Characterization of adherence, cytotoxicity and biofilm formation by Gardnerella vaginalis

Patterson, Jennifer

26 April 2010

Worldwide, bacterial vaginosis (BV) is the most common vaginal disorder in women of childbearing age. BV is of major clinical importance due to its ability to significantly affect pregnancy outcome and enhance the transmission and acquisition of HIV. BV is characterized by a dramatic shift in the vaginal microflora; in most BV cases, the predominant bacterial species is Gardnerella vaginalis. It has been demonstrated that G. vaginalis forms an adherent biofilm on the vaginal epithelium of women with BV. Furthemore, evidence suggests that the high rate of recurrence associated with BV is related to incomplete eradication of the biofilm. The overall goal of this study was to characterize G. vaginalis virulence properties, including biofilm formation, in order to better understand the pathogenesis of BV and to improve available treatment methods. In an effort to tease apart the uncertain etiology of this disorder, we utilized in vitro assays to compare three virulence properties of G. vaginalis relative to other BV-associated anaerobes. Only G. vaginalis demonstrated all three virulence properties, including robust biofilm formation. It has been shown that the biofilm phenotype allows its constituent bacteria to be resistant to many negative environmental stimuli. Therefore, we studied the susceptibilities of biofilm vs. planktonic cultures to H2O2 and lactic acid. Biofilms tolerated higher concentrations of both chemicals; however, when the biofilm was proteolytically disrupted, sensitivity to the chemicals returned to planktonic levels. Since our data suggested a critical role for a protein in biofilm formation, a partial genome sequence of G. vaginalis was searched for sequence homology to known biofilm adhesins using the tBLASTn program. This revealed an open-reading frame encoding a hypothetical protein with significant homology to the staphylococcal Bap protein. Antibody towards a portion of the identified gene product was produced in rabbits by inoculation of a recombinant peptide to an antigenic region of the protein. Antibody inhibition assays against biofilm formation, adherence, initial adherence and aggregation were conducted. Relative expression levels of the biofilm-associated protein were analyzed under different conditions by western blot analysis. Finally, the protein was expressed in heterologous hosts and analyzed for an increase in biofilm formation.

biofilm

bacterial vaginosis

Gardnerella

biofilm associated protein

Medicine and Health Sciences

Investigating telomerase regulation in human breast cancer cells : a search for telomerase repressor sequences localised to chromosome 3P

Linne, Hannah Louise

January 2015

Cellular immortality is one of the ten hallmarks of human cancer and has been shown to be an essential prerequisite for malignant progression (Hanahan and Weinberg., 2011, Newbold et al., 1982, Newbold and Overell., 1983). In contrast, normal human somatic cells proliferate for a limited number of population doublings before entering permanent growth arrest known as replicative senescence. This is thought to be due to the progressive shortening of telomeric sequences with each round of cell division. Over 90% of human tumours, but not the majority of human somatic cells, have been found to express telomerase activity (Kim et al., 1994). The rate-limiting component of the human telomerase enzyme is the telomerase reverse transcriptase subunit, which is encoded by the hTERT gene. Transfection of hTERT cDNA into normal human fibroblasts and epithelial cells may sometimes be sufficient to confer cellular immortality (Newbold., 2005, Stampfer and Yaswen., 2002). Therefore, de-repression of hTERT and telomerase re-activation are thought to be critical events in human carcinogenesis and is the predominant mechanism by which cancer cells maintain their proliferative capacity. Previously, our group has shown that introduction of a normal, intact copy of human chromosome 3 into the 21NT primary breast cancer cell line by microcell-mediated monochromosome transfer (MMCT), is associated with strong telomerase repression and induction of cell growth arrest within the majority of hybrid clones (Cuthbert et al., 1999). Structural mapping of chromosome 3 within telomerase-positive revertent clones revealed two regions of deletion: 3p21.3-p22 and 3p12-p21.1, thought to harbour the putative telomerase repressor sequence(s). Subsequent studies showed that the chromosome 3p-encoded telomerase repressor sequence(s) mediates its function by means of transcriptional silencing of hTERT, in part, through chromatin remodelling of two sites within intron 2 of the hTERT gene (Ducrest et al., 2001, Szutorisz et al., 2003). Attempts to achieve positional cloning of hTERT repressor sequences on chromosome 3p identified two interesting candidates; the histone methyltransferase SETD2 and an adjacent long non-coding RNA (lncRNA) sequence known as FLJ/KIF9-AS1 (Dr. T. Roberts, unpublished data). Through MMCT-mediated introduction of intact chromosomes 3 and 17 into the 21NT cell line, I have demonstrated that at least two as yet unidentified telomerase repressor sequences (one located on each of these two normal chromosomes) may function to repress telomerase activity within the same breast cancer cell line, which suggests that multiple, independent telomerase regulatory pathways may be inactivated within the same cancer type. Furthermore, by examining the consequences of forced SETD2 and FLJ expression within the 21NT cell line, together with siRNA-mediated knockdown of SETD2 within a single telomerase-repressed 21NT-chromosome 3 hybrid, I have provided evidence to show that neither of these two candidate genes may function as a regulator of hTERT transcription. Through interrogation of relevant literature, a set of four candidate 3 telomerase regulatory genes (BAP1, RASSF1A, PBRM1 and PARP-3) were selected for further investigation based on their location within the 3p21.1-p21.3 region together with their documented role in the epigenetic regulation of target gene expression. Using mammalian expression vectors containing candidate gene cDNA sequences, my colleague Dr. T. Roberts and I demonstrated that forced overexpression of BAP1 and PARP-3 within the 21NT cell line is associated with consistent, but not always sustained, repression of hTERT transcriptional activity and telomerase activity. It is therefore possible that at least two sequences may exist on chromosome 3p that function collectively to regulate hTERT expression within breast cancer cells. Finally, using an in vitro model of human mammary epithelial cell (HMEC) immortalization, involving the targeted abrogation of two pathologically relevant genes, p16 and p53 to generate a series of variant clones at different stages of immortal transformation (developed by my colleague Dr. H. Yasaei), I have shown that single copy deletions on chromosome 3p are a frequent, clonal event, specifically associated with hTERT de-repression and immortal transformation. Subsequent high-density single nucleotide polymorphism (SNP) array analysis of immortal variants carried out by Dr. H. Yasaei, identified a minimal common region of deletion localized to 3p14.2-p22. Together, these findings provide additional evidence to show that chromosome 3p may harbour critical hTERT repressor sequences, that are lost as an early event during breast carcinogenesis.

616.99

Functional and mechanistic characterization of ubiquitin fusion degradation 1 in MYC-driven leukemogenesis

Huiting, Leah

24 October 2018

Tumor cells often hijack endoplasmic reticulum (ER) mediated signaling to facilitate tumor progression by adapting to the cellular stress evoked by oncogene overexpression and adverse microenvironment. Despite the prevalence of MYC-driven cancers, how the MYC oncoprotein regulates ER stress response pathways during tumorigenesis remains incompletely understood. Here we show that MYC drives continuous upregulation of ubiquitin fusion degradation 1 (UFD1) during T-cell acute lymphoblastic leukemia (T-ALL) development. As the E2 component of an ER-associated degradation (ERAD) complex, UFD1 facilitates the elimination of misfolded/unfolded proteins from the ER. We found that genetic and pharmacological disruption of UFD1 function exacerbates ER stress and activates the unfolded protein response (UPR). Specifically, UFD1 knockdown in human T-ALL cells impairs ERAD and promotes the proapoptotic UPR through the PERK-CHOP-BCL2 axis. This effect is demonstrated by an upregulation of PERK, phospho-PERK and its downstream effector CHOP, as well as a downregulation of BCL2 and BCLxL. Indeed, CHOP inactivation or BCL2 overexpression is sufficient to rescue tumor-cell apoptosis induced by UFD1 knockdown. Allelic loss of ufd1 in zebrafish similarly induces tumor-cell apoptosis and impairs MYC-driven T-ALL progression without affecting general animal health. These studies establish the UFD1-mediated ER stress response as an important mediator of MYC-driven tumor progression and suggest strategies for targeted therapy in T-ALL, and perhaps other MYC-driven cancers. Although UFD1-specific inhibitors have yet to be developed, inhibitors that target the p97 co-factor in UFD1-mediated ERAD are readily available. Importantly, we show that treatment with CB-5083, a selective and oral bioactive inhibitor of p97, can effectively kill human MYC-overexpressing T-ALL patient cells ex vivo and inhibits tumor progression in zebrafish models of MYC-driven T-ALL. Thus, CB-5083 treatment may represent an effective targeted therapy for T-ALL, especially relapsed/refractory ones with gain-of-function NOTCH1 mutations and thus MYC-overexpression.

Pharmacology

Zebrafish

Ubiquitin fusion degradation 1

A auto-organização feminista como processo de aprendizagem coletiva: a experiência da Rede Xique-Xique / Feminist self-organization as a collective learning process: experiences from Xique-Xique Network, 2014

Castro, Mariana Pereira de

13 March 2014

Esta pesquisa apresenta um estudo de caso cujo objetivo é descrever os saberes produzidos no processo de auto-organização de grupos de mulheres da Rede Xique-Xique de Comercialização Solidária, nos municípios de Mossoró, Upanema, Governador Dix-Sept Rosado, Baraúna, Grossos, Tibau e Apodi, no estado do Rio Grande do Norte. Trata-se de uma análise sócio histórica e econômica das categorias discursivas de termos como \'mulheres\', \'trabalho, \'família\' e \'história\', assim como da capacidade de transformação social que estes saberes apresentam. A pesquisa de campo foi guiada essencialmente pelo método da observação participante, com procedimentos aplicados pelo método biográfico, mais especificamente pela história de vida. Sobre a coleta dos dados, foram realizadas 11 entrevistas individuais com as mulheres dos grupos auto-organizados; uma entrevista com a coordenadora do CF8 e uma entrevista coletiva, na qual estavam presentes mulheres participantes de seis grupos da região. Além das entrevistas, foram realizadas visitas aos grupos produtivos, participação em reuniões e seminários promovidos pela Rede Xique-Xique ou instituições parceiras. Para analisar todos os dados registrados, as entrevistas foram transcritas e categorizadas. A análise foi realizada a partir do objetivo apresentado e da referenciação das categorias supracitadas, com o auxílio do Software NVivo10. Nesse sentido, foi possível descrever e apreender que o processo de auto-organização dessas mulheres permite a construção de um ato comunicativo entre estas, que por sua vez possibilita a produção de saberes. Esse ato comunicativo torna-se emancipatório na medida em que se caracteriza como uma prática constante de autorreflexão a respeito dos efeitos da organização produtiva autogerida e contribui assim com a transformação de vida dessas mulheres. Sobre a estrutura textual do presente trabalho, a dissertação está dividida em três capítulos. O primeiro capítulo trata da descrição dos aspectos sócio históricos do estado do Rio Grande do Norte e sua relação constitutiva com a ação atual da Rede Xique-Xique. O capítulo dois descreve a estrutura de princípios ou pilares que sustentam a prática da Rede: agroecologia, economia solidária e feminismo. No capítulo três, com base nas categorias discursivas propostas, analiso as histórias de vidas das mulheres entrevistadas durante o trabalho de campo. Por fim, as considerações finais são apresentadas. / This research presents a case study which aims to describe the knowledge produced in the process of self-organizing groups of women Xique-Xique Network Marketing Partnership located in Mossoró, Upanema, Governador Dix-Sept Rosado, Baraúna, Grossos, Tibau e Apodi in the state of Rio Grande do Norte. It is a historical and socioeconomic analysis of the discursive categories of terms such as \'women\', \'work\', \'family\' and \'history\', as well as the ability to social transformation this knowledge presents. The field research was guided essentially by the method of participant observation with procedures applied by the biographical method, more specifically the history of life. On data collection, 11 individual interviews with women of self-organized groups were conducted; interview with the coordinator of the CF8 and a press conference, in which women from six groups in the region were present. Besides the interviews, visits to productive groups, participation in meetings and seminars sponsored by Xique-Xique Network or partner institutions were conducted. To analyze all the recorded data, the interviews were transcribed and using NVivo10, categorized. The analysis was based on the discursive and historical referencing of the above categories. Thus, it was possible to describe and understand that the process of self-organization of these women allows the construction of a communicative act between them, which in turn enables the production of knowledge. This communicative act becomes emancipatory in that it is characterized as a constant practice of self-reflection about the effects of self-managed productive organization and thus contributes to the transformation of these women\'s lives. On the textual structure of the present paper, it is divided into three chapters. The first chapter presents the description of the historical and social aspects of the state of Rio Grande do Norte and its constitutive relationship with the Xique-Xique Network current action. Chapter two describes the structure of principles that support the practice of the group: agroecology, economic solidarity and feminism. In chapter three, based on the discursive categories proposed, I analyze the life histories of the women interviewed during the field work. Finally, the concluding remarks are presented.

Associated labor

Auto-organização

Mulheres

Self-organization

Trabalho Associado

Women

Expression of rho kinase in cardiovascular diseases. / CUHK electronic theses & dissertations collection

January 2011

Furthermore, ACS patients with a high N-terminal pro-B-type natriuretic peptide (NT-proBNP) and a high ROCK activity on admission had a five-fold risk to experience a cardiovascular event, when compared to those with low NT-proBNP and low ROCK activity. In addition, patients with high NT-proBNP and high ROCK activity were also more likely to die or experience a cardiovascular event at two years when comparing to those with high NT-proBNP and low ROCK activity. / In both ACS and CHF study cohorts, all the clinical parameters were recorded and analyzed. / In the first part of this thesis, 176 ACS patients and 51 control subjects were studied. All The patients were enrolled between December 2007 and May 2009 and followed up till 15th March 2010 (mean: 15.4+/-7.6 months, from 0.5 month to 27.5 months). The main outcome measures were all cause mortality, readmission with ACS or congestive heart failure (CHF) at 2 years from presentation. Altogether, there were 23 deaths (13.1%),33 readmissions with ACS (18.8%) and 13 admissions with CHF (7.4%) within 2 years. / Recent studies have shown that ROCK may playa pivotal role in cardiovascular diseases such as vasospastic angina, ischemic stroke, heart failure and metabolic syndrome via its involvement in regulation of vascular tone, endothelial dysfunction, inflammation, and remodeling. Indeed, inhibition of ROCK by statins or other selective inhibitors leads to upregulation and activation of endothelial nitric oxide synthase (eNOS) and reduction of vascular inflammation and atherosclerosis. In this thesis, we hypothesized that ROCK activity is increased in a selected population of patients with acute coronary syndrome (ACS) and congestive heart failure (CHF) and that ROCK activity is able to predict long-term clinical outcomes in these two populations. / Rho/rho-kinase (ROCK) is a serine-threonine protein kinase, which is one of the first immediate downstream targets of RhoA and expressed ubiquitously. ROCK is involved in many cellular functions, such as, cell growth, migration, apoptosis via actin cytoskeleton organization, and gene expression. They regulate cell contraction through serine-threonine phosphorylation of adducin, ezrin-radixin-moesin proteins, LIM kinase, myosin light chain phosphatase, and Sodium-Hydrogen ion (Na/H) exchanger. / The main findings are: ROCK activity was increased in ST elevation myocardial infarction (STEMI), non-STEMI (NSTEMI) and unstable angina (UA) groups when comparing with disease controls and healthy controls. On multivariate analysis, heart failure symptom on presentation, LDL-C level, and number of diseased coronary vessels were independent predictors of ROCK activity in ACS patients. / The ROCK activity in CHF patients was significantly higher than that of the disease control and normal control groups. New York Heart Association (NYHA) class, low left ventricular ejection fraction (LVEF) and high creatinine were independent predictors of the baseline ROCK activity in CHF. In terms of long-term heart failure mortality, ROCK activity was not an independent predictor. However, combining ROCK activity and NT-proBNP provided an incremental value in predicting long-term heart failure mortality over NT-proBNP alone. / Thus, increased ROCK activity is likely involved in cardiovascular diseases and further studies would be helpful to elucidate the potential role of ROCK activity inhibition in cardiovascular diseases. / We also recruited a group of 178 patients with CHF. All the patients were enrolled between December 2007 and January 2009 and followed up until 1st February 2010 (mean: 14.4+/-7.2 months, from 0.5 month to 26 months) or until the occurrence of cardiac death. Forty-five patients died (25.3%) within 2 years follow up. / Dong, Ming. / Adviser: Cheuk Man Yu. / Source: Dissertation Abstracts International, Volume: 73-04, Section: B, page: . / Thesis (Ph.D.)--Chinese University of Hong Kong, 2011. / Includes bibliographical references (leaves 140-164). / Electronic reproduction. Hong Kong : Chinese University of Hong Kong, [2012] System requirements: Adobe Acrobat Reader. Available via World Wide Web. / Electronic reproduction. [Ann Arbor, MI] : ProQuest Information and Learning, [201-] System requirements: Adobe Acrobat Reader. Available via World Wide Web. / Abstract also in Chinese.

Cardiovascular system--Diseases

Protein kinases

Cardiovascular Diseases

rho-Associated Kinases

The importance and mechanism of mitochondrial damage associated molecular patterns (DAMPs) in the pathogenesis of trauma haemorrhage induced inflammation and organ injury

Aswani, A. D.

January 2016

Trauma is a leading cause of death worldwide with 5.8 million deaths occurring yearly. Almost 40% of trauma deaths are due to bleeding and occur in the first few hours after injury. Of the remaining severely injured patients up to 25% develop a dysregulated immune response leading to multiple organ failure (MOF). Despite improvements in trauma care, the morbidity and mortality of this condition remains very high. Massive traumatic injury can overwhelm endogenous homeostatic mechanisms even with prompt treatment. The underlying mechanisms driving MOF are also not fully elucidated. As a result, successful therapies for trauma-related MOF are lacking. Trauma causes tissue damage that releases a large number of endogenous damage-associated molecular patterns (DAMPs). Mitochondrial DAMPs released in trauma, such as mitochondrial DNA (mtDNA), could help to explain part of the immune response in trauma given the structural similarities between mitochondria and bacteria. MtDNA, like bacterial DNA, contains an abundance of highly stimulatory unmethylated CpG DNA motifs that signal through Toll-like receptor (TLR)-9 to produce inflammation. MtDNA has been shown to be highly damaging when injected into healthy animals causing acute organ injury to develop. Elevated circulating levels of mtDNA have been reported in trauma patients but an association with clinically meaningful outcomes has not been established in a large cohort. The first aim of this PhD thesis was to determine whether mtDNA released after trauma haemorrhage is sufficient for the development of MOF. Secondly, I then aimed to determine the extent of mtDNA release with varying degrees of tissue injury and haemorrhagic shock in a clinically relevant rodent model. My final aim was to determine whether neutralising mtDNA at a clinically relevant time point in vivo would reduce the severity of organ injury in this model.

616.8

Cancer biomarkers, and novel techniques for detection

Jamal, Tameem

02 November 2017

Technologies for early detection of tumors is critical for better therapy outcome and overall change in cancer survival. These assays must be capable of detecting tumors at early stages in order to prevent metastasis of the tumor and help reduce mortality. Biological molecules can serve as markers that can indicate the presence of cancerous cells. Current biomarkers approved by the FDA include CA 125, which is a tumor associated antigen (TAA). However, the sensitivities of these TAAs is not high enough to detect at early stages of disease. Recent technologies have found that antibodies that recognize these TAAs, also known as autoantibodies, provide more sensitive means to screen for tumors. This review aims to present recent literature data relative to the field of cancer diagnosis and treatment. However, one should note that this article covers only fraction of the broad science behind this subject.

Oncology

Autoantibodies

Biomarkers

Cancer

Immunology

Early detection

Tumor associated antigen

Galectin-3 regulation of non small cell lung cancer growth

Kouverianou, Eleni

January 2014

Galectin-3 is a β-galactoside binding lectin expressed in tumour cells and macrophages and has been associated with increased malignancy in a variety of cancers. Previous work has shown that galectin-3 is an important regulator of macrophage function, promoting an alternative (M2) phenotype which potentiates chronic inflammation and fibrosis. Tumour associated macrophages (TAMs) adopt an M2 phenotype and are thought to promote tumour growth by down regulating T cell effector function and promoting angiogenesis. This project examines the hypothesis that host galectin-3 promotes lung cancer growth and spread. In order to test this hypothesis, Lewis Lung Carcinoma tumour growth and metastasis was investigated in strain matched mice either expressing or deficient in galectin-3. The Lewis Lung Carcinoma cell line (LLC1) is a spontaneous lung carcinoma line, derived from C57BL/6 mice, which readily forms tumours when transplanted. Furthermore, LLC1 cells were stably transfected with a Luciferase expressing vector in order to assist detection of tumour growth and metastasis in vivo. An orthotopic model of LLC1 growth suggested that galectin-3-/- animals do not support lung carcinoma growth and spread. This finding was confirmed by a subcutaneous model of cancer growth, where it was found that wild type animals display a higher proportion of macrophages expressing a prototypic M2 marker around tumour sites compared to galectin-3-/- animals. M2-promoting cytokine transcripts were also reduced in galectin-3-/- mice. Additionally, tumours of wild type mice were more invasive and presented more mature blood vessels compared to galectin-3-/- mice. To specifically address the role of recruited cells on tumour growth, metastasis and the inflammation profile around tumour sites, in relation to galectin-3 expression, bone marrow cells (BMCs) were transplanted from wild type to galectin-3-/- mice and vice versa. It was shown that galectin-3 positive BMCs restore the wild type phenotype of tumour growth in galectin-3-/- mice, while galectin-3 deficient BMCs impair tumour growth in wild type animals. Furthermore, macrophage ablation experiments demonstrated incapacity for tumour establishment in the absence of macrophages. A series of experiments investigating reported inhibition of galectin-3 by modified citrus pectin (MCP) via competitive inhibition did not provide conclusive results. MCP had no effect in vivo, but was able to inhibit LLC1 cell growth in vitro. Most importantly though, results were inconclusive as to whether galectin-3 binds MCP. Some ligand displacement was seen, but direct binding of the molecules could not be shown. In general, the results obtained demonstrate a strong pro-tumoural effect of galectin-3 on growth, tissue invasion and metastasis of LLC1 tumours via an increased proportion of Ym1-expressing macrophages around tumour sites. It was shown that macrophages are key cells for tumour initiation and that BMC phenotype in relation to galectin-3 expression determines the phenotype of tumour development in subcutaneous and orthotopic LLC1 models. Therefore, galectin-3 has a strong regulatory effect on tumour phenotype and could present a key target in the management of lung carcinomas.

616.99

Apoptosis-driven activation of macrophages by starry-sky B-cell lymphoma

Willems, Jorine Joanna Lamberta Paulina

January 2015

In high-grade ‘starry-sky’ non-Hodgkin’s lymphoma (NHL), particularly Burkitt’s lymphoma (BL), large numbers of apoptotic tumour cells are engulfed by infiltrating tumour-associated macrophages (TAM). In situ studies suggest that in starry-sky TAM in a xenograft model of BL various tumour-promoting, trophic, angiogenic, tissue remodelling, and anti-inflammatory pathways are activated. Furthermore, apoptotic cells have been shown to activate expression of tumour-promoting matrix metalloproteinases in macrophages. This work investigates the hypothesis that apoptotic cells or factors released from apoptotic cells induce additional aspects of the starry-sky TAM signature, which serve to promote tumour growth. Macrophages at different stages of maturation, cultured in vitro in the presence of large numbers of apoptotic cells, were shown to differ in phenotype, giving credibility to the hypothesis. Less mature mouse bone marrow-derived macrophages (BMDM) were better at migrating towards apoptotic cells, whereas mature BMDM were better at phagocytosing them. Lactoferrin, which is released from cells undergoing apoptosis and inhibits the migration of neutrophils, was selected as a candidate mediator in the activation of macrophages by apoptotic cells. Lactoferrin was shown to bind viable human and murine monocytes and macrophages, however only high concentrations, which are unlikely to be physiologically or clinically relevant, were found to affect expression of starry-sky TAM genes or reduce classically-activated macrophage cytotoxicity. The direct effect of apoptotic cells on macrophage activation was assessed. Mature BMDM were not used for these studies as their development in vitro in a highly apoptotic environment was judged likely to bias their activation state toward that of TAM, therefore macrophages were first classically-activated with IFN-γ and LPS. This reduced the expression of many starry-sky TAM genes, including several genes associated with responses to apoptotic cells. However, classical activation did not inhibit apoptotic cell engulfment, but rather enhanced it. Co-culture with apoptotic cells, but not viable cells, increased the gene expression of Gas6, Mrc1, Cd36, Timp2, and Pparg, and the latter was dependent on direct interaction with macrophages rather than factors released from apoptotic cells. Furthermore, classically-activated macrophages were found to induce apoptosis in lymphoma cells, and although pre-co-culture of the macrophages with apoptotic cells did not reduce their ability to induce apoptosis, it enhanced tumour cell growth. Macrophage deficiency of IL-4Rα or galectin-3 did not affect classically-activated macrophage responses to apoptotic cells. However, classical activation of galectin-3 deficient macrophages appeared to restore the decreased ability of galectin-3 deficient, untreated macrophages to phagocytose apoptotic cells. Because of the unique new method of laser-capture microdissection by which starry-sky TAM signatures were established, direct comparisons with expression databases of tissue and in vitro cultured macrophages were not possible, but indirect comparisons suggest starry-sky TAM activation reflects the activation phenotype of a mixture of tissue macrophages. Furthermore, it highlighted phagocytosis as one of the most important pathways activated by starry-sky TAM. Together the results presented here suggest apoptotic lymphoma cells can shape TAM activation signatures in starry-sky NHL, even when macrophages are pre-activated to induce apoptosis in lymphoma cells. This is important when considering the consequences of anti-cancer therapies that induce apoptosis or aim to redirect phagocyte activation.

616.99

Taxonomia e sistemática de Entomolepididae Brady, 1899 (Copepoda, Siphonostomatoida) / Taxonomy and systematics of Entomolepididae Brady, 1899 (Copepoda, Siphonoitomatoida)

Soares, Roberta Canário

21 May 2018

Entomolepididae é uma família de sifonostomatóides com distribuição cosmopolita. Até o momento, é composta por 9 gêneros e 19 species, com maior diversidade no Indo-Pacífico. Entomolepididade encontra-se dividida em duas subfamílias que diferem, basicamente, pelo número de segmentos pedígeros entre o cefalotórax e o escudo terminal - Parmulodinae apresenta apenas um segmento enquanto que Entomolepinae possui dois segmentos. Assim como nas subfamílias, é comum encontrar sobreposições nas diagnoses do gênero. Apesar de ser um grupo relativamente antigo, não há na literatura dados acerca das relações entre as espécies de Entomolepididae. Assim, esta tese teve por objetivo realizar uma revisão taxonômica e um estudo filogenético da família Entomolepididae. Ao estudar os espécimes tipos de Parmulodes verrucosus, e Entomopsyllus stocki, foi possível identificar inconsistências que levaram à redescrição da primeira e a adição de notas na descrição da segunda espécie. O estudo da fauna associada à esponjas do gênero Aplysina permitiu a identificação de 4 novas espécies de Spongiopsyllus: S. atypicus, S. stocki, S. boxshalli e S. hoi. O estudo filogenético incluiu as 23 espécies de Entomolepididade, conhecidas até então, além de 3 espécies de Asterocheridae como grupos-externos, e como resultado, foi obtida apenas 1 árvore maximamente parcimoniosa. Apenas a subfamília Entomolepinae foi recuperada como grupo monofilético. Dentre os gêneros de Entomolepididae, apenas Entomopsyllus não é monofilético. Spongiopsyllus mostrou-se um clado próximo à Entomopsyllus. A evolução de Entomolepididae envolveu muitos caracteres homoplásticos, tornado difícil o reconhecimento de padrões / Entomolepididae is a cosmopolitan siphonostomatoid family. Until now, the family is composed by 9 genera and 19 species with major diversity on Indo-Pacific Ocean. Entomolepididade has two subfamilies which differs basically by the number of pedigerous segments between the cephalotorax and the terminal shield - Parmulodinae show one segment instead Entomolepinae has two segments. As in the subfamilies, is common to find overlaps in genera diagnosis. Despite its ancient characteristics, do not have in the literature data concerning the relationships among Entomolepididae species. Thus, this thesis aimed to make a taxonomic revision and a phylogenetic study of Entomolepididae. The analyze of Parmulodes verrucosus, and Entomopsyllus stocki type specimens allowed the identification of incongruences that led to the redescription of the first and to the descriptional notes of the second species. The study of associated fauna of Aplysina sponges allow the idenification of 4 new Spongiopsyllus species: S. atypicus, S. stocki, S. boxshalli and S. hoi. The phylogenetic study include all 23 known Entomolepididae species, in addition to 3 Asterocheridae species as outgroups, resulting in 1 most parsimonious tree. Only the subfamily Entomolepinae was recovered as monophyletic. Among the genera, just Entomopsyllus was non-monophyletic. Spongiopsyllus is a clade close to Entomopsyllus. The Entomolepididae evolution involved many homoplastic characters which become difficult the identification of patterns

Associated copepods

Copépodes associados

Crustacea

Crustacea

Filogenia

Phylogeny