The role of the fms-intronic regulatory element (FIRE) in macrophage development

Rojo Gutiérrez, Rocío Patricia

January 2018

Macrophages belong to the mononuclear phagocyte system and they perform fundamental roles to maintain homeostasis in the organism. Macrophage development, survival, proliferation and functionality depend upon the colony stimulating factor 1 (CSF1) and interleukin-34 (IL-34), which signal through the CSF1 receptor (CSF1R). CSF1R is a type III tyrosine kinase receptor that is present in the plasma membrane of monocytes and macrophages. Mutations in Csf1r in mice produce the loss of many tissue macrophage populations and multiple developmental abnormalities. In humans, abnormal enhancement of CSF1R expression has been correlated to adverse prognosis in a subset of carcinomas; and mutations in the human CSF1R are associated with an autosomal-dominant neurodegenerative disease. CSF1R is encoded by the c-fms proto-oncogene and its expression is partially controlled by the fms-intronic regulatory element (FIRE). The FIRE sequence is highly conserved across species and contains binding motifs for multiple transcription factors, which are relevant for haematopoiesis. Previous results from murine Csf1r transgenes showed that FIRE is essential for driving Csf1r expression, and that interactions between FIRE and multiple myeloid transcription factors contribute to maximal regulatory activity. This project aimed to study the role of FIRE in its normal chromatin context, in vivo. A FIRE knockout (FIRE-/-) mouse model was generated using the CRISPR/Cas9 technology in mouse embryonic stem cells (ESCs) and in mice. In ESCs, the deletion severely compromised the differentiation of macrophages from embryoid bodies generated in vitro. In mice, the frequency of the FIRE- /- genotype in the progeny does not follow a Mendelian distribution and about 5% of the offspring developed hydrocephalus. Unlike Csf1r -/-mice, which die before weaning, most surviving FIRE-/- mice grew normally and were fertile. The impact of the mutation on macrophage populations is selective. FIRE-/- mice are not monocyte deficient (identified as F4/80+ Csf1r+ cells in peripheral blood), although these cells have reduced levels of Csf1r mRNA and do not bind porcine CSF1 Fc fusion protein. The development of peritoneal macrophages and Iba-1+ microglia was abolished, but Adgre1+ (F4/80+) macrophage populations in liver and spleen were unaffected. Csf1r was greatly reduced in bone marrow progenitors, but about 30% of these cells were able to differentiate into macrophages in vitro, upon exposure to recombinant human CSF1 (rhCSF1). This study shows that FIRE is essential for the development of a subset of tissue-resident macrophage populations. In FIRE-/- mice, potential compensation from additional regulatory elements within Csf1r might underlie the development of unaffected tissue-resident macrophages.

Aumento da expressão do receptor Toll-like 2 em monócitos do sangue periférico de pacientes com artrite psoriásica / Increased expression of Toll-like receptor 2 in peripheral blood monocytes from patients with psoriatic arthritis

Solange Carrasco

27 May 2014

INTRODUÇÃO: Os receptores Toll-like 2 e 4 (TLR-2 e TLR-4) são capazes de ativar células imunes inatas em resposta a bactérias Gram-positivas e Gram-negativas, respectivamente. Na artrite psoriásica (APs), doença articular inflamatória crônica, fatores genéticos, ambientais e infecciosos parecem estar envolvidos. OBJETIVO: Avaliar as expressões dos receptores: TLR-2; TLR-4; CD114 e do CD116 em monócitos e neutrófilos do sangue periférico de pacientes com APs e adicionalmente a prevalência do HLA-B27. MÉTODOS: Quarenta e cinco pacientes com diagnóstico de APs conforme os critérios CASPAR e 32 indivíduos saudáveis foram estudados. Dentre os 45 pacientes, 27 apresentavam APs ativa (DAS28 > 2,6) e 18 APs inativa (DAS28 < 2,5). A leitura das expressões do TLR-2, TLR-4, CD14, CD66, CD114, CD116 e do HLA-B27 foi realizada por citometria de fluxo no FACSCalibur da marca Becton-Dickson, utilizando anticorpos monoclonais da BD Biosciences, anti-humanos produzidos em murino. Os anticorpos monoclonais (AcMo) para marcar receptores de membrana empregados foram: CD14 conjugado com PerCP-Cy5.5 para marcar população de monócitos; CD66 conjugado com PE e FITC para população de neutrófilos; CD114 para marcar receptor de fator estimulatório de colônias de granulócitos e CD116 para marcar receptor de fator estimulatório de colônia de granulócitos-macrófagos. A análise estatística utilizou o teste U de Mann-Whitney e o teste exato de Fisher. Os valores obtidos em porcentagem foram expressos como média ± intervalo interquartil, de acordo com uma distribuição não-paramétrica, avaliados pelo teste de Shapiro-Wilk. RESULTADOS: Demonstramos aumento de expressão do TLR-2 em monócitos periféricos de pacientes com APs, APs ativa e APs inativa comparados aos controles (p < 0,002; p < 0,001 e p < 0,04, respectivamente). A expressão do TLR-4 foi similar nos pacientes com APs, APs ativa e APs inativa e controles (p < 0,23; p < 0,33 e p < 0,29, respectivamente). A expressão do receptor GCSF (CD114) e do receptor GM-CSF (CD116) foi similar nos pacientes e controles nas populações de monócitos e neutrófilos (p > 0,05). O HLA-B27 foi positivo em 1/3 dos pacientes com APs e 6% dos controles. Nos pacientes HLA-B27+ comparados aos controles HLA-B27+, a porcentagem de expressão do TLR-2 nos monócitos foi significantemente maior (p < 0,004). CONCLUSÃO: O aumento da expressão do TLR-2 em monócitos de pacientes com APs reforça o papel da imunidade inata e sugere que a exposição a bactérias Gram-positivas possa ter um papel na indução da resposta inflamatória nesta doença / INTRODUCTION: Toll-Like receptors 2 and 4 (TLR-2 and TLR-4) are able of activating innate immune cells in response to Gram-positive and Gram-negative bacteria, respectively. In Psoriatic Arthritis (APs), chronic inflammatory joint disease and genetic, environmental and infectious factors seems to be involved. OBJECTIVES: Evaluate expressions of TLR-2; TLR-4; CD114 and CD116 receptors in monocytes and neutrophils from peripheral blood patients with APs and additionally the prevalence of HLA-B27. METHODS: Forty five patients diagnosed with APs according with CASPAR criteria and 32 health individuals were studied. Among the 45 patients, 27 presented active APs (DAS28 > 2,6) and 18 inactive APs (DAS28 < 2,5). The evaluation of the TRL-2, TLR-4, CD14, CD66, CD114, CD116 and HLA-B27 expressions was held by flow cytometry in FACSCalibur from Becton-Dickson, utilizing BD Biosciences\' monoclonal antibodies, anti-human produced in mice. The monoclonal antibodies (AcMo) used to mark membrane receptors were: CD14 in conjunction with PerCP-Cy 5.5 to mark population of monocytes; CD66 in conjunction with PE and FITC for population of neutrophils; CD114 to mark stimulatory factor receptor for granulocyte colonies and CD116 to mark stimulatory factor receptor for granulocyte-macrophage colony. The statistical analysis utilized Mann-Whitney\'s U test and Fisher\'s exact test. The values obtained as percentages were expressed as median ± interquartile range, consistent with a non-parametrical distribution, assessed by Shapiro-Wilk\'s test. RESULTS: Increased expression of TLR-2 in peripheral monocytes of patients with APs, active APs and inactive APs compared to controls (p < 0.002; p < 0.001 and p < 0.04, respectively). TLR-4 expression was similar in patients with APs, active APs and inactive APs and controls (p < 0.23; p < 0.33 and p < 0.29 respectively). The expression of the G-CSF (CCD114) receptor and GM-CSF (CD116) receptor were similar in patients and controls in populations of monocytes and neutrophils (p > 0.05). HLA-B27 was positive in 1/3 of the patients with APs and 6% of the controls. The percentage of expression of TLR-2 in HLA-B27 + patients compared to HLA-B27 + controls was significantly higher (p < 0.004). CONCLUSION: Increased of TLR-2 receptors expression in patients with APs monocytes reinforces the role of innate immunity and suggests that the exposure to Gram-positive bacteria may have a role in the induction of the inflammatory response in this diseases

Artrite psoriásica

HLAB27

Imunidade inata

Monócitos

Neutrófilos

Receptores Toll-like

HLAB27

Innate immunity

Monocytes

Neutrophils

Psoriatic arthritis

Toll-like receptors

Função fagocítica em leucócitos humanos silenciados ou mutados para AIRE. / Phagocytic function of human leukocytes silenced or mutated AIRE.

Carvalho, Marina Uchôa Wall Barbosa de

19 June 2013

A APECED é uma doença que apresenta autoimunidade e susceptibilidade a Candida albicans. Nosso grupo observou que a proteína AIRE participa da via da Dectina-1, importante contra a C. albicans. Neste projeto, investigamos como a ausência de AIRE influencia em eventos para a eliminação do patógeno via Dectina-1. Assim, avaliamos o burst oxidativo, expressão de moléculas do sistema NADPH oxidase e fagocitose por células de paciente com APECED e células THP-1 silenciadas para AIRE. Não houve diferença no burst oxidativo e na expressão dos componentes do sistema NADPH oxidase por estas células e as células silenciadas fagocitam menos que as células selvagens. Observamos que não há diferença na expressão flavocitocromo b558 e p40phox do paciente comparado ao controle. Em paralelo, mostramos que as células do paciente apresentaram um burst oxidativo e fagocitose diminuídos comparado ao controle. Estes resultados sugerem que há um defeito no reconhecimento via Dectina-1, gerando uma diminuição da fagocitose que pode dificultar sua eliminação. / The APECED is a syndrome with autoantibodies and Candida albicans susceptibility. Our group has noted that AIRE protein is required for dectin-1 signaling, important against C. albicans. In this project, we investigate how the absence of AIRE influences in events for elimination of pathogen via dectin-1. We evaluated reactive oxygen species production, expression of NADPH oxidase molecules and phagocytosis by APECED pacient cells or AIRE silent THP-1 cells. We didnt observe differences in oxidative burst and expression of NADPH oxidase components by these cells and silent cells phagocytize less than wild-type cells. We observed no difference in flavocytochrome b558 and p40phox expression in paciente cells and control. In parallel, we showed that pacient cells has a decrease in burst oxidative and phagocytosis compared to control. Our results suggest that there is a defect in pathogen recognition via dectin-1, resulting in decrease on phagocytosis that can hamper their elimination.

Candida albicans

Candida albicans

Cell culture

Cell immunology

Cultura de células

Immunology

Imuninade natural

Imunologia celular

Imunopatologia

Monócitos

Monocytes

Natural immunity

Síntese de proteínas do sistema complemento por células dendríticas derivadas de monócitos na presença de sobrenadante tumoral. / Synthesis of complement proteins by monocyte-derived dendritic cells developed in the presence of tumor supernatants.

Cechim, Giovana

03 February 2012

O processo de apresentação antigênica realizado pelas células dendríticas (DC) aos linfócitos T constitui o passo inicial da geração da resposta imune anti-tumoral. As neoplasias interferem nesse processo alterando funcionalmente as DCs. Entre os fatores que influenciam a função das DCs, está a proteína C3 do sistema complemento. Assim, este trabalho investigou a influência de fatores solúveis dos sobrenadantes tumorais das linhagens de glioblastoma humano A172 e U87MG sobre a síntese de C3 pelas DCs derivadas de doadores saudáveis in vitro. A fenotipagem indicou que os sobrenadantes, especialmente da linhagem U87MG, parece estar modulando a expressão das moléculas CD14, CD80, CD86, CD83, CD274 e CD11b. Já a expressão do gene C3 parece sofrer uma modulação geralmente negativa pelo sobrenadante da linhagens U87MG enquanto a linhagem A172 tende a exercer o efeito inverso. / Antigen presentation by dendritic cells (DC) to T cells is the first step to generate an antitumor immune response. Tumors interfere in this process, affecting DCs function. One of the factors that affect DCs´s function is the complement system protein C3, which is produced by these cells. In this work, we investigated the influence of tumor supernatants derived from human glioma cells lines U87MG and A172 in the production of complement protein C3 by monocyte-derived dendritic cells from healthy donors in vitro. DC phenotyping indicated that the supernatants seem to modulate the expression of CD14,CD80,CD86, CD83, CD274 and CD11b. The expression of C3 gene, was negatively modulated by U87MG supernatant while the A172 supernatant seemed to exert the reverse effect.

Células dendríticas

Dendritic cells

Immunoproteins

Imunoproteínas

Monócitos

Monocytes

Neoplasias do sistema nervoso

Neoplasms of the nervous system

Sistema complemento

System complement

Cd40-mediated Signaling of Interleukin-1(beta) Synthesis and Rescue from Apoptosis in Monocytes: Modulation by Il-4 and Il-10

Poe, Jonathan C.

01 December 1997

To date, the cellular mechanisms involved in the progression of diseases characterized by chronic inflammation, such as rheumatoid arthritis (RA), remain largely unknown. However, cell-to-cell contact interactions between CD4+ helper T (Th) cells and monocytes have been implicated in the induction and maintenance of pro-inflammatory cytokine synthesis that is characteristic to the pathogenesis of RA. One such cytokine produced during monocyte-Th cell contact is interleukin (IL)-1 β, a mediator directly involved in the characteristic tissue destruction that occurs in the synovia of individuals with RA. Previous studies in our laboratories have shown that ligation of CD40 on monocytes with CD40 ligand (CD40L) present on activated Th cells induces monocyte IL-1β synthesis and rescues monocytes from apoptosis. These findings suggest a role for CD40 signaling of monocyte activation in the exacerbation and maintenance of chronic inflammatory responses. This dissertation represents efforts to elucidate components of the CD40 signaling pathway critical to monocyte activation and how CD40-mediated signaling events are modulated by the anti-inflammatory cytokines IL-4 and IL-10. Using either monocytes isolated from human peripheral blood or a monocytic cell line (THP-1), cellular kinases and transcription factors activated upon CD40 ligation were examined by western blot analyses and electrophoretic mobility shift assays (EMSA), respectively. CD40-dependent interleukin-1β synthesis in monocytes was abrogated by inhibitors of protein tyrosine kinase (PTK) activity but not by inhibitors of protein kinase C (PKC). The extracellular signal-regulated kinases 1 and 2 (Erk1/Erk2) mitogen-activated protein kinases (MAPK's) were specifically activated upon CD40 ligation, and specific inhibition of Erk1/Erk2 activation diminished IL-10 production in a dose-dependent manner. Both IL-4 and IL-10 reduced Erk1/Erk2 activation and synergized in this effect. Finally, STAT3, a member of the family of transcription factors involved in cytokine signaling, was highly phosphorylated in monocytes treated with IL-10 or with IL-10 and IL-4 in combination but not with IL-4 alone. Together these results suggest that in monocytes (1) CD40-mediated IL-1β synthesis and NF-κB activation require PTK activity, (2) CD40-mediated IL-1β production is critically dependent upon Erk1/Erk2 activity, (3) both IL-4 and IL-10 target the Erk1/Erk2 signaling cascade in the downregulation of IL-1β synthesis, (4) IL-4 and IL-10 have divergent effects on the CD40 signaling pathway in that these cytokines are synergistic with respect to their ability to inhibit CD40-mediated Erk1/Erk2 activation and IL-1β synthesis, and differ in their ability to block CD40-mediated rescue from apoptosis, and (5) STAT3 activation may be directly involved in the downregulatory effects of IL-10 on CD40 signaling. (Abstract shortened by UMI.)

Apoptosis

CD40-mediated

Health and environmental sciences

Immunology

Interleukin-1 beta

Interleukin-4

Interleukin-10

Monocytes

Signaling

Immunology and Infectious Disease

Eosinophil Cationic Protein : Expression Levels and Polymorphisms

Byström, Jonas

January 2002

<p>The eosinophil cationic protein (ECP) is usually associated with the eosinophil granulocyte. In this thesis the presence and production of this protein has been studied in two other cells. The circulating monocyte was found to contain ECP mRNA and small amounts of ECP, one thousand times less than that found in the eosinophil. The production decreased by differentiation of the myelomonoblastic cell line U937 into a macrophage phenotype. Submucosal lung macrophages did not stain for ECP and alveolar macrophages did not contain ECP mRNA. The circulating neutrophil contains ECP at a level hundred fold less than the eosinophil. We found that the protein is located to the primary granules of the neutrophil but could detect no ECP mRNA in the cell. It was shown in vitro that the protein was taken up by the cell and partly transported to the primary granules. The uptake did not seem to be receptor mediated. Upon stimulation of the neutrophils, ECP previously taken up, was re-secreted. </p><p>The ECP protein is heterogeneous both to molecular characteristics and to function. To evaluate if a genetic component is involved, the ECP gene was analysed in 70 individuals. Three single nucleotide polymorphisms (SNP´s) were found, denoted 277(C>T), 434(G>C) and 562(G>C). The two first were located to the mature peptide-coding region and would change the amino acids, arg45cys and arg97thr. The prevalence of the most common SNP, 434, was evaluated in two eosinophil-related diseases, allergy/asthma and Hodgkin Lymphoma (HL). Forty-three HL patients were evaluated and it was found that the 434GG was significantly more prevalent in patients having nodular sclerosis (NS) as compared to other histologies (p=0.03). Erythrocyte sedimentation rate was also related to the 434GG genotype (p=0.009). In 209 medical students 434GG was more common (p=0.002) in those who indicated allergy. The genotype was unrelated to the production of IgE antibodies to allergens. In analysis of 76 subjects with asthma it was found that the 434GG genotype was significantly more common among allergic asthmatics (p=0.04). Asthma and HL-NS are characterized by fibrosis and eosinophils and ECP has been suggested in fibrosis development. </p>

Medical sciences

Eosinophils

Neutrophils

Monocytes

Macrophages

mRNA

eosinophil cationic protein

DNA

polymorphism

Hodgkin Lymphoma

asthma

allergy

MEDICIN OCH VÅRD

MEDICINE

MEDICIN

Eosinophil Cationic Protein : Expression Levels and Polymorphisms

Byström, Jonas

January 2002

The eosinophil cationic protein (ECP) is usually associated with the eosinophil granulocyte. In this thesis the presence and production of this protein has been studied in two other cells. The circulating monocyte was found to contain ECP mRNA and small amounts of ECP, one thousand times less than that found in the eosinophil. The production decreased by differentiation of the myelomonoblastic cell line U937 into a macrophage phenotype. Submucosal lung macrophages did not stain for ECP and alveolar macrophages did not contain ECP mRNA. The circulating neutrophil contains ECP at a level hundred fold less than the eosinophil. We found that the protein is located to the primary granules of the neutrophil but could detect no ECP mRNA in the cell. It was shown in vitro that the protein was taken up by the cell and partly transported to the primary granules. The uptake did not seem to be receptor mediated. Upon stimulation of the neutrophils, ECP previously taken up, was re-secreted. The ECP protein is heterogeneous both to molecular characteristics and to function. To evaluate if a genetic component is involved, the ECP gene was analysed in 70 individuals. Three single nucleotide polymorphisms (SNP´s) were found, denoted 277(C&gt;T), 434(G&gt;C) and 562(G&gt;C). The two first were located to the mature peptide-coding region and would change the amino acids, arg45cys and arg97thr. The prevalence of the most common SNP, 434, was evaluated in two eosinophil-related diseases, allergy/asthma and Hodgkin Lymphoma (HL). Forty-three HL patients were evaluated and it was found that the 434GG was significantly more prevalent in patients having nodular sclerosis (NS) as compared to other histologies (p=0.03). Erythrocyte sedimentation rate was also related to the 434GG genotype (p=0.009). In 209 medical students 434GG was more common (p=0.002) in those who indicated allergy. The genotype was unrelated to the production of IgE antibodies to allergens. In analysis of 76 subjects with asthma it was found that the 434GG genotype was significantly more common among allergic asthmatics (p=0.04). Asthma and HL-NS are characterized by fibrosis and eosinophils and ECP has been suggested in fibrosis development.

Medical sciences

Eosinophils

Neutrophils

Monocytes

Macrophages

mRNA

eosinophil cationic protein

DNA

polymorphism

Hodgkin Lymphoma

asthma

allergy

MEDICIN OCH VÅRD

MEDICINE

MEDICIN

Regulation of tissue factor expression in myeloid and monocytic leukaemia cells

Tenno, Taavo

January 2001

Tissue factor (TF) is a transmembrane glycoprotein that initiates the blood coagulation cascade and is also involved in cell migration, tumour metastasis and angiogenesis. Pathologic expression of tissue factor by monocytes contributes to several thrombotic complications like acute coronary artery disease and disseminated intravascular coagulation. The aim of this thesis was to investigate the clinically important pathologic expression of TF in myelo-monocytic leukaemia cells and reveal the cellular signals leading to the suppression of TF expression. The studies in this thesis indicate that TF is a marker of immature myelo-monocytic cells. Markedly higher levels of TF were expressed in immature myelo-monocytic cell lines compared to mature monocyte-like cells. Induction of terminal differentiation in immature cells resulted in down-regulation of TF expression, irrespective of the specific phenotypes induced by retinoic acid (RA) or vitamin D3 in monoblastic U-937 cells. TF suppression was also found independent of differentiation pathways, i.e. monocytic or granulocytic. The nuclear receptor activation requirements for transcriptional suppression of TF by retinoic acid (RA) were shown to differ between acute promyelocytic leukaemia (APL) NB4 and U-937 cells. In NB4 cells the binding of the agonist to the RA receptor (RAR)α alone is needed for down-regulation of TF, whereas ligand binding to both RARαand retinoic X receptor was necessary for efficient suppression of TF expression in U-937 cells. To analyse the transcriptional regulation of TF, stable NB4 and U-937 clones expressing the luciferase gene under the control of various 5' flanking regions of the TF gene were selected. Different promoter regions were found to control the basal TF transcriptional activity. Analysis of protein binding to the 140 bp promoter region, responsible for basal TF activity in NB4 cells, revealed binding of RFX-1. RA suppressed the promoter activity in NB4, but not in U-937 cells. The ectopic expression of the APL fusion proteins PML/RARα or PLZF/RARα in U-937 reporter clones were shown to confer sensitivity to RA-induced suppression of TF promoter activity. These results provide a more detailed picture of TF regulation in leukaemic and haematopoietic cells and may have a bearing on new clinical treatment strategies in APL and other leukaemias.

Medical sciences

tissue factor

blood coagulation

monocytes

cell differentiation

retinoic acid

vitamin D3

acute promyelocytic leukaemia

MEDICIN OCH VÅRD

MEDICINE

MEDICIN

Immune maturation in early childhood and the influence of herpesvirus infections

Sohlberg, Ebba

January 2013

The quality of immune responses develops from birth into adulthood and in the context of the host microbial environment. The aim of this work was to study immune maturation during childhood, and how this process can be affected by the common herpesviruses; Epstein-Barr virus (EBV) and cytomegalovirus (CMV). In paper I we studied monocytes, an important cell type for immunity in the newborn. We showed that the neonatal monocyte subsets exist in similar frequencies as adult subsets, and have a potent capacity for pro-inflammatory cytokine production. In paper II, III and IV we studied the effects of EBV and CMV infections on immune cell function in children. In paper II we found that monocyte-induced NK-cell production of IFN-γ, and plasma IFN-γ levels, were decreased in 2-year old EBV- and/or CMV-seropositive children and mostly so in co-infected children. In paper III we found that in 5-year old children, EBV and CMV co-infection was associated with the highest levels of differentiated NKG2C+ NK cells. CMV+ children had higher plasma IFN-γ and IL-15 levels and higher NK-cell cytotoxic capacity. In vitro PBMC systems showed elevated frequencies of NKG2C+ NK cells in the presence of EBV-infected cells. In paper IV we showed that a child’s age and subsequent capacity for anti-viral cytokine production affects in vitro EBV infection in terms of B-cell proliferation and B-cell acquisition of memory phenotype. PBMC from CMV+ children had lower EBV-induced accumulation of switched memory B cells, which was connected to high prevalence of CD57+CD8+ T cells and IFN-γ production. Taken together, this thesis work shows that monocyte subsets at birth can give potent functional responses and that latency with EBV and CMV has a significant effect on the differentiation process and functional capacity of anti-viral effector cells during childhood. This in turn could affect responses to related or unrelated infections or even to non-invasive antigens such as allergens. / <p>At the time of the doctoral defense, the following papers were unpublished and had a status as follows: Paper 3: Manuscript. Paper 4: Manuscript.</p>

Immune differentiation

monocytes

NK cells

B cells

T cells

Epstein-Barr virus; EBV

cytomegalovirus; CMV

IFN-γ

Effect Of Glycodelin A On Cells Of The Immune System Insights Into GdA-Induced Signaling In Monocytes, B And NK Cells

Alok, Anshula

01 1900

Glycodelin is a 162 amino acid dimeric, glycosylated, secretory protein of the lipocalin superfamily. Its classification as a lipocalin(carriers of small hydrophobic molecules) is based mainly on the presence of lipocalin signature motifs in its primary sequence and no ligand for this protein has been identified till date. Glycodelin has 40-55% sequence identity with β-lactoglobulin which is the second type member of the lipocalin superfamily (the first being retinol binding protein (RBP). Glycodelin is primarily a primate specific protein (though there have been isolated reports of mRNA in mice and rats) with many isoforms secreted by various tissues, predominantly of the reproductive tract. These isoforms, being the product of the same gene, are identical in primary sequence and differ only in their glycosylation due to differences in tissue origin; hence they may be better addressed as glycoforms of glycodelin. The main glycoforms of glycodelin reported till now are GdA, GdS, GdM, GdF and GdC. Each glycoform of the protein has a varied function, dictated or modulated largely by the complex glycans on its surface. GdA, the most well studied glycoform of glycodelin, is secreted by the endometrium under progesterone control and accumulates in the amniotic fluid (from where it is isolated.). GdA has been subclassifed as an immunocalin (immuno-modulatory lipocalins) due to the many immuno-modulatory functions pertaining to tissue differentiation, implantation and angiogenesis and most sifnificantly, modulation of immune responses at ehe feto-maternal interface. The fetus expresses paternal allo-antigens on its surface and would be regarded as foreign or non-self by the maternal immune system. Yet the fetus is not rejected, and is in fact protected from attack by the maternal immune system by a variety of tolerogenic mechanisms. GdA is the most abundant secretary glycoprotein of the primate uterine compartment during implantation and early pregnancy. It has been shown to have inhibitory effect on innate as well as adaptive and humoral immune responses. It inhibits the proliferation of T and B cells, Nk cytoxocity and suppresses monocyte chemotaxis. It also skews the cytokine profile from Th1 to Th2 and inhibits IL1 and IL2 secretion from mitogenically stimulated lymphocyte and mononuclear cell cultures. In our laboratory, we have demonstrated earlier that the inhibitory effect of GdA on T cell proliferation is due to apoptosis being induced. The apoptotic signaling induced by GdA was found to be caspase dependent and follows the intrinsic mitochondrial stress induced pathway of apoptosis. Having determined the effect of glycodelin A on T cells, we wanted to look at its effect on other cells playing a role in immune responses. We decided to look at its effect, if any, on the innate immune system. Chapter 1 of the thesis describes our studies on the effect of GdA on monocytes. We have looked at the effect of GdA on primary monocytes isolated from blood of healthy human volunteers and found that GdA induces apoptosis of primary monocytes and this appears to be mediated through a caspase independent pathway. The mitochondrial membrane potential of primary monocytes was lost upon GdA treatment therefore the mitochondria seem to be involved in the apoptotic cascade. As the yield of monocytes from peripheral blood is very low, further studies on the effect of GdA on monocytes were carried out using a human monocytic cell line, THP1, as a model system. We have demonstrated the GdA is able to inhibit the proliferation of these cells and also induce apoptosis in them. We also found that this signaling is partially caspase-dependent and involvement of other caspase independent pathways is possible. Further, we have shown that there is no effect of GdA on the phagocytic ability of these cells after differentiation into the macrophage lineage. However, when added before differentiation, glycodelin is able to inhibit the phagocytic ability of THP1 cells. We also found that THP1 cells were relatively resistant to GdA-induced apoptosis post differentiation into macrophages. We have also looked at the effect of GdA on B cells using primary B cells as well as a B cell line U266B1 as our model system. GdA was shown to inhibit the proliferation of primary B cells as well as of the cell line. The protein was not able to induce apoptosis in the primary cells (both activated as well as unactivated cells) as well as in the cell line. Treatment of the cells with MAP kinase inhibitors also did not render them susceptible to GdA induced apoptosis(as has been seen in the case of U937 cells). U266B1 cells remained relatively resistant to GdA-induced apoptosis even when treated for long periods. They did not undergo significant necrosis uponGdA treatment even though the proliferation of these cells was inhibited by the protein. We were surprised to find that there was loss of mitochondrial membrane potential of the cells upon GdA treatment even when there was no cell death. The reason for this is not clear. The inhibition of proliferation of B cells by GdA does not involve caspases and the signalilng induced by GdA in these cells seems to be different to that induced in T cells atleast downstream of the mitochondria as the cells cannot proliferate in presence of GdA but seem immune to further damage or apoptosis. These studies have been described in chapter 2 of the thesis. The third and final chapter of the thesis deals with our investigation into the effect of GdA on Nk cells. GdA, in an earlier report, has been shown to inhibit the activity of circulatory NK cells. However, the mechanism of this action has not been delineated. We made attempts to determine the effect of GdA on NK cells using a human NK cell line YT Indy as our model system, as isolation and culture of primary Nk cells in good numbers is difficult. Preliminary studies revealed that GdA triggered apoptosis in these cells. However, the process was found to be caspase independent. Another surprising finding was that GdA did not bring about significant loss of mitochondrial membrane potential of these cells, implying that the involvement of mitochondria in the apoptotic signaling in these cells may be at the later stages, as amplifiers rather than initiators, as has been seen in the case of T cells and monocytes.

Glycodelin A (GdA)

Amino Acids

Immunity

Signal Transduction

Cell Immunity

Macrophages

Monocytes

NK Cells

B Cells

Monocytic Cells

Biochemistry