Showing total 42 results

1. Immune responses in newly developed short-lived SAM mice II. SELECTIVELY IMPAIRED T-HELPER CELL ACTIVITY IN <em>IN VITRO</em> ANTIBODY RESPONSE.

Author

Hosokawa, T., Hosono, M., Hanada, K., Aoike, A., Kawai, K., and Takeda, T.

Subjects

T cells, LEUCOCYTES, IMMUNOGLOBULINS, ANTIGENS, LYMPHOCYTES, CELL culture

Abstract

New short-lived strains of mice (SAM-P), which have been developed by Takeda et al. (1981), show a defective antibody response to T dependent (TD) antigen in vitro, as demonstrated in the accompanying paper (see page 419). In the present study, we investigated the cellular site of the defect, using a cell culture system. In this paper, it is demonstrated that T-helper (Th) cell activity for the antibody response to TD antigen is impaired, while other cellular immune responses, e.g. mixed leucocyte reaction, cytotoxic T-lymphocyte response, and delayed-type hypersensitivity reaction, are normal. These results suggest that the defect in T-helper subset is limited in helper function for the antibody response, and that the helper function for the cell-mediated immune responses is intact. These two functions of the T-helper subset are apparently regulated in a different manner. The SAM-P strains of mice may thus serve as an appropriate model for studying functional heterogeneity in T-helper/inducer cell subsets. [ABSTRACT FROM AUTHOR]

Published

1987

2. Fact and Speculation on the Function of Immune Response Genes in Antigen Presentation.

Author

Werdelin, O.

Subjects

IMMUNE response, ANTIGENS, LYMPHOCYTES, IMMUNOLOGY, T cells, LEUCOCYTES

Abstract

Immune responsiveness of guinea pigs to dinitrophenyl-poly-L-lysine and to the lysine rich random co-polymer of L-glutamic acid and L-lysine are both controlled by a single gene, the `poly-L-Iysine gene'. This paper reviews recent experiments which demonstrate that these two antigens specifically compete with one another for being presented to T cells by the same antigen-presenting cells. This finding is interpreted to mean that antigens to which responsiveness is controlled by the same single gene compete for the Ir gene product of antigen-presenting cells. The review discusses if the products of the immune response genes-presumably the Ia antigens-may constitute a third specific antigen recognition system. It further speculates if this idea may help to provide insight into the phenomenon of histocompatibility-restriction and into the nature of the mixed leucocyte reaction. [ABSTRACT FROM AUTHOR]

Published

1981

3. HLA-D/DR Restriction of Macrophage-dependent Antigen Activation of Immune T Lymphocytes: Cross-reacting Allogeneic HLA-D/DR May Partly Substitute for Self HLA-D/DR.

Author

Bergholtz, B. O., Thoresen, A. B., and Thorsby, E.

Subjects

MACROPHAGES, ANTIGENS, IMMUNITY, T cells, LYMPHOCYTES, LEUCOCYTES

Abstract

Optimal proliferative response of T lymphocytes to purified protein derivative of tuberculin (PPD) in vitro requires that antigen be presented by autologous macrophages or allogeneic macrophages sharing HLA-D/DR determinants with the T cell donor. In some cases, however, T cells may respond to a limited extent to PPD in association with macrophages expressing different HLA-D/DR determinants. In this paper experiments are presented where various combinations of T cells and HLA-D/DR disparate macrophages were stimulated with PPD. We often found a strong PPD-specific response in HLA-D/DR-incompatible combinations in which the macrophages carried HLA-DR antigens known from serological studies to be cross-reactive with those of the T cell donor than in combinations in which this was not the case. Thus, the cross-reactions detected by serology may sometimes be reflected on a functional level in T lymphocyte/macrophages cooperation. [ABSTRACT FROM AUTHOR]

Published

1980

4. Preparation and characterization of murine monoclonal antibodies to swine lymphocyte antigens.

Author

Lie, W.-R., Rothschild, M. F., and Warner, C. M.

Subjects

MONOCLONAL antibodies, HYBRIDOMAS, T cells, ANTIGENS, LEUCOCYTES, ENZYME-linked immunosorbent assay

Abstract

A panel of monoclonal antibodies (mAb) was developed by the fusion of Sp2/0 myeloma cells and spleen cells from mice immunized with peripheral blood mononuclear cells (PMNC) or T cells from NIH swine leucocyte antigen (SLA) inbred miniature swine. Twenty stable hybridoma clones were isolated that secreted mAb that reacted with swine PMNC, as determined by an enzyme-linked immunosorbent assay (ELISA). The binding profile to swine PMNC and the ability to fix complement of these mAb were investigated by flow cytometric analyses. The molecular weights of the antigens recognized by six of the mAb were determined by immunoprecipitation of 125I-surface-labelled PMNC, followed by SDS-PAGE under reducing conditions. The most interesting mAb, 7-34-1 (IgG2a), precipitated a putative MUC class I molecule composed of a 50,000 MW heavy chain and a 12,000 MW light chain (β2m). This is the third SLA class I-reactive monoclonal antibody to be described for swine. Properties of the mAb described in this paper, mAb 7-34-1, are different from the two other SLA class I-specific mAb that have been described elsewhere in the literature (mAb 74-11-10 and mAb FF85). M onoclonal antibody 7-34-1 recognized class I antigens of SLA haplotypes a, c and din an equivalent manner. This mAb should be especially useful as a general anti- SLA class I reagent for experiments on NIH miniature swine. [ABSTRACT FROM AUTHOR]

Published

1988

5. IgG2 deficiency in a healthy blood donor. Concomitant lack of IgG2, IgA and IgE immunoglobulins and specific anti--carbohydrate antibodies.

Author

Hammarström, L. and Smith, C. I. E.

Subjects

IMMUNOGLOBULINS, ANTIGENS, BLOOD plasma, LEUCOCYTES, T cells, ORGANIC compounds

Abstract

Lack of serum IgG2, IgA and IgE was found in a healthy male adult blood donor. No secretory IgA could be demonstrated. In vitro activation of lymphocytes did not induce IgA secreting cells although no class specific suppressor cells could be found. Normal or slightly subnormal titres to a variety of bacterial and viral antigens were demonstrated whereas anti-carbohydrate antibodies (anti-teichoic acid, anti-dextran and anti-pneumococcal polysaccharide) were virtually absent. Isoagglutinins and heteroagglutinins were present in somewhat lower concentrations than normal. [ABSTRACT FROM AUTHOR]

Published

1983

6. Epimedium Polysaccharide Ameliorates Benzene-Induced Aplastic Anemia in Mice.

Author

He, Jin, Han, Ru, Yu, Gongchang, Lavin, Martin F., Jia, Qiang, Cui, Ping, and Peng, Cheng

Subjects

ERYTHROCYTES, SUBCUTANEOUS injections, REACTIVE oxygen species, ANIMAL experimentation, ANTIGENS, APLASTIC anemia, APOPTOSIS, BONE marrow, DOSE-effect relationship in pharmacology, HEMOGLOBINS, HERBAL medicine, IMMUNITY, LEUCOCYTES, CHINESE medicine, MICE, ONCOGENES, ORAL drug administration, POLYSACCHARIDES, STEM cells, T cells, OXIDATIVE stress, BENZENE derivatives, CASPASES, PLATELET count, DRUG administration, DRUG dosage

Abstract

Benzene (BZ) is an important occupational and environmental pollutant. Exposure to BZ may cause aplastic anemia which is characterized as bone marrow hematopoietic failure. In order to reduce the harmful effects of this pollutant, it is necessary to identify additional preventative measures. In this study, we investigated the protective effects of epimedium polysaccharide (EPS), a natural compound with antioxidant and immune-enhancing potency, on aplastic anemia induced by benzene exposure in mice. Male CD-1 mice were randomly divided into five groups including control, BZ (880 mg/kg), LE (EPS low-dose, 20 mg/kg + BZ), ME (EPS middle-dose, 100 mg/kg + BZ), and HE (EPS high-dose, 200 mg/kg + BZ) groups. Animals were exposed to BZ by subcutaneous injection in the presence or absence of EPS via oral administration. All mice were treated 3 times a week for 8 consecutive weeks to develop a mouse model of benzene-induced aplastic anemia (BIAA). Results showed that BZ induced a significant decrease in both white and red blood cells, platelet counts, and hemoglobin level compared with that in the control group (p < 0.01). Treatment of EPS led to a protective effect against these changes particularly in the highest-dose group (HE, p < 0.01). EPS also recovered the decreased number of nucleated cells in peripheral blood cell smears and femur biopsies by BZ exposure. The increased level of reactive oxygen species (ROS) in bone marrow mononuclear cells (BMMNCs) in mice from the BZ group was significantly lower (p < 0.01) in the mice from the highest concentration of EPS (HE) group when compared with that from the control group. In addition, BZ exposure led to a significant increase in the apoptosis rate in BMMNCs which was prevented by EPS in a dose-dependent manner (p < 0.01). The antiapoptosis effect of EPS was through reversing apoptotic proteins such as BAX, Caspase-9 and Caspase-3, and Bcl-2. Finally, EPS treatment partially restored the levels of T cells and the different subtypes except CD80+ and CD86+ compared with the BZ group (HE, p < 0.05). These results suggest that EPS has protective effects against BIAA via antioxidative stress, immune modulation, and antiapoptosis mechanisms. [ABSTRACT FROM AUTHOR]

Published

2020

7. A mechanism of T cell dependent selection of antigen engaged Germinal Center B cells.

Author

Krishna, Vinod and Bachman, Kurtis E.

Subjects

B cells, GERMINAL centers, T cells, IMMUNOGLOBULIN producing cells, LEUCOCYTES, SPERM competition

Abstract

A model of B cell affinity selection is proposed, and an explanation of peripheral tolerance mechanisms through antibody repertoire editing is presented. We show that affinity discrimination between B cells is driven by a competition between obtaining T cell help and removal of B cells from the light zone, either through apoptosis or by a return to the dark zone of germinal centers. We demonstrate that this mechanism also allows for the negative selection of self reactive B cells and maintenance of B cell tolerance during the Germinal Center reaction. Finally, we demonstrate that clonal expansion upon return to the Germinal Center dark zone amplifies differences in the antigen affinity of B cells that survive the light zone. [ABSTRACT FROM AUTHOR]

Published

2018

8. Dietary supplementation with blueberry partially restores T-cell-mediated function in high-fat-diet-induced obese mice.

Author

Lewis, Erin D., Ren, Zhihong, DeFuria, Jason, Obin, Martin S., Meydani, Simin N., and Wu, Dayong

Subjects

BLUEBERRIES, CELL proliferation, ADIPOSE tissues, ANIMAL experimentation, ANTIGENS, CELLULAR immunity, CYTOKINES, DIETARY supplements, FAT content of food, IMMUNITY, INTERFERONS, LEUCOCYTES, LOW-fat diet, MICE, OBESITY, PLANT proteins, T cells, TUMOR necrosis factors, LIPOPOLYSACCHARIDES

Abstract

Blueberry, rich in antioxidant and anti-inflammatory phytochemicals, has been demonstrated to lower inflammatory status in adipose induced by high-fat diet (HFD) and obesity. The effect of blueberry on systemic immune functions has not been examined. C57BL/6 mice were randomised to one of three diets – low-fat diet (LFD), HFD and HFD plus 4 % (w/w) blueberry (HFD+B) – for 8 or 12 weeks. Ex vivo T-cell mitogens (concanavalin A (Con A); phytohaemagglutinin), T-cell antibody (anti-CD3; anti-CD3/CD28)-stimulated T-cell proliferation and cytokine production were assessed. After 8 weeks, both HFD groups weighed more (>4 g) than the LFD group; after 12 weeks, HFD+B-fed mice weighed more (>6 g) and had 41 % more adipose tissue than HFD-fed mice (P<0·05). After 12 weeks, T-cell proliferation was less in both HFD groups, compared with the LFD group. HFD-associated decrements in T-cell proliferation were partially (10–50 %) prevented by blueberry supplementation. At 12 weeks, splenocytes from HFD mice, but not from HFD+B mice, produced 51 % less IL-4 (CD3/CD28) and 57 % less interferon-γ (Con A) compared with splenocytes from LFD mice (P<0·05). In response to lipopolysaccharide challenge, splenocytes from both HFD groups produced 24–30 % less IL-6 and 27–33 % less TNF-α compared with splenocytes from LFD mice (P<0·05), indicating impaired acute innate immune response. By demonstrating deleterious impacts of HFD feeding on T-cell proliferation and splenocyte immune responses, our results provide insights into how HFD/obesity can disrupt systemic immune function. The protective effects of blueberry suggest that dietary blueberry can buttress T-cell and systemic immune function against HFD-obesity-associated insults. [ABSTRACT FROM AUTHOR]

Published

2018

9. Dendritic Cells Utilize the Evolutionarily Conserved WASH and Retromer Complexes to Promote MHCII Recycling and Helper T Cell Priming.

Author

Graham, Daniel B., Osborne, Douglas G., Piotrowski, Joshua T., Gomez, Timothy S., Gmyrek, Grzegorz B., Akilesh, Holly M., Dani, Adish, Billadeau, Daniel D., and Swat, Wojciech

Subjects

DENDRITIC cells, BIOLOGICAL evolution, T helper cells, PRIMING (Psychology), ANTIGENS, LEUCOCYTES

Abstract

Immature dendritic cells (DCs) maintain a highly dynamic pool of recycling MHCII that promotes sampling of environmental antigens for presentation to T helper cells. However, the molecular basis of MHCII recycling and the cellular machinery that orchestrates MHCII trafficking are incompletely understood. Using a mouse model we show that WASH, an actin regulatory protein that facilitates retromer function, is essential for MHCII recycling and efficient priming of T helper cells. We further demonstrate that WASH deficiency results in impaired MHCII surface levels, recycling, and an accumulation of polyubiquitinated MHCII complexes, which are subsequently slated for premature lysosomal degradation. Consequently, conditional deletion of the Wash gene in DCs impairs priming of both conventional and autoimmune T helper cells in vivo and attenuates disease progression in a model of experimental autoimmune encephalitis (EAE). Thus, we identify a novel mechanism in which DCs employ the evolutionarily conserved WASH and retromer complex for MHCII recycling in order to regulate T helper cell priming. [ABSTRACT FROM AUTHOR]

Published

2014

10. Molecular characterization of swine leukocyte antigen gene diversity in purebred Pietrain pigs.

Author

Essler, Sabine E., Ertl, Werner, Deutsch, Julia, Ruetgen, Barbara C., Groiss, Sandra, Stadler, Maria, Wysoudil, Bhuma, Gerner, Wilhelm, Ho, Chak‐Sum, and Saalmueller, Armin

Subjects

MAJOR histocompatibility complex, LEUCOCYTES, T cells, ANTIGENS, GLYCOPROTEINS, IMMUNE response, SWINE

Abstract

The porcine major histocompatibility complex ( MHC) harbors the highly polymorphic swine leukocyte antigen ( SLA) class I and II gene clusters encoding glycoproteins that present antigenic peptides to T cells in the adaptive immune response. In Austria, the majority of commercial pigs are F2 descendants of F1 Large White/ Landrace hybrids paired with Pietrain boars. Therefore, the repertoire of SLA alleles and haplotypes present in Pietrain pigs has an important influence on that of their descendants. In this study, we characterized the SLA class I ( SLA-1, SLA-2, SLA-3) and class II ( SLA-DRB1, SLA-DQB1, SLA-DQA) genes of 27 purebred Pietrain pigs using a combination of the high-resolution sequence-based typing ( SBT) method and a low-resolution ( Lr) PCR-based method using allele-group, sequence-specific primers ( PCR- SSP). A total of 15 class I and 13 class II haplotypes were identified in the studied cohort. The most common SLA class I haplotype Lr-43.0 ( SLA-1*11 XX- SLA-3*04 XX- SLA-2*04 XX) was identified in 11 animals with a frequency of 20%. For SLA class II, the most prevalent haplotype, Lr-0.14 [ SLA-DRB1*0901- SLA-DQB1*0801- SLA-DQA*03 XX], was found in 14 animals with a frequency of 26%. Two class II haplotypes, tentatively designated as Lr- Pie-0.1 [ SLA-DRB1*01 XX/be01/ha04- SLA-DQB1*05 XX- SLA - DQA*blank] and Lr- Pie-0.2 [ SLA-DRB1*06 XX- SLA-DQB1*03 XX- SLA-DQA*03 XX], appeared to be novel and have never been reported so far in other pig populations. We showed that SLA genotyping using PCR- SSP-based assays represents a rapid and cost-effective way to study SLA diversity in outbred commercial pigs and may facilitate the development of more effective vaccines or identification of disease-resistant pigs in the context of SLA antigens to improve overall swine health. [ABSTRACT FROM AUTHOR]

Published

2013

11. The humanized anti-HLA-DR moAb, IMMU-114, depletes APCs and reduces alloreactive T cells: implications for preventing GVHD.

Author

Chen, X, Chang, C-H, Stein, R, and Goldenberg, D M

Subjects

GRAFT versus host disease prevention, ANTIGEN presenting cells, ANTIGENS, LEUCOCYTES, DENDRITIC cells, T cells, MONOCLONAL antibodies

Abstract

In contrast to the conventional immunosuppressive agents and nonselective T-cell-depleting antibodies, selective depletion of donor alloreactive T cells and/or host APCs, particularly DCs, represents a novel approach that can effectively control GVHD with less or no impairment of T-cell-mediated antiviral and GVL immunity. Here we report that IMMU-114, a humanized anti-human leukocyte antigen-DR (HLA-DR) moAb, efficiently depleted human PBMCs of all APCs, including B cells, monocytes, myeloid DC type-1 (mDC1), mDC2 and plasmacytoid DCs (pDCs). Early and late apoptosis of mDC1, mDC2 and pDCs, and late apoptosis of all APC subsets, were increased by IMMU-114 treatment. Although IMMU-114 had little, if any, effect on the survival and apoptosis of non-B lymphocytes (>80% of which are T cells and ∼1-2% of T cells express HLA-DR), it selectively inhibited the proliferation of purified HLA-DR+ T cells rather than HLA-DR− T cells. As a consequence, IMMU-114 treatment resulted in suppressed T-cell proliferation and reduced CD25+ alloreactive T cells in allogeneic MLRs. Given the critical roles of APCs and alloreactive T cells in the pathogenesis of GVHD, these results suggest that IMMU-114 may have therapeutic potential against GVHD. [ABSTRACT FROM AUTHOR]

Published

2012

12. Lack of Functional Selectin Ligand Interactions Compromises Long Term Tumor Protection by CD8+ T Cells.

Author

Stark, Felicity C., Gurnani, Komal, Sad, Subash, and Krishnan, Lakshmi

Subjects

T cells, LEUCOCYTES, ANTIGENS, LYMPH nodes, FUCOSYLTRANSFERASES, DENDRITIC cells

Abstract

Central memory CD8+ T cells expressing the adhesion molecule CD62L (L-selectin) are potent mediators of anti-cancer immunity due to their ability to proliferate extensively upon antigen re-stimulation. The interaction of selectin with its ligands mediates leukocyte rolling along high endothelial venules. Mice deficient in α(1,3) Fucosyltransferase IV and VII (FtDKO) lack functional L, P and E selectin ligands. Thus, we addressed whether the lack of selectin ligand interactions alters tumor protection by CD8+ T cells in FtDKO mice. Listeria monocytogenes-OVA (LM-OVA) infection evoked potent OVAspecific CD8+ T cells that proliferated and contracted at similar kinetics and phenotype in FtDKO and wild-type mice. Additionally, OVA-specific CD8+ T cells in both mouse strains exhibited similar phenotypic differentiation, in vivo cytolytic activity and IFN-γ expression. However, FtDKO mice succumbed to B16-OVA tumors significantly earlier than wild-type mice. In contrast, FtDKO mice evoked strong recall memory CD8+ T cell responses and protection to systemic LM-OVA rechallenge. The diminished tumor protection in FtDKO mice was not related to defective antigen presentation by dendritic cells or reduced proliferation of antigen-specific CD8+ T cells. However, WT or FtDKO OVA-specific CD8+ T cells showed significantly reduced ability to traffic to lymph nodes upon adoptive transfer into naïve FtDKO recipients. Furthermore, FtDKO OVA-specific CD8+ T cells displayed poor ability to infiltrate tumors growing in WT mice. These results reveal that selectin ligand expression on host endothelium as well CD8+ T cells may be important for their efficient and continued extravasation into peripheral tumors. [ABSTRACT FROM AUTHOR]

Published

2012

13. The Shc Family Protein Adaptor, Rai, Negatively Regulates T Cell Antigen Receptor Signaling by Inhibiting ZAP-70 Recruitment and Activation.

Author

Ferro, Micol, Savino, Maria Teresa, Ortensi, Barbara, Finetti, Francesca, Genovese, Luca, Masi, Giulia, Ulivieri, Cristina, Benati, Daniela, Pelicci, Giuliana, and Baldari, Cosima T.

Subjects

T cells, CELL growth, CYTOSOL, LEUCOCYTES, ANTIGENS

Abstract

Rai/ShcC is a member of the Shc family of protein adaptors expressed with the highest abundance in the central nervous system, where it exerts a protective function by coupling neurotrophic receptors to the PI3K/Akt survival pathway. Rai is also expressed, albeit at lower levels, in other cell types, including T and B lymphocytes. We have previously reported that in these cells Rai attenuates antigen receptor signaling, thereby impairing not only cell proliferation but also, opposite to neurons, cell survival. Here we have addressed the mechanism underlying the inhibitory activity of Rai on TCR signaling. We show that Rai interferes with the TCR signaling cascade one of the earliest steps -recruitment of the initiating kinase ZAP-70 to the phosphorylated subunit of the TCR/CD3 complex, which results in a generalized dampening of the downstream signaling events. The inhibitory activity of Rai is associated to its inducible recruitment to phosphorylated CD3, which occurs in the physiological signaling context of the immune synapse. Rai is moreover found as a pre-assembled complex with ZAP- 70 and also constitutively interacts with the regulatory p85 subunit of PI3K, similar to neuronal cells, notwithstanding the opposite biological outcome, i.e. impairment of PI-3K/Akt activation. The data highlight the ability of Rai to establish interactions with the TCR and key signaling mediators which, either directly (e.g. by inhibiting ZAP-70 recruitment to the TCR or sequestering ZAP-70/PI3K in the cytosol) or indirectly (e.g. by promoting the recruitment of effectors responsible for signal extinction) prevent full triggering of the TCR signaling cascade. [ABSTRACT FROM AUTHOR]

Published

2011

14. Lymphocyte Cell-Cycle Inhibition by HLA-G Is Mediated by Phosphatase SHP-2 and Acts on the mTOR Pathway.

Author

Ketroussi, Farah, Giuliani, Massimo, Bahri, Rajia, Azzarone, Bruno, Charpentier, Bernard, and Durrbach, Antoine

Subjects

LYMPHOCYTES, CELL cycle, PHOSPHATASES, LEUCOCYTES, ANTIGENS, T cells, IMMUNOGLOBULINS, CELL proliferation

Abstract

Human leukocyte antigen G (HLA-G) is involved in regulating T-cell responses through its interaction with inhibitory receptors belonging to the immunoglobulin-like transcript family (ILT). In this context, we investigated the pathways involved in the control of cell-cycle entry of T cells following HLA-G interaction with its inhibitory receptor. We show that HLA-G acts through its interaction with the LILRB1 receptor expressed on T lymphocytes. Both HLA-G and LILRB1 antibodies block the inhibitory effect of HLA-G and restore T-cell proliferation. The interaction of HLA-G with T lymphocytes is associated with phosphorylation of SHP-2 phosphatase, but not SHP-1. In addition, in activated T cells, their incubation with HLA-G is not associated with a decrease in the TCR or CD28 downstream pathways, but is associated with dephosphorylation of the mTOR molecule and p70S6K. In contrast, Akt, which acts upstream of mTOR, is not affected by HLA-G. The inhibition of SHP-2 by NSC-87877(5 μM), a chemical inhibitor of SHP-2, or the use of siRNA, abrogates dephosphorylation of mTOR and impairs the overexpression of p27kip in the presence of HLA-G. Together, these results indicate that HLA-G is associated with activation of phosphatase SHP-2, which inhibits the mTOR pathway and favors the inhibition of the cell-cycle entry of human-activated T cells. [ABSTRACT FROM AUTHOR]

Published

2011

15. Dynamic Imaging of the Effector Immune Response to Listeria Infection In Vivo.

Author

Waite, Janelle C., Leiner, Ingrid, Lauer, Peter, Rae, Chris S., Barbet, Gaetan, Huan Zheng, Portnoy, Daniel A., Pamer, Eric G., and Dustin, Michael L.

Subjects

IMMUNE response, LISTERIOSIS, LISTERIA monocytogenes, DENDRITIC cells, MICROSCOPY, BLOOD flow, ANTIGENS, T cells, LEUCOCYTES

Published

2011

16. Mutational Escape in HIV-1 CTL Epitopes Leads to Increased Binding to Inhibitory Myelomonocytic MHC Class I Receptors.

Author

Yue Yang, Jinghe Huang, Toth, Ildiko, Lichterfeld, Mathias, and Yu, Xu G.

Subjects

GENETIC mutation, GENETICS, T cells, LYMPHOCYTES, EPITOPES, ANTIGENS, DENDRITIC cells, MONOCYTES, LEUCOCYTES

Abstract

Escape mutations in HIV-1 cytotoxic T cell (CTL) epitopes can abrogate recognition by the TCR of HIV-1-specific CD8+ T cells, but may also change interactions with alternative MHC class I receptors. Here, we show that mutational escape in three HLA-A11-, B8- and B7- restricted immunodominant HIV-1 CTL epitopes consistently enhances binding of the respective peptide/MHC class I complex to Immunoglobulin-like transcript 4 (ILT4), an inhibitory myelomonocytic MHC class I receptor expressed on monocytes and dendritic cells. In contrast, mutational escape in an alternative immunodominant HLA-B57- restricted CTL epitope did not affect ILT4-mediated recognition by myelomonocytic cells. This suggests that in addition to abrogating recognition by HIV-1-specific CD8 T cells, mutational escape in some, but not all CTL epitopes may mediate important immunoregulatory effects by increasing binding properties to ILT4, and augmenting ILT4-mediated inhibitory effects of professional antigen-presenting cells. [ABSTRACT FROM AUTHOR]

Published

2010

17. Risk, Characteristics and Biomarkers of Cytokine Release Syndrome in Patients with Relapsed/Refractory AML or MDS Treated with CD3xCD123 Bispecific Antibody APVO436.

Author

Uckun, Fatih M., Watts, Justin, Mims, Alice S., Patel, Prapti, Wang, Eunice, Shami, Paul J., Cull, Elizabeth, Lee, Cynthia, Cogle, Christopher R., and Lin, Tara L.

Subjects

BIOMARKERS, INTERLEUKINS, MYELODYSPLASTIC syndromes, OBESITY, CYTOKINES, INTRAVENOUS therapy, STEROIDS, LEUCOCYTES, TOCILIZUMAB, DEXAMETHASONE, ACUTE myeloid leukemia, MONOCLONAL antibodies, ANTINEOPLASTIC agents, DISEASE incidence, RACE, LEUKEMIA, OSTEOBLASTS, CYTOKINE release syndrome, DISEASE relapse, RISK assessment, CANCER patients, SEX distribution, TREATMENT effectiveness, DESCRIPTIVE statistics, IMMUNOPHENOTYPING, T cells, BONE marrow, ANTIGENS, PREANESTHETIC medication, DISEASE remission, DISEASE risk factors, SYMPTOMS

Abstract

Simple Summary: Cytokine release syndrome is a potentially life-threatening complication of therapy with T-cell engaging bispecific antibodies. Here we evaluated the risk, characteristics and biomarkers of treatment-emergent cytokine release syndrome in patients with relapsed/refractory acute myeloid leukemia or myelodysplastic syndrome who received weekly intravenous infusions of the CD3xCD123 bispecific antibody APVO436. Cytokine release syndrome was encountered in 10 of 46 patients (21.7%) treated with APVO436 with a cumulative Grade 3/4 cytokine release syndrome incidence of 8.7%. Cytokine profiling in patients who developed cytokine release syndrome after APVO436 infusion indicated that the predominant cytokine in this inflammatory cytokine response was IL-6. The findings from this research provide new insights regarding the biology and effective management of cytokine release syndrome in leukemia patients treated with T-cell redirecting bispecific antibodies. We evaluate the risk, characteristics and biomarkers of treatment-emergent cytokine release syndrome (CRS) in patients with relapsed/refractory acute myeloid leukemia (AML) or myelodysplastic syndrome (MDS) who received APVO436 during the dose-escalation phase of a Phase 1B study (ClinicalTrials.gov, identifier: NCT03647800). Of four patients who developed Grade ≥ 3 CRS, two received steroid prophylaxis. The dose level, gender, race, obesity, or baseline hematologic parameters in peripheral blood did not predict the risk of CRS. Patients with a higher leukemia burden as determined by a higher total WBC, higher percentage of blasts in bone marrow, or higher percentage of blasts in peripheral blood (by hematopathology or immunophenotyping) did not have a higher incidence of CRS. There was an age difference between patients who did versus patients who did not develop CRS (72.9 ± 1.6 years (Median 73.5 years) vs. 63.3 ± 2.3 years (Median: 65.0 years), which was borderline significant (p = 0.04). Premedication with steroids did not eliminate the risk of CRS. Cytokine profiling in patients who developed CRS after APVO436 infusion indicates that the predominant cytokine in this inflammatory cytokine response was IL-6. APVO436-associated CRS was generally manageable with tocilizumab with or without dexamethasone. Notably, the development of CRS after APVO436 therapy did not appear to be associated with a response. The prolonged stabilization of disease, partial remissions and complete remissions were achieved in both patients who experienced CRS, as well as patients who did not experience CRS after APVO436 infusions. [ABSTRACT FROM AUTHOR]

Published

2021

18. An investigation to assess the potential of CD25highCD4+ T cells to regulate responses to donor alloantigens in clinically stable renal transplant recipients.

Author

Akl, Ahmed, Jones, Nicholas D., Rogers, Nichola, Bakr, Mohamed Adel, Mostafa, Amani, El Shehawy, EL Metwaly, Ghoneim, Mohamed A., and Wood, Kathryn J.

Subjects

T cells, ANTIGENS, KIDNEY diseases, KIDNEY transplantation, TRANSPLANTATION of organs, tissues, etc., LEUCOCYTES, HOMOGRAFTS

Abstract

Regulatory T cells are enriched within CD25highCD4+ leukocytes, however their role in renal transplant recipients with stable function vs. recipients with biopsy-proven chronic allograft dysfunction remains unclear. We therefore studied the number, phenotype, and function of CD25highCD4+ cells in the peripheral blood of 30 renal transplant recipients of living-related grafts, comprising 15 rejection-free recipients with stable graft function (Group A) and 15 with biopsy-proven chronic graft dysfunction (Group B). A higher absolute number of CD25highCD4+ cells were present in the peripheral blood of rejection-free recipients (Group A) vs. those recipients with chronic graft dysfunction (Group B) ( P = 0.019); but there was no significant difference with healthy volunteers ( P = 0.084). In carboxyfluorescein diacetate succinimidyl ester-mixed leukocyte culture assays, depletion of CD25highCD4+ revealed active regulation in 11 (74%) of 15 rejection-free recipient samples (Group A) in response to donor- but not third party-leukocytes, whereas no regulatory activity was observed in any samples from recipients with chronic graft dysfunction (Group B). In conclusion, these data provide evidence for the presence of an increased number of CD25highCD4+ T cells with donor-specific regulatory activity in the peripheral blood of renal transplant recipients with stable graft function compared with recipients with chronic graft dysfunction. [ABSTRACT FROM AUTHOR]

Published

2008

19. CD11c+ antigen presenting cells from the alveolar space, lung parenchyma and spleen differ in their phenotype and capabilities to activate naïve and antigen-primed T cells.

Author

Kugathasan, Kapilan, Roediger, Elizabeth K., Small, Cherrie-Lee, McCormick, Sarah, Pingchang Yang, and Zhou Xing

Subjects

DENDRITIC cells, CELLS, LEUCOCYTES, T cells, ANTIGENS

Abstract

Background: The lung is divided into two major compartments: the alveolar space and the parenchyma. The alveolar macrophages are the first line of leukocytes in the lung taking up incoming microbes or microbial antigens whereas the parenchymal dendritic cells (DCs) are believed to be the sole potent antigen presenting cells (APCs) in the lung. Both resting alveolar macrophages and parenchymal DCs express CD11c. Several important questions remain to be elucidated: 1] to which extent the alveolar space and lung parenchymal CD11c+ APCs differ in their phenotype and ability to activate naïve T cells; 2] whether they differ in their ability to activate antigen-experienced or -primed T cells; and 3] whether these lung CD11c+ APC populations differ from the splenic CD11c+ APCs which have been commonly used for understanding APC biology. Results: CD11c+ APCs from the alveolar space, lung parenchyma, and the spleen display differential co-stimulatory molecule expression and cytokine responsiveness upon stimulation. Alveolar space APCs are weak activators of naïve T cells compared to lung parenchymal and splenic CD11c+ APC populations. However, alveolar space APCs are able to potently activate the in vivo microbial antigen-primed T cells to a similar extent as lung parenchymal and splenic APCs. Conclusion: Together our findings indicate that alveolar CD11c+ APCs have a specialized T cell-activating function, capable of activating antigen-primed, but not naïve, T cells whereas lung CD11c+ APCs are capable of activating both the naïve and antigen-primed T cell populations. [ABSTRACT FROM AUTHOR]

Published

2008

20. Role of Human Leucocyte Antigen DQ in the Presentation of T Cell Epitopes in the Major Cow’s Milk Allergen αs1-Casein.

Author

Ruiter, B., Rozemuller, E. H., van Dijk, A. J., Garssen, J., Bruijnzeel-Koomen, C. A. F. M., Tilanus, M. G., Knol, E. F., and van Hoffen, E.

Subjects

FOOD allergy, HLA histocompatibility antigens, MILK, LEUCOCYTES, ANTIGENS, T cells, EPITOPES

Abstract

Background: Little is known about the association between human leucocyte antigen (HLA) and cow’s milk allergy (CMA). The aim of the present study was to determine the HLA restriction of T cell clones (TCCs) specific to αs1-casein, the most abundant milk protein, and to study possible HLA class II allele associations with CMA. Methods: αs1-Casein-specific TCCs were derived from 6 children with CMA, 9 atopic children without CMA and 5 non-atopic children. T cell epitope specificity was defined by stimulation with overlapping peptides, spanning the αs1-casein molecule. HLA restriction was determined in proliferation assays using antibodies blocking either HLA-DP, HLA-DQ or HLA-DR. HLA genotyping was performed in 32 subjects with CMA, 23 atopic and 22 non-atopic individuals. Results: Ten TCCs were restricted to HLA-DQ, 6 TCCs to HLA-DR and 4 TCCs to HLA-DP. The sequence in αs1-casein that was most immunogenic to T cells from children with CMA contained T cell epitopes restricted to DQB1*0201, DPB1*0401 and DRB1*1501. The DQB1*0501 allele frequency was lower in children with CMA than in non-atopic children, but this difference could not be confirmed in an additional group of subjects with and without CMA. Conclusions: HLA-DQ plays a substantial role in the presentation of T cell epitopes in αs1-casein. However, HLA class II allele frequencies do not show major differences between cow’s milk allergic, atopic and non-atopic subjects. T cell epitopes in the most immunogenic region are presented by various abundantly present HLA genotypes. Therefore, this sequence may be a suitable target for peptide immunotherapy. Copyright © 2007 S. Karger AG, Basel [ABSTRACT FROM AUTHOR]

Published

2007

21. The human cathepsin H gene encodes two novel minor histocompatibility antigen epitopes restricted by HLA-A*3101 and -A*3303.

Author

Torikai, H., Akatsuka, Y., Miyazaki, M., Tsujimura, A., Yatabe, Y., Kawase, T., Nakao, Y., Tsujimura, K., Motoyoshi, K., Morishima, Y., Kodera, Y., Kuzushima, K., and Takahashi, T.

Subjects

MINOR histocompatibility antigens, GRAFT versus host disease, LYMPHOCYTES, T cells, LEUCOCYTES, ANTIGENS, EPITOPES

Abstract

Minor histocompatibility antigens (mHags) play crucial roles in the induction of graft versus host disease (GVHD) and/or graft versus leukaemia (GVL) effects following human leucocyte antigen (HLA)-identical haematopoietic stem cell transplantation (HSCT). Using HLA-A*3101- and -A*3303-restricted cytotoxic T lymphocyte (CTL) clones generated from different post-HSCT recipients, we identified two novel mHag epitopes encoded by the leader sequence of cathepsin H (CTSH) isoform a. The nonameric sequence ATLPLLCAR was defined as an HLA-A*3101-restricted epitope (CTSHR/A31), while a decameric peptide featuring a one N-terminal amino acid extension, WATLPLLCAR, was presented by HLA-A*3303 (CTSHR/A33). The immunogenicity of both epitopes was totally dependent on the polymorphic C-terminal arginine residue and substitution with glycine completely abolished binding to the corresponding HLA molecules. Thus, the immunogenicity of this mHag is exerted by differential HLA binding capacity. CTSH is relatively ubiquitously expressed at protein levels, thus it may be involved in GVHD and anti-leukaemic/tumour responses. Interestingly, however, CTL clones predominantly lysed targets of haematopoietic cell origin, which could not be explained in terms of the immunoproteasome system. Although the mechanisms involved in the differential susceptibility remain to be determined, these data suggest that CTSH-encoded mHags could be targets for GVL effects. [ABSTRACT FROM AUTHOR]

Published

2006

22. The Direct Pathway of Human T-Cell Allorecognition is not Tolerized by Stimulation with Allogeneic Peripheral Blood Mononuclear Cells Irradiated with High-Dose Ultraviolet Ba.

Author

Wallgren, A. C., Alder, J., Andersson, B., Karlsson-Parra, A., and Bäcker, A. E.

Subjects

BLOOD transfusion, GRAFT versus host disease, LEUCOCYTES, LABORATORY rodents, IMMUNOLOGY, T cells, IRRADIATION, ANTIGENS

Abstract

Transfusions of high-dose (≥10,000 Joule/m2) ultraviolet-B (UVB)-irradiated allogeneic leukocytes in rodent models have been shown to induce immunologic tolerance that is mediated by allospecific regulatory CD4+ T cells. Whether these regulatory T cells recognize alloantigens through the direct or indirect pathway of allorecognition is controversial. Here, we demonstrate that the proliferative response obtained in standard primary mixed leukocyte reactions (MLRs) with human peripheral blood mononuclear cells (PBMCs) reflected a CD4+ T-cell-dependent direct pathway of allorecognition and that high-dose UVB irradiation of PBMCs totally inhibited their capacity to induce a proliferative alloresponse. Re-stimulation with γ-irradiated PBMCs from the same allogeneic donor (secondary MLR) elicited a proliferative and Th1-deviated response that was similar to the response induced in unprimed PBMCs. Finally, high-dose UVB was found to induce a rapid and massive apoptosis of irradiated PBMCs. Collectively, these data indicate that leukocytes irradiated with high-dose UVB are unable to prime for unresponsiveness or immune deviation in T cells directly recognizing allogeneic major histocompatibility complex molecules. Because it is well-established that antigens within transfused apoptotic cells are captured by resident tolerogenic spleen dendritic cells, we propose that tolerance induced by transfusions of high-dose UVB-irradiated leukocytes primarily involve T cells indirectly recognizing alloantigens. [ABSTRACT FROM AUTHOR]

Published

2006

23. Exogenous and endogenous glycolipid antigens activate NKT cells during microbial infections.

Author

Mattner, Jochen, DeBord, Kristin L., Ismail, Nahed, Goff, Randal D., Cantu, Carlos, Zhou, Dapeng, Saint-Mezard, Pierre, Wang, Vivien, Gao, Ying, Yin, Ning, Hoebe, Kasper, Schneewind, Olaf, Walker, David, Beutler, Bruce, Teyton, Luc, Savage, Paul B., and Bendelac, Albert

Subjects

GLYCOLIPIDS, ANTIGENS, KILLER cells, T cells, LEUCOCYTES, PATHOGENIC microorganisms, CELL receptors

Abstract

CD1d-restricted natural killer T (NKT) cells are innate-like lymphocytes that express a conserved T-cell receptor and contribute to host defence against various microbial pathogens. However, their target lipid antigens have remained elusive. Here we report evidence for microbial, antigen-specific activation of NKT cells against Gram-negative, lipopolysaccharide (LPS)-negative alpha-Proteobacteria such as Ehrlichia muris and Sphingomonas capsulata. We have identified glycosylceramides from the cell wall of Sphingomonas that serve as direct targets for mouse and human NKT cells, controlling both septic shock reaction and bacterial clearance in infected mice. In contrast, Gram-negative, LPS-positive Salmonella typhimurium activates NKT cells through the recognition of an endogenous lysosomal glycosphingolipid, iGb3, presented by LPS-activated dendritic cells. These findings identify two novel antigenic targets of NKT cells in antimicrobial defence, and show that glycosylceramides are an alternative to LPS for innate recognition of the Gram-negative, LPS-negative bacterial cell wall. [ABSTRACT FROM AUTHOR]

Published

2005

24. A listing of human tumor antigens recognized by T cells.

Author

Renkvist, Nicolina, Castelli, Chiara, Robbins, Paul F., and Parmiani, Giorgio

Subjects

ANTIGENS, TUMORS, LYMPHOCYTES, LEUCOCYTES, B cells, T cells, SUPPRESSOR cells, INTERLEUKIN-2

Abstract

This article presents a list of human tumor antigens recognized by T cells.

Published

2001

25. Increased expression of ICAM-1, E-selection, and VCAM-1 by cultured human endothelial cells upon exposure to haptens.

Author

Wildner, O., Lipkow, Th., and Knop, J.

Subjects

ALLERGENS, ANTIGENS, T cells, LYMPHOCYTES, LEUCOCYTES, IMMUNOFLUORESCENCE

Abstract

Contact allergens induce several accessory signals which promote the activation of antigen-specific T cells. One of these signals is the increased expression of adhesion molecules on antigen-presenting cells and endothelial cells. Epicutaneous application of non-toxic doses of 2,4-dinitrofluorobenzene (DNFB) onto the skin of non-sensitized individuals elicited progressive staining for ICAM-1 on dermal microvascular endothelial cells. To elucidate the question of whether contact allergens can act directly on endothelial cells to elevate their expression of surface structures that bind leukocytes, confluent monolayers of human umbilical vein endothelial cells were incubated with the contact allergens NiSO[4sub], CoSO[4sub] or DNFB. The ICAM-1, E-selectin and HLA-DR expression were quantified by immunofluorescence flow cytometric analysis. Furthermore VCAM-1, E-selectin and ICAM-1 transcription were demonstrated by Northern blot hybridization. Constitutive ICAM-1 expression on HUVEC increased similarly to that obtained after LPS (20 μg/mI) stimulation after 4 and 24 hours of incubation with I or 2 mM NiSO[4sub] or CoSO[4sub], respectively. Pulse-stimulation with 100 or 500 nM DNFB resulted in a modest but significant increase of ICAM-1-positive cells. E-selectin and VCAM-l were not expressed on untreated HUVEC; 4 to 6 hours exposure to nickel sulfate and LPS resulted in a potent induction of E-selectin and VCAM-1 expression. DNFB and PMA had no significant influence on VCAM-l expression. None of the tested contact allergens was capable of inducing HLA-DR expression on EC at 48 to 72 hours. Enhanced expression of adhesion molecules may be an important early unspecific mechanism for induction and elicitation of a contact dermatitis. [ABSTRACT FROM AUTHOR]

Published

1992

26. Human T cell responses to recombinant mite antigens of <em>Dermatophagoides farinae</em>.

Author

Fujh, S., Ono, K., Shigeta, S., Jyo, T., and Yamasuita, U.

Subjects

LYMPHOCYTES, LEUCOCYTES, T cells, IMMUNOGLOBULINS, ANTIGENS, IMMUNITY

Abstract

We studied T cell responses to four glutathione S transferase (GST)-fused mite antigens prepared in our laboratory using peripheral blood lymphocytes from mite-sensitive patients with bronchial asthma. Of the four recombinant antigens, purified GST-Mag3 had the strongest ability to cause patients' lymphocytes to proliferate, and its potency was almost comparable to that of crude mite bodies (Dfb) and faeces (Dff) antigens and a purified major antigen, Der f 2. The responder lymphocytes were mainly T cells, because the proliferative response was depleted by the treatment of lymphocytes with anti-CD3 antibody and complement, but not with anti-CD20 antibody and complement. The responsiveness of lymphocytes to GST-Mag3 correlated with that to Der f 2, but GST-Mag3 displayed slightly higher activity to stimulate lymphocytes than Der f 2. Simultaneously, the levels of Dff- and GST-Mag3- specific IgE antibodies correlated with the responsiveness of lymphocytes to GST-Mag3. These results suggest that Mag3 is a new valuable antigen for the response of T cell proliferation in mite-sensitive patients. [ABSTRACT FROM AUTHOR]

Published

1997

27. Selective IgM deficiency in adults: phenotypically and functionally altered profiles of peripheral blood lymphocytes.

Author

Ohno, T., Inaba, M., Kuribayashi, K., Masuda, T., Kanoh, T., and Uchino, H.

Subjects

IMMUNOGLOBULIN M, LYMPHOCYTES, ANTIGENS, T cells, LEUCOCYTES, PATIENTS

Abstract

Peripheral blood lymphocytes from four patients with selective IgM deficiency were examined phenotypically and functionally. Although B cell subpopulations determined by surface immunoglobulins were within normal or nearly normal range, T8+ cells were significantly increased and T4/T8 ratios were inverted in three patients. IgM specific hyporesponsiveness in the PWM-driven immunoglobulin production system was observed in all four patients. Ia-like antigen positive T cells were increased in two patients; both had increased Leu2a+ Leu15+ suppressor-effector cells. In addition, Leu3a+Leu8+ suppressor-inducer cells were increased in one of these two patients. Excessive (either IgM-specific or isotype non-specific) suppressor activity of T cells and IgM specific hyporesponsiveness of non-T cells were observed in these two patients in the recombination plaque assay. Although these results showed the complexity of the pathogenesis of this syndrome, they suggested that suppressor-associated T cells may play a role in some patients with selective IgM deficiency. [ABSTRACT FROM AUTHOR]

Published

1987

28. HNK-1 monoclonal antibody (Leu-7) in the identification of abnormal expansions of large granular lymphocytes.

Author

Pandolfi, F., Semenzato, G., de Rossi, G., Quinti, Isabella, Guglielmi, C., Pezzutto, A., Lopez, Mauela, Tonietti, G., Fontana, L., Abo, T., and Aiuti, F.

Subjects

MONOCLONAL antibodies, LEUCOCYTES, T cells, ANTIGENS, CELL proliferation, IMMUNITY

Abstract

Among 12 cases of chronic T lymphoproliferative disorders we observed, six patients showed an expansion of mononuclear cells with azurophilic granules usually referred to as large granular lymphocytes or LGL. Cells obtained from five patients with these abnormal LGL proliferations were studied with several surface markers including their reactivity with the HNK-1 monoclonal antibody reported to be specific for LGL. Ceils in four out of five cases were HNK-t positive. Whereas normal LGL have been reported to be unreactive with several T cell markers, three cases showed the co-existence of HNK-1 and surface markers expressed by T cells. Two cases were characterized by the proliferation of OKT8 cells. Cells from one patient were HNK-l positive but did not express T or monocytic antigens. These cells were apparently not completely mature since 2-naphthyl acetate acid esterase activity was negative. Cells from the remaining case were HNK-1 negative and positive for T and monocytic antigens. An increase of OKT-10 cells was observed in only one patient. Our data indicate that proliferations of LGL represent a remarkable proportion of the rare cases of sheep erythrocyte rosetting chronic lymphocytic leukaemias or lymphomas. Besides the morphology of LGL, the rosetting ability and the negativity for peroxidase, cells from these cases showed a vast heterogeneity of other structural and functional markers, possibly reflecting different stages in the maturation of these cells. The HNK-1 monoclonal antibody proved to bean important marker in the identification of these cases. [ABSTRACT FROM AUTHOR]

Published

1983

29. Variable effect on peripheral blood leucocytes during JE virus infection of man.

Author

Chaturvedi, U. C., Mathur, Asha, Tandon, Pushpa, Natu, S. M., Rajvanshi, Suman, and Tandon, H. O.

Subjects

ENCEPHALITIS, LEUCOCYTES, BLOOD cells, LYMPHOCYTES, T cells, ANTIGENS, PHAGOCYTOSIS

Abstract

The peripheral blood leucocytes of twenty-four cases of Japanese encephalitis (JE) were studied and the findings were compared with those in twenty-five normal healthy controls of matching age and sex. In the early phases of the disease marked neutrophil leucocytosis was seen which returned to almost normal levels by the fourth week. Lymphopenia was associated with diminished T lymphocytes but the number of B lymphocytes remained within the normal range. Though the number of T lymphocytes was reduced, their function of leucocyte migration inhibition in the presence of JE virus antigen was significantly higher. The phagocytic activity of the neutrophils, as shown by the uptake of neutral red dye, was diminished but the phagocytic activity of monocytes as shown by the uptake of neutral red dye or ingestion of latex particles remained unaffected. HI antibodies against JE virus were significantly higher in cases of encephalitis as compared with the control group. Thus, JE virus infection in man has a variable effect on different components of the peripheral blood leucocytes. [ABSTRACT FROM AUTHOR]

Published

1979

30. Migration inhibition of T lymphocytes from human peripheral blood by specific antigen and lymphokines.

Author

Kowalczyk, Danuta and Zembala, Marek

Subjects

CELL migration, BLOOD cells, LYMPHOCYTES, T cells, ANTIGENS, LYMPHOKINES, LEUCOCYTES

Abstract

The inhibition of migration of human peripheral blood cells in the presence of PPD was studied. It was found that migration inhibition of peripheral blood mononuclear cells (MN) from Mantoux-positive donors was far greater than the migration inhibition of peripheral blood leucocytes (PBL). Moreover, MN cells and T lymphocytes showed larger and more uniform areas of migration. In contrast, the migration of B lymphocytes and monocytes was poor. Further analysis using purified subpopulations of MN cells showed that PPD inhibited the migration of T lymphocytes but not of B lymphocytes and monocytes. Corresponding to these findings, lymphokine-containing supernatants also inhibited the migration of purified T cells from Mantoux-negative donors. It was concluded that the T lymphocyte was the predominant cell in the MN cell population which migrated, and was subject to inhibition by PPD or lymphokines. These results imply that the movement of human T lymphocytes may be influenced by soluble factors from antigen-activated sensitized cells. [ABSTRACT FROM AUTHOR]

Published

1978

31. Expression on procine γδ lymphocytes of a phylogenetically conserved surface antigen previously restricted in expression to ruminant γδ T lymphocytes.

Author

Carr, M.M., Howard, C.J., Sopp, P., Manser, J.M., and Parsons, K.R.

Subjects

LYMPHOCYTES, T cells, IMMUNE system, SWINE, ANTIGENS, IMMUNOLOGY, LEUCOCYTES

Abstract

A 180,000 MW molecule has been identified on porcine leucocytes that is the homologue of the 215,000/300,000 MW WC1 (T19) leucocyte antigen previously considered to be restricted to ruminants. In ruminants the WC1 molecule is expressed by a T-cell subpopulation that is CD2-CD4-CD8-CD5+ and that is γδ T-cell receptor positive (TcR+). In pigs, the 180,000 MW molecule, identified by a new monoclonal antibody CC101, is expressed by a γδ TcR+ T-cell subpopulation that is also CD2-CD4 CD8. The p180+ cells are a major T-cell subpopulation comprising approximately 40% of the peripheral blood mononuclear cells from 6-9-month-old pigs. Expression of p180 identifies the majority of the CD2-CD4-CD8- T cells in porcine blood. The p180+ T cells have a distribution in lymphoid tissues that is distinct from that oft cells that express the CD2, CD4 or CD8 molecules. They are evident particularly in the thymic medulla, the epithelium, lamina propria and interfollicular areas of the small intestine, and the superficial dermis of the skin, but largely absent from conventional T-dependent areas of secondary lymphoid tissue. [ABSTRACT FROM AUTHOR]

Published

1994

32. Effects of Cyclic GMP-Agonists on Ciclosporin-Induced Suppression of Human Lymphokine Production.

Author

Svenson, M. and Bendtzen, K.

Subjects

LYMPHOKINES, LEUCOCYTES, ANTIGENS, T cells, LYMPHOCYTES, IMMUNITY

Abstract

Ciclosporin (Cs) inhibits the elaboration of the lymphokine leukocyte migration inhibitory factor (LIF) from human blood mononuclear cells (MNC) stimulated with recall antigen. This inhibition was counteracted by 3 &time; l0-3 M dibutyryl-cyclic GMP and 8-bromo-cyclic GMP and by the cyclic GMP-agonists, sodium nitroprusside (NaNPr), ascorbic acid (As A), sodium azide (NaN3) and carbacholine. Using 5 &time; l0-5 M NaNPr, 1 &time; l0-3 M NaN3, or 3 &time; 10-3 M As A1 25-50-, 4-8- and 2-3-fold elevations of MNC and T-lymphocyte cyclic GMP-levels were obtained independently of the presence of Cs. NaNPr was the most potent of these three cyclic GMP-agonists in counteracting the effect of Cs. The results indicate that intracellular cyclic GMP is a major factor involved in the reversal of Cs-induced inhibition of LIF-production. None of the cyclic GMP-analogues or -agonists by themselves possessed Interleukin 1-like activity, measured by their ability to induce LIF-production by macrophage-depleted T-lymphocytes challenged by recall antigen. [ABSTRACT FROM AUTHOR]

Published

1985

33. Murine APC Activation in the Xenogeneic MLC.

Author

Benfield, M. R., Witson, J. C., Alter, B. J., and Bach, F. H.

Subjects

T cells, CELL proliferation, HUMAN beings, ANTIGENS, LEUCOCYTES, CYTOKINES

Abstract

Purified human T cells proliferate in response to direct and indirect presentation of human alloantigens. However,, until recently it was believed that human T cells could respond only indirectly to murine xenoantigens. We recently used the mixed leucocyte culture (MLC) to demonstrate that purified human T cells proliferate in response to direct presentation of murine xenoantigens by murine antigen-presenting cells (APC) in the presence of human cytokines. We suggested that cytokines might function poorly across species barriers. In this study, we demonstrate that although proliferation occurs in the presence of exogenously added cytokines, the precursor frequency of responding human T cells is much lower in a xenogeneic than in an allogeneic MLC. We demonstrate that human T cells also proliferate in response to murine APC in the presence of murine cytokines., and murine cytokines augment the proliferative response seen in a human anti-human MLC, ruling out the possibility that an absolute cytokine incompatibility exists between these species. We show that exogenously added human IL-I causes maximal proliferation of human T cells in response to murine xenoantigens only when added early in the culture. We further demonstrate that murine APC preincubated in human rIL-1, and washed extensively, prior to use as stimulating cells, cause human T-cell proliferation without the need for exogenously added cytokines. Finally, we noted that during interactions of human T cells and murine APC, little to no IL-1 is produced, whereas after the addition of exogenous IL-1, a marked increase in the production of IL-I is seen. These data suggest that during interactions between human T cells and murine APC, the murine cells do not receive adequate stimulation to produce sufficient costimulatory signals to allow proliferation of the human T cells. [ABSTRACT FROM AUTHOR]

Published

1993

34. The Role of the CD8-Positive Subset of T Cells in Proliferative Responses to Soluble Antigens.

Author

Bruserud, Ø., Sollid, L., Gaudernack, G., and Thorsby, E.

Subjects

T cells, LYMPHOCYTES, IMMUNITY, IMMUNOGLOBULINS, ANTIGENS, LEUCOCYTES

Abstract

The role of CD8 (T8, Leu 2)-positive T lymphocytes in the proliferative T-lymphocyte response to mumps and Coxsackie B4 viral antigens in vitro was investigated. The frequency among enriched T-lymphocyte blasts of antigen-reactive T lymphocytes (ARTL) restricted by different DR-associated elements was investigated, using antigenic restimulation with allogeneic antigen-presenting cells in a limiting dilution assay. A decreased frequency of DR3- restricted and an increased frequency of DR4-restricted mumps and Coxsackie B4 ARTL were seen in the limiting dilution assay, whether or not HLA class I determinants were shared in the antigenic restimulation. Removal of CDS-positive cells did not increase the primary in vitro responsiveness to mumps and Coxsackie B4 viral antigens, and did not change the DR-associated differences in the frequency of ARTL seen in the limiting dilution assay. [ABSTRACT FROM AUTHOR]

Published

1986

35. HLA Class-II-Specific T-Lymphocyte Clones with Dual Alloreactive Functions.

Author

Flomenberg, N., Duffy, E., and Dupont, B.

Subjects

HLA histocompatibility antigens, T cells, ANTIGENS, IMMUNOGLOBULINS, LEUCOCYTES, HLA class II antigens

Abstract

The relationship between T lymphocytes that proliferate in response to HLA class II antigens and those that mediate the cytotoxic response toward HLA class II target antigens was investigated. Alloreactive T-cell clones were derived under conditions in which the likelihood of clonality was high. Three populations of HLA class-II-specific T cells were identified. Two of these populations exhibited only HLA class-II-directed cytotoxicity or HLA class-II-induced proliferation. The third population of T cells exhibited both of these responses. [ABSTRACT FROM AUTHOR]

Published

1984

36. The Availability for Recognition of Normal H--2 Antigens by Cytotoxic T Lymphocytes on a Rauscher--Virus--transformed Cell, RBL--5A.

Author

Watson, A., Zarling, D. A., and Bach, F. H.

Subjects

LYMPHOCYTES, T cells, CELL membranes, ANTIGENS, MOUSE leukemia, LEUCOCYTES

Abstract

The availability for recognition of cell surface H-2Db antigenic determinants on RBL-5A cells in comparison to normal C57BL/6 cells was investigated by an in vitro immunological assay. No differences in the immunological recognition of the H-2Db antigens on RBL-5A cells compared to normal C57UL/6 cells were detected. This assay system, however, readily detected changes in the H-2Kb determinant profile on target cells from the C57BL/6 H-2Kb region mutant strains H(zl) and H(z170) when compared to normal C57BL/6 mice. The result obtained with RBL-5A target cells therefore suggests that Rauscher murine leukaemia virus transformation does not induce, either genotypically or phenotypically, an immunologically recognizable alteration of the H-2Db antigen profile on this cell. [ABSTRACT FROM AUTHOR]

Published

1979

37. Generation of T Memory Cells in One-Way Mixed Lymphocyte Culture.

Author

Häyry, P. and Andersson, L. C.

Subjects

T cells, LYMPHOID tissue, CELL culture, IMMUNOGLOBULINS, LEUCOCYTES, ANTIGENS

Abstract

Neither normal CBA (H-2k) nor purified spleen T cells respond in vitro to soluble or insoluble membrane preparations or to ultraviolet-light-inactivated stimulator cells of the allogeneic DBA/2 (H-2d) strain. However, CBA spleen cells deprived of phagocytic cells show a slight proliferative response under these conditions. After being primed against mitomycin-blocked DBA/2 cells in one-way mixed lymphocyte culture, the secondary blast-derived T `memory' cells display a good secondary blast (proliferative) response to both membrane antigens and to ultraviolet-light-inactivated stimulator cells. In addition to this, the secondary T lymphocytes--in contrast to nonprimed T cells--respond by cytotoxicity when ultraviolet-light-inactivated cells are used as the second stimulant. [ABSTRACT FROM AUTHOR]

Published

1976

38. The tissue distribution of T lymphocytes expressing different CD45 polypeptides.

Author

Janossy, G., Bofill, M., Rowe, D., Muir, J., and Beverley, P. C. L.

Subjects

LYMPHOCYTES, T cells, GROWTH factors, LEUCOCYTES, ANTIGENS, IMMUNE system

Abstract

The distribution of T lymphocytes expressing the different polypeptides of the leucocyte common antigen (LCA) family detected by CD45R and UCHL1 antibodies has been studied in normal lymphoid tissues. In the thymus most cortical thymocytes express UCHL1 and co-express CD4 and CD8. The more mature membrane CD3+ (mainly medullary) T cells are heterogeneous and may express both UCHL1 and CD45R weakly or be restricted to display CD45R or UCHLI alone. In the medulla both the CD45R+ and UCHL1+ subpopulations contain single positive CD4 and CDS cells. In tonsils, germinal centre T cells are almost exclusively UCHL1+, CD4+ and a proportion also express HNK-l (Leu 7) antigen. In the paracortical areas approximately equal numbers of CD45R+ and UCHL1+ cells are found but these separately occupy nests of cells containing one or the other type. Again, both CD45R+ and UCHL1+ cells include single CD4+ and CD8+ lymphocytes. A small proportion (<5%) of strongly CD45R+, UCHL1+ double-stained cells are also seen, and these probably represent recently activated lymphocytes. In the gut, small clusters of such strongly double- labelled cells are in the submuscular mucosae while cells of the lamina propria are almost exclusively UCHL1+. Many intra-epithelial lymphocytes are only weakly positive or negative for UCHL l and appear to be CD45R+ . These results are consistent with the view that expression of different CD45 polypeptides identifies successive stages of thymocyte-T-cell maturation and that following their thymic education, unprimed T lymphocytes are CD45R+, while primed memory T cells arc UCHL1+. These populations occupy different microenvironments. [ABSTRACT FROM AUTHOR]

Published

1989

39. Cellular events during memory T-cell activation <em>in vitro</em>: the UCHL1 (180,000 MW) determinant is newly synthesized after mitosis.

Author

Akbar, A.N., Timms, A., and Janossy, G.

Subjects

T cells, MITOSIS, ANTIGENS, GOLGI apparatus, CELL proliferation, LEUCOCYTES

Abstract

After T-cell activation, a switch of leucocyte common antigen (LCA) expression occurs which is detected by the disappearance of CD45R and the appearance of UCHL1 positivity. Upon activation of CD45R+ T cells by phytohaemagglutinin (PHA), the IL-2 receptor (IL-2R) develops at 15 hr and blast cells enter the S phase at 20 hr, while remaining UCHL1-. At 40 hr, mitotic cells continue to express CD45R determinants, but weak UCHL1 reactivity is now detectable on 15-20% of these cells. By inhibiting the separation of daughter cells with cytochalasin D, it can be demonstrated that the UCHL1 antigen is newly synthesized in the Golgi apparatus before insertion into the membrane after the first mitosis. At 65 hr after activation, 80% of proliferating cells are UCHL1+. T cells undergo a similar development during allogeneic activation, and specific alloresponsive cells, tested in secondary mixed lymphocyte reaction (MLR), become greatly enriched among the proliferating UCHL1+ cells. Conversely, after a primary MLR, residual CD45R+ T cells are unresponsive to the original stimulus but can still proliferate in response to unrelated alloantigens. These results clarify both the time-course of the acquisition of UCHL1 antigen during the proliferative cycle of activated T cells, and indicate the shift of antigen responsive T-cell populations from the CE45R+ to the UCHL1+ pool. [ABSTRACT FROM AUTHOR]

Published

1989

40. Distribution and functional characteristics of antigen-specific helper T cells arising after Peyer's patch immunization.

Author

Dunkley, M. L. and Husband, A. J.

Subjects

ANTIGENS, T cells, IMMUNITY, GENETICS, LYMPH nodes, LEUCOCYTES, IMMUNOSUPPRESSION

Abstract

Antigen-specific T-helper cells for IgA responses arise in Peyer's patches (PP) following their immunization by subserosal injection of keyhole limpet haemocyanin (KLH). These are of the W3/25 phenotype and the W3/25 receptor is shown here to be involved in their helper function. These cells originate in PP and migrate via mesenteric lymph nodes (MLN) to thoracic duct lymph, although the MLN appear to be unnecessary for the induction or maturation of antigen-specific helper cells collected in thoracic duct lymph after intra-Peyer's patch (i.p.p.) immunization. KLH-specific helper cells can be detected subsequently in the intraepithelial lymphocyte population and also among lamina propria lymphocytes. The helper cells also relocate to PP distant to their site of origin where they are retained only when antigen is present. While i.p.p. immunization is an efficient route for the induction of IgA helper cells in gut-associated lymphoid tissue, it differs from oral immunization in that concomitant induction of antigen-specific splenic suppressor cells does not occur, indicating a role for epithelial antigen processing in this phenomenon. [ABSTRACT FROM AUTHOR]

Published

1987

41. Direct blockade of antigen-reactive B lymphocytes by immune complexes. An 'off' signal for precursors of IgM-producing cells provided by the linkage of antigen- and Fc-receptors.

Author

Oberbarnscheidt, J. and Kolsch, E.

Subjects

LYMPHOCYTES, ANTIGENS, B cells, LEUCOCYTES, T cells, IMMUNOGLOBULINS

Abstract

Antigen-antibody complexes efficiently inhibit the induction of antibody formation. Using Mishell-Dutton cultures, it can be demonstrated that neither T cells nor their products are required for this inhibition of IgM PFC formation. The blockade is at the level of B cells and cannot be overcome by LPS or TRF. The data demonstrate that cross-linking of antigen- and Fc-receptors by antigen-antibody complexes is a blocking signal for B cells. [ABSTRACT FROM AUTHOR]

Published

1978

42. TL we meet again.

Author

Nagler, Cathryn and Wroblewska, Joanna

Subjects

MAJOR histocompatibility complex, MOLECULES, LEUKEMIA, ANTIGENS, T cells, INTESTINAL mucosa, LEUCOCYTES

Published

2011