the main cause of subfertility in mares. The non-suppurative endometritis is characterised by infiltration of the endometrium with lymphocytes, plasma cells and/or macrophages. So far, the cause and pathogenesis of non-suppurative endometritis are unclear. The subclassification of the immune cell populations involved will likely provide important information on the etiology and pathogenesis of this disease. Available antibodies are often established exclusively for immunohistochemistry on cryostat sections of native frozen equine tissue. However, this method is impractical for the routine diagnostic work-up. The aim of the present study was: 1. To reveal the method most suitable for a routine diagnostic work-up in combination with proper tissue preservation, staining results as well as histological and immunohistochemical analysis; 2. To establish an immunohistochemical method for the detection of lymphocytes and macrophages including their subpopulations in fixed equine tissue samples; 3. To characterize the immune cell populations in fixed endometria of mares without and with non-suppurative endometritis. Material & methods: Equine endometrial tissue and intestinal lymph node were obtained from five mares during post mortem examination and were either fixed in formalin, HOPE® or IHC Zinc Fixative. Aditionally snap frozen tissue samples were processed for cryostat sectioning. HE stained cryostat sections and fixed paraffin embedded tissue samples (formalin, HOPE®, IHC Zinc Fixative) of the equine endometrium were analysed regarding tissue preservation, staining results and artefacts. To establish lymphocyte markers (anti-CD3, anti-CD4 and anti-CD8) immunohistochemically on cryostat sections and fixed paraffin embedded tissue samples (formalin, HOPE®, IHC Zinc Fixative) equine lymph node was used as reference. Formalin fixed and zinc fixed tissue samples with macrophage populations (liver, small intestine, intestinal lymph node) from four mares were used for the immunohistochemical establishment of the macrophage markers (anti-CD172a, anti-CD14, anti-CD206). The immunoreactivity of the primary antibodies was compared. The results of the comparative analysis revealed the most suitable alternative fixation method (zinc fixation). Finally, 28 zinc fixed endometrial biopsies were evaluated semiquantitatively with regard to the numbers of CD3+, CD4+, CD8+, CD20+ lymphocytes, CD172+, CD14+, CD206+ macrophages as well as plasma cells. Four mares had no evidence of endometritis and represent the control group. The remaining 24 mares showed a mild superficial non-suppurative endometritis. The comparative analysis was performed in serial sections within five randomly selected high power fields (400x). Positive cells were counted separately within the luminal and glandular epithelium, the stratum compactum and the stratum spongiosum. Results: 1. The zinc fixation provides excellent staining results, tissue preservation and allows histological and immunohistochemical analysis. It has even some advantages compared to the HOPE® fixation regarding the routine diagnostic work-up. The zinc fixation produces less artefacts. 2. The zinc fixation allows the immunohistochemical detection of all applied T- and B-lymphocyte-, helper- and cytotoxic-T-cell- and macrophage-markers and the histochemical detection of plasma cells (methyl green-pyronin stain) within equine fixed tissue. 3. Endometria with non-suppurative endometritis have higher numbers of CD3+, CD4+, CD8+, CD20+, CD172a+, CD206+ as well as plasma cells within the stratum compactum and stratum spongiosum than endometria without inflammation. The average cell count of CD3+ lymphocytes within the stratum compactum was approximately 3 x higher within inflamed endometria than this value obtained from endometria without endometritis. Few CD20+ B cells and CD172+ macrophages as well as variable numbers of plasma cells could be detected within the stratum compactum of mares with non-suppurative endometritis. Endometria with and without inflammation showed marked differences in the numbers of CD4+ and CD8+ T cells. Conclusion: The zinc fixation can be easily incoorporated into the routine diagnostic work-up and offers additional application possibilities. Immunohistochemical phenotyping of immune cells in the equine endometrium can be performed on fixed endometrial biopsies of the mare. Furthermore, a widespread applicability is possible, e. g. on other equine organs. These findings suggest the existence of different forms of non-suppurative endometritis. The established method will likely assist to reveal possible etiologies and predisposing conditions for non-suppurative endometritis.:INHALTSVERZEICHNIS I ABKÜRZUNGSVERZEICHNIS II 1 EINLEITUNG 1 2 LITERATURÜBERSICHT 2 2.1 Das Endometrium der Stute 2 2.1.1 Endometritiden 4 2.1.1.1 Eitrige Endometritis 4 2.1.1.2 Nicht-eitrige Endometritis 5 2.1.1.3 Sonderformen 6 2.1.2 Resistant und susceptible mares 8 2.1.3 Entzündungszelltypisierung im Endometrium der Stute 10 2.1.4 Diagnostische Bedeutung des Endometriumbioptates 13 2.2 Immunologie 14 2.2.1 T-Lymphozyten 14 2.2.2 B-Lymphozyten 17 2.2.3 Makrophagen 18 2.2.4 Immunhistochemische Charakterisierung von equinen Entzündungszellen 21 2.3 Fixierungsmethoden 24 2.4 Fazit aus der Literatur bezüglich der Fragestellung dieser Arbeit 26 3 PUBLIKATIONEN 28 3.1 Publikation 1 inkl. Stellungnahme zum Eigenanteil 28 3.2 Publikation 2 inkl. Stellungnahme zum Eigenanteil 39 4 DISKUSSION 53 4.1 Etablierung alternativer Methoden zur Gewebefixierung 54 4.2 Immunhistochemische Detektion von Immunzell- (sub-)populationen 59 4.3 Erkenntnisse im Hinblick auf die Pathogenese nicht-eitriger Endometritiden 60 5 ZUSAMMENFASSUNG 63 6 SUMMARY 65 7 LITERATURVERZEICHNIS 67 8 DANKSAGUNG 81

info:eu-repo/classification/ddc/636.089

ddc:636.089

THE EFFECT OF CURCUMIN ON LEWIS LUNG CARCINOMA

Yan, Dejun

01 July 2011

No description available.

Animals

Biochemistry

Biology

Biomedical Research

Biophysics

Cellular Biology

Health Sciences

Medicine

Molecular Biology

Oncology

Pharmacology

Physiology

CURCUMIN

LEWIS LUNG CARCINOMA

CURCUMIN-SURVIVING SUBPOPULATIONS

STROMA

LIGHT