Monocyte activation drives preservation of membrane thiols by promoting release of oxidised membrane moieties via extracellular vesicles.

The redox state of cellular exofacial molecules is reflected by the amount of available thiols. Furthermore, surface thiols can be considered as indicators of immune cell activation. One group of thiol containing proteins, peroxiredoxins, in particular, have been associated with inflammation. In this study, we assessed surface thiols of the U937 and Thp1 monocyte cell lines and primary monocytes in vitro upon inflammatory stimulation by irreversibly labelling the cells with a fluorescent derivative of maleimide. We also investigated exofacial thiols on circulating blood mononuclear cells in patients with rheumatoid arthritis and healthy controls. When analysing extracellular vesicles, we combined thiol labelling with the use of antibodies to specific CD markers to exclude extracellular vesicle mimicking signals from thiol containing protein aggregates. Furthermore, differential detergent lysis was applied to confirm the vesicular nature of the detected extracellular events in blood plasma. We found an increase in exofacial thiols on monocytes upon in vitro stimulation by LPS or TNF, both in primary monocytes and monocytic cell lines (p<0.0005). At the same time, newly released extracellular vesicles showed a decrease in their exofacial thiols compared with those from unstimulated cells (p<0.05). We also found a significant elevation of surface thiols on circulating monocytes in rheumatoid arthritis patients (p<0.05) and newly released extracellular vesicles of isolated CD14+ cells from rheumatoid arthritis patients had decreased thiol levels compared with healthy subjects (p<0.01). Exofacial peroxiredoxin 1 was demonstrated on the surface of primary and cultured monocytes, and the number of peroxiredoxin 1 positive extracellular vesicles was increased in rheumatoid arthritis blood plasma (p<0.05). Furthermore, an overoxidised form of peroxiredoxin was detected in extracellular vesicle-enriched preparations from blood plasma. Our data show that cell surface thiols play a protective role and reflect oxidative stress resistance state in activated immune cells. Furthermore, they support a role of extracellular vesicles in the redox regulation of human monocytes, possibly representing an antioxidant mechanism.

Is there a possibility of intrasystem regulation by hormones produced by the immune cells? Experiments with extremely low concentrations of histamine.

The effect of histamine in 10 -9 , 10 -12 , 10 -15 and 10 -18 molar concentrations was studied on the beta-endorphin and triiodothyronine (T 3 ) content of peritoneal immune cells (lymphocytes, monocyte-granulocyte group and mast cells), using immunocytochemical flow cytometric method. The lower concentrations (10 -15 and 10 -18 M) were effective, where endorphin content was significantly lowered and T 3 content was significantly elevated. The results call attention to the extreme sensitivity of histamine receptors in this hormonal index and to the specific response by hormone production to histamine, in the immune cells. The new data support the earlier hypothesis, that there is a hormonal network inside the immune system.

Effects of different fixatives on demonstrating epinephrine and ACTH hormones in Tetrahymena.

The unicellular Tetrahymena produces, contains, and secretes many hormones characteristic of higher animals. We tested three fixatives, formaldehyde, N-(3-dimethylaminopropyl)-N'-ethylcarbodiimide hydrochloride (EDAC), and glutaraldehyde for suitability for immunocytochemical demonstration of epinephrine and adrenocorticotropic harmone (ACTH) in Tetrahymena. Using flow cytometric immunocytochemistry, staining of ACTH was highest after EDAC fixation and that of epinephrine after glutaraldehyde fixation. Using laser scanning confocal microscopy, formaldehyde fixation prevented staining. Glutaraldehyde fixation produced high autofluorescence, which obscured specific staining. After EDAC fixation, ACTH was localized in the ciliary row; however, demonstration of epinephrine was not improved. Our results show that there is no "fixative for any hormone." Different fixatives are needed to demonstrate different hormones in Tetrahymena.

Influence of perinatal stress on the hormone content in immune cells of adult rats: dominance of ACTH.

Rat dams were stressed by total deprivation of food and water for 48 h just before or directly after delivery and the offspring were studied when adult. The immune cells' hormone content (ACTH, histamine, serotonin, and T(3)) was measured by immunocytochemical flow cytometry. The elevation of ACTH content in males was convincing in each cell type (lymphocytes, monocytes and granulocytes, and mast cells). The change in histamine and T(3) content was inconsistent, while serotonin level did not change at all. As ACTH is the key hormone in the General Adaptation Syndrome, it seems likely that the perinatal stress primarily caused elevation in ACTH level and it was provoking the life-long hormonal imprinting. There was a difference between the reaction of males and females (with males' advance), which points to the gender dependence of the phenomenon. It is important that the effect of stress on the offspring was similar in case of direct (prenatal, in the mother) and indirect (postnatal, transmitted by milk) stress treatment, which calls attention to the danger of stress during this latter period.

Gender dependence in the hormone content of the immune cells.

Adrenocorticotropic hormone (ACTH), endorphin, progesterone and triiodothyronine (T3) content of immune cells (lymphocytes, monocyte-macrophage-granulocyte group and mast cells of peritoneal fluid, blood lymphocytes and thymic lymphocytes) was studied by immunocytochemistry and flow cytometric analysis and compared in young (four weeks old) and sexually matured (two and a half months old) male and female rats. In most of cases, cells of female animals contained significantly more hormones, however, in the young group ACTH content of blood lymphocytes was double in males than that of females. In adults only T3 content of mast cells was higher in males. Progesterone was present only in the cells of the young group. The results show that i) hormone content in the immune cells is gender-dependent with the adventage of females and ii) this difference is not influenced by the sexual maturation.

Thyrotropic hormone (TSH) regulation of triiodothyronine (T(3)) concentration in immune cells.

OBJECTIVE: Cells of the immune system (peritoneal lymphocytes, monocytes, granulocytes and mast cells as well as thymocytes) contain triiodothyronine (T(3)). The aim of the present experiments was to study whether thyrotropic hormone (TSH) regulates or not the T(3) concentration of these cells. METHODS: Peritoneal fluid and thymus cells of adult rats were studied by immunocytochemistry, combined with flow cytometry for triiodothyronine content with or without in-vitro TSH treatment. In addition, adult female CD1 mice were treated in vivo with 10 or 40 mU TSH and after 1 hour peritoneal immune cells were studied using the above mentioned method. RESULTS: Both in vitro (in rat) and in vivo (in mice) TSH treatments significantly elevated the T(3) content in each cell type. In vitro TSH 0.1 mU/ml cell suspension was enough to provoke about 50 % increase in T(3) production. CONCLUSION: T(3) concentration in immune cells seems to be regulated by TSH, similarly to the T(3) in the thyroid. Considering the large number of immune cells in an organism, TSH regulation of their T(3) content could have an important physiological and pathological role, both in and beyond the immune system.

Highlights of a new type of intercellular communication: microvesicle-based information transfer.

Microvesicles (MVs) are membrane-covered cell fragments released by most cell types during apoptosis or activation. They are increasingly considered to play a pivotal role in information transfer between cells. Their presence and role have been proven in several physiological and pathological processes, such as immune modulation in inflammation and pregnancy, or blood coagulation and cancer. MVs represent a newly recognized system of intercellular communications. They not only may serve as prognostic markers in different diseases, but could also hold the potential to be new therapeutic targets or drug delivery systems. The present overview aims to highlight some aspects of this new means of cellular communication: "microvesicular communication".

Presence and distribution of biogenic amines (histamine, serotonin and epinephrine) in immunophenotyped human immune cells.

OBJECTIVE: In animal experiments many hormones were demonstrated in immune cells. However, very few data are at our disposal in the case of human immune cells. In an earlier experiment, ACTH, endorphin and T(3) were studied and found in different subsets of human immune cells. Here, three biogenic amines (histamine, serotonin and epinephrine) were studied. METHODS: Biogenic amine content of immunophenotyped human lymphocytes from 15 blood donors were investigated by multicolor flow cytometry using anti-biogenic amine antibodies. Monocytes and granulocytes separated by size and granularity were also studied. RESULTS: Each biogenic amine could be detected in each subset of leukocytes, except epinephrine and serotonin in granulocytes. Activated T cells contained a higher amount of the amines, and CD19+B cells a higher amount of histamine, related to the whole lymphocyte population and to other subsets. Monocytes contained more histamine and epinephrine than lymphocytes and granulocytes contained twice as much histamine as monocytes and three times as much as lymphocytes. CONCLUSION: Human lymphocytes contain the three biogenic amine, similar to rat. However, while each amine was present in monocytes, in granulocytes serotonin and epinephrine were not demonstrated. The results call attention to the possible extrapolation of animal data to human lymphocytes and monocytes, but in the case of granulocytes, caution is needed. Taking into consideration earlier results, activated T cells appear to have an important role in the loss or production of hormones inside the immune system.

T lymphocytes are targets for platelet- and trophoblast-derived microvesicles during pregnancy.

Microvesicles (MVs) can derive from several cell types and their membranes contain cell surface elements. Their role is increasingly recognized in cell-to-cell communication, as they act as both paracrine and remote messengers, occurring in circulating form as well as in plasma. Successful pregnancy requires a series of interactions between the maternal immune system and the implanted fetus, such that the semi-allograft will not be rejected. These interactions occur at the materno-placental interface and/or at a systemic level. In the present study we identified for the first time the in vivo plasma pattern of the MVs of third-trimester, healthy pregnant women, their cellular origin, and their target cells using flow cytometry and confocal laser microscopy. We searched for the cellular target molecules of thrombocyte-derived MVs with the help of neutralizing antibodies. We examined the in vitro effects of MVs on STAT3 phosphorylation of primary lymphocytes and Jurkat cells. We found that both placental trophoblast-derived and maternal thrombocyte-derived MVs bind to circulating peripheral T lymphocytes, but not to B lymphocytes or NK cells. We were able to show that the P-selectin (CD62P)-PSGL-1 (CD162) interaction is one mechanism binding platelet-derived MVs to T cells. We were also able to demonstrate that MV-lymphocyte interactions induce STAT3 phosphorylation in T cells. Our findings indicate that both thrombocyte- and trophoblast-derived MVs may play an important role in the immunomodulation of pregnancy. We suggest that the transfer of different signals via MVs represents a novel form of communication between the placenta and the maternal immune system, and that MVs contribute to the establishment of stable immune tolerance to the semi-allograft fetus.

Effects of sodium fluoride (NaF) on the cilia and microtubular system of Tetrahymena.

The effect of the nucleophilic reagent NaF on the microtubular system of Tetrahymena was studied by using scanning electron microscopy (SEM), confocal microscopy, and flow cytometry. Treatments with 40 mM NaF significantly reduced the amount of alpha-tubulin while 80 mM treatment did not alter its quantity. One possible explanation for this alpha-tubulin overexpression is that the higher amount of alpha-tubulin enables this organism to carry out the appropriate function of the cytoskeleton under this undesirable influence of higher amounts of 80 nM NaF. However, the amount of acetylated tubulin increased in a dose-dependent manner. The cilia became fragile under the effect of 80 mM NaF. Confocal microscopy revealed that after 40 mM NaF treatment transversal microtubule bands (TMs) and longitudinal microtubule bands (LMs) as well as basal bodies (BBs) were extremely strong decorated with anti-acetylated tubulin antibody and TM-localization abnormalities were visible. In the 80 mM NaF-treated cells, the deep fiber of oral apparatus was very strongly labeled, while the TMs and LMs were less decorated with anti-acetylated tubulin antibody, and LM deformities were visible. It is supposed that post-translational tubulin modifications (e.g., acetylation) defend the microtubules against the NaF-induced injury. NaF is able to influence the activity of several enzymes and G-proteins, therefore is capable to alter the structure, metabolism, and the dynamics of microtubular system. The possible connection of signaling and cytoskeletal system in Tetrahymena is discussed.

Histidine decarboxylase (HDC) knock out mouse immune cells have altered expression of ACTH, triiodothyronine and endorphin.

OBJECTIVE: In earlier experiments the immune cells of HDC gene knock-out (HDC-KO) mice contained significantly more serotonin, than those of the wild ones. It was supposed that serotonin, being another biogenic amine, replenishes histamine deficiency. Now we extended our earlier studies to the investigation of the levels of other hormones (adrenocorticotropic hormone [ACTH], beta-endorphin, triiodothyronine [T(3)]) in this knockout model. METHODS: Peritoneal lavage fluid samples and thymuses were gained from HDC-KO and wild type mice. Their cells were prepared for flow cytometry and confocal microscopy by using specific antibodies to the three hormones (1st antibodies) and 2nd antibody to the 1st antibodies. The results of wild type and KO animals were compared. RESULTS: In KO animals the ACTH content in mast cells was significantly reduced and in thymic lymphocytes halved. Endorphin content was reduced both in peritoneal and thymic lymphocytes as well as in mast cells. T(3) content showed a two and a half-fold elevation in the monocyte-macrophage-granulocyte group. The confocal microscopic analysis showed the characteristic picture of HDC-KO mast cells, their cytoplasm being almost free of granules. CONCLUSION: Knock-out of the histidine decarboxylase gene causes a general endocrine imbalance in the hormones which are related to histamine, inside the immune cells. Levels of some hormones are elevated, others decreased.

Serotonin content is elevated in the immune cells of histidine decarboxylase gene knock-out (HDCKO) mice. Focus on mast cells.

OBJECTIVE: Biogenic amines, histamine and serotonin are present in the granules and nucleus of mast cells. We wanted to study the presence, amount and localization of serotonin in mast cells and other cells of the immune system, under conditions of histamine deficiency caused by knock out of histamine decarboxylase gene (HDCKO). METHODS: Wild type and histamine deficient HDCKO mice were studied for serotonin content of the immune cells (lymphocytes as well as the monocyte-granulocyte-mast cell group) using flow cytometry and confocal microscopy. Groups of mice were kept either on complete rodent chow or on a histamine-free diet for a month before the experiments. RESULTS: The amount of serotonin was significantly higher in the KO animals, irrespective of the diet. Confocal microscopy demonstrated the presence of serotonin in the nucleus of mast cells in the wild type animals, while it was not present in the KO mice. Furthermore, in the cytoplasm (granules) of KO mast cells a bright fluorescence was observed in contrast to the pale fluorescence of wild animals. CONCLUSION: It seems likely that serotonin replaces the deficient histamine in the heparin-biogenic amine complex in the mast cell granules.

Transgenerational effect of neonatal vitamin A or D treatment (hormonal imprinting) on the hormone content of rat immune cells.

Male offspring of neonatally vitamin A or D treated (hormonally imprinted) rat dams were studied for hormone (adrenocorticotrophine [ACTH], beta-endorphin, histamine, triiodothyronine [T3]) content in immune cells, by using immunocytochemical methods for flow cytometry and confocal microscopy. ACTH and T3 were almost doubled in the lymphocytes of vitamin A treated mothers' offspring, while histamine decreased to a one-third in the histamine content of vitamin D treated mothers' offspring. Part of the animals received vitamin treatment again 24 hours before measurement, however, only endorphin content elevated moderately. In the offspring of untreated dams administered with vitamin D 24 hours before measurement, each cell type studied (lymphocyte, monocyte-granulocyte group, mast cell) had a one-third lower T3 content, which shows that vitamin D treatment can influence hormone content of immune cells. The experiments call attention to the transgenerational effect of perinatal treatment with lipid-soluble, intracellular receptor-bound vitamins.

Histamine regulates placental cytokine expression--in vivo study on HDC knockout mice.

Successful pregnancy is closely related to polarization toward a Th2 type immune response. As histamine is known to initiate Th2 dominance during inflammatory processes we raised the question whether histamine has any effect on the actual tuning of proper cytokine balance for the proceeding of the gestation. Histamine has multiple functions in the process of pregnancy, different studies have shown the direct and/or indirect presence of histamine action in the placenta as well. As HDC is the unique histamine producing enzyme in eukaryotes, we used HDC (so endogenous histamine)-deficient knockout mice as reliable model for studying histamine-related processes in vivo. We examined the placental histamine content and the expression of histamine receptors and Th1/Th2/Th3 type cytokines in the placenta. We showed for the first time the influence of histamine on the orchestrated regulation of placental cytokine expression. In the absence of local histamine the cytokine balance is shifted toward Th1 types at the maternal-placental interface, threatening pregnancy. We also measured splenic lymphocyte subpopulation ratios in pregnant and non-pregnant mice and found that in pregnancy they are independent of the presence of histamine.

In vitro effect of hormones on the hormone content of rat peritoneal and thymic cells. Is there an endocrine network inside the immune system?

OBJECTIVE: The cells of the immune system contain hormones and receptors for hormones. However, the hormonal interactions between the cells are not elucidated. In the present experiments the effect of four hormones (insulin, oxytocin, gonadotropin and epidermal growth factor) on the production of three hormones (ACTH, endorphin, triiodothyronine) in immune cells was studied. METHODS: Hormone content of peritoneal immune cells (lymphocytes, monocyte-macrophage-granulocyte group [mo-gran], mast cells) as well as thymic cells of 100 g male rats, in vitro-treated or not treated with hormones mentioned above, were determined by flow cytometry, using specific antibodies. RESULTS: All of the hormones studied influenced the hormone concentration of immune cells significantly. The width of the effects was different in the following order: oxytocin > gonadotropin > EGF > insulin. In the case of oxytocin, 8/12 of the hormone/cell group were affected, while treatment with insulin affected only 4/12. The reaction measured by the hormone production was also different: ACTH production was reduced everywhere except in the insulin-thymocyte setup. Endorphin and T3 production was always elevated. Cells of the mo-gran group were more sensitive to hormonal regulation than peritoneal lymphocytes. CONCLUSION: The results mean that immune cells can be regulated by the neuroendocrine system and could also be able to play a role in endocrine regulation. In addition, taking into account the localization of these cells in the immune organs, there is the possibility of autocrine and paracrine regulation inside the immune system. Considering that the hormones, contained or sensed by the cells of the immune system are influencing each other, the concept of a hormonal network within the immune system can be proposed.

A soluble factor(s) released by MRC-5 cells early and late after human cytomegalovirus infection induces maturation of monocyte-derived dendritic cells.

A human cytomegalovirus (HCMV) strain passaged 10 times on MRC-5 human fibroblast cells failed to express immediate early (IE) antigens in immature dendritic cells (iDCs) after infection. However, both the early and the late HCMV conditioning medium, harvested from MRC-5 cells at 24 h or 7-9 days after infection, respectively, induced a higher ratio of DCs expressing maturation markers (CD40, CD83, CD86 and HLA-DR) on the surface of the cells. HCMV conditioning medium, ultracentrifuged to remove virus particles, exhibited a similarly enhanced expression of DC maturation markers. DCs treated with HCMV conditioning medium harvested late after infection increased the percentages of autologous CD4+ and CD8+ cells of seropositive donors to produce IFN-gamma and stimulated HCMV-specific lymphoproliferative responses. The early HCMC conditioning medium was also able to induce the functional maturation of DCs, as demonstrated by supplementing this medium with a Chlamydia pneumoniae antigen.

EDAC fixation increases the demonstrability of biogenic amines in the unicellular Tetrahymena: a flow cytometric and confocal microscopic comparative analysis.

Earlier experiments demonstrated the presence of hormones of the higher ranked animals in Tetrahymena. In the present experiments two fixatives, paraformaldehyde, which is commonly used and a carbodiimide, EDAC that was recommended by Panula et al. for the immunocytochemistry of histamine, are compared in Tetrahymena for the demonstration of histamine and serotonin by using flow cytometry and confocal microscopy. Both hormone levels were significantly higher after EDAC fixation; serotonin almost doubled and histamine was more than fivefold. The confocal microscopic pictures were clearer and the hormones' localization was easier. The results support earlier observations on the presence of these hormones in Tetrahymena and points to the advantage of EDAC fixation for demonstrating these hormones immunocytochemically.

Prolonged effect of stress (water and food deprivation) at weaning or in adult age on the triiodothyronine and histamine content of immune cells.

We used two days of total water and food deprivation as stress for female rats at weaning (three weeks old) and at adult age (two and a half months old). Triiodothyronine (T3) and histamine content of immune cells (lymphocytes, mast cells and monocyte-macrophage-granulocyte group in peritoneal fluid; lymphocytes, granulocytes and monocytes in blood; and lymphocytes in thymus) were studied three weeks after stress application using specific antibodies for flow cytometry and confocal microscopy. The stress at weaning increased T3 content of thymus lymphocytes. In case of adult T3, there was a cell type independent significant effect of stress, decreasing values in peritoneal fluid and slightly increasing effect in the blood. Histamine content of granulocytes was also significantly elevated. The experiments demonstrate that not only fetal or neonatal stress has long-lasting consequences, but also stress events in later periods of life in cells (organs) that are continuously differentiating. We will go on to discuss the importance of T3 and histamine in connection with stress and immunity.

Increased interferon-gamma- and interleukin-4-synthesizing subsets of circulating T lymphocytes in pregnant asthmatics.

BACKGROUND: Pregnancy frequently interferes with the course of bronchial asthma, and asthmatic pregnant women experience less successful pregnancies. T lymphocytes synthesizing IL-4 or IFN-gamma are important in allergic mechanisms of the airways as well as in materno-fetal immunity. OBJECTIVE: We hypothesized that pregnancy (a T helper-2 polarized state) of asthmatics will enhance the number of circulating T2 lymphocytes, but decrease the subset-producing IFN-gamma (T1 lymphocytes) and thereby cause a culminating T2 dominance with possible clinical consequences. METHODS: IL-4- or IFN-gamma-producing T lymphocytes were determined by flow cytometry in healthy (n=8) and asthmatic (n=13) non-pregnant women and healthy (n=18) and asthmatic (n=48) pregnant women of similar chronological and gestational (2nd-3rd trimester) age and asthma severity (Global Initiative for Asthma II-III). RESULTS: In the blood of non-pregnant women--healthy or asthmatic--the numbers of IL-4- and IFN-gamma+ T cells were very low (<10/microL blood). In contrast, in asthmatic pregnant women, the cell counts were 182+/-27 and 39+/-6 for IFN-gamma+ and IL-4+ T cells/microL blood, respectively (both P<0.05 vs. respective control values of non-pregnant asthmatics). Within the asthmatic pregnant group, significant negative correlations were revealed between the numbers of IFN-gamma+ or IL-4+ T cells and maternal peak expiratory flow as well as birth weight of newborns (both P<0.05). CONCLUSION: These data show a previously unknown immunological interference between asthma and pregnancy. The culminating proliferation of IFN-gamma+ and IL-4+ T lymphocytes may potentially impair maternal airway symptoms as well as fetal development.

Three-generation investigation on serotonin content in rat immune cells long after beta-endorphin exposure in late pregnancy.

Female rats were treated with beta-endorphin on the 19th day of pregnancy. Serotonin content of immune cells (peritoneal lymphocytes, monocyte-macrophage-granulocyte group (mo-gran), mast cells, blood lymphocytes, granulocytes and monocytes, thymus lymphocytes) were studied in the mothers (P-generation four weeks after delivery), in the male offspring (F1) generation (at seven weeks), in the female offspring (four weeks after their own delivery) and in their offspring (F2 generation, at seven weeks). P-mother cells' serotonin content was not influenced by endorphin treatment, while F1 generation's mo-gran and blood lymphocyte serotonin content was reduced (in contrast, histamine content of mo-gran increased). Four weeks after delivery, an increase in serotonin content was observed in the F1 generation in the peritoneal lymphocytes and mast cells as well as in blood lymphocytes. In contrast, serotonin content was reduced in blood granulocytes and monocytes. In the F2 (grandson) generation, a reduction in mast cell serotonin content and sensitization of blood and thymic lymphocytes to repeated endorphin treatment was provoked. The significant changes were more expressed in the F2 generation compared to F1, also appearing earlier. The results unequivocally suggest that the increase in endorphin levels during late pregnancy can cause permanent changes in the F1 and F2 generations, which means that the imprinting effect can be transgenerationally transmitted.