Characterization of an immunosuppressant protein from Dermacentor andersoni (Acari: Ixodidae) salivary glands.

A 36-kDa soluble protein was found in the salivary glands of female Dermacentor andersoni (Stiles) ticks that suppressed the in vitro proliferative response of murine splenocytes to concanavalin A (Con A). Incubating the purified protein with splenocytes reduced the incorporation of thymidine into the DNA of proliferating T-lymphocytes by more than 90% compared with cells exposed to Con A and buffer alone. The N-terminal amino acid sequence of the immunosuppressant protein was determined to be NH2-Leu-His-Lys-Ala(Asp)-Lys-Ile-Val-Lys-Leu-Thr -Glu-Glu-Ala -Arg-Lys-Tyr-Val-Gly-Arg-Xxx-Xxx-Thr-Thr-Ala-Leu-Gly-. Although the sequence exhibited a modest degree of similarity with a segment of immunoglobulin-binding protein found in several species of mammals, the mode of action of the immunosuppressant protein is unknown. This protein may play an important role in suppressing the host's acquisition of resistance to ticks.

Infestation with pathogen-free nymphs of the tick Ixodes scapularis induces host resistance to transmission of Borrelia burgdorferi by ticks.

Female BALB/c mice were infested four times with pathogen-free Ixodes scapularis nymphs prior to infestation with nymphs infected with Borrelia burgdorferi B31. Each infestation was separated by a 14-day tick-free period. Mean weights of fed ticks and percentage reaching repletion did not indicate development of acquired resistance. Only 16.7% of mice repeatedly infested with pathogen-free ticks prior to infected I. scapularis nymph challenge became positive for B. burgdorferi. One hundred percent of control mice infested only with infected ticks were culture positive for B. burgdorferi.

Dermacentor andersoni: salivary gland proteins suppressing T-lymphocyte responses to concanavalin A in vitro.

Salivary glands obtained from feeding adult female Dermacentor andersoni (Acari:Ixodidae) were fractionated using differential centrifugation, detergents, centrifugal concentrators incorporating filter membranes with various molecular weight cutoffs, and preparative SDS-PAGE. A lymphocyte proliferation assay was used to evaluate the effects of salivary gland fractions on ConA-induced blastogenesis of normal murine splenocytes. Lipid, soluble, and detergent-soluble fractions were found to significantly suppress ConA-induced proliferation of splenocytes. Fractions containing soluble proteins suppressed splenocyte proliferation by ca. 26%. Suppressant activity in these fractions was due to components with molecular weights greater than 30 kDa. This suppression of splenocyte proliferation occurred with as little as 0.25 microgram protein per well. Salivary gland preparative SDS-PAGE fractions containing one or more soluble polypeptides or proteins with molecular weights in the range 36 to 43 kDa significantly suppressed murine splenocyte responses to ConA in vitro.

Effects of Dermacentor andersoni (Acari: Ixodidae) salivary gland extracts on Bos indicus and B. taurus lymphocytes and macrophages: in vitro cytokine elaboration and lymphocyte blastogenesis.

Cattle and laboratory animal species-acquired resistance to tick infestation has an immunological basis involving antigen presenting cells, B-lymphocytes, T-lymphocytes, and cytokines. Tick infestation has been shown to impair guinea pig antibody responses to a thymic-dependent antigen and in vitro responsiveness of lymphocytes to T-cell mitogens. Tick salivary gland extracts inhibited in vitro proliferative responses of normal murine lymphocytes to the T-cell mitogen concanavalin A (Con A) and enhanced reactivity of normal B-lymphocytes to the mitogen E. coli lipopolysaccharide (LPS). Salivary gland extracts collected daily during engorgement were shown to inhibit normal murine macrophage elaboration of interleukin-1 (IL-1) and tumor necrosis factor alpha (TNF) as well as murine T-lymphocyte production of interleukin-2 (IL-2) and interferon-gamma (IFN-G). Peripheral blood mononuclear cells collected from purebred Bos indicus and B. taurus were significantly inhibited in their in vitro responses to Con A by salivary gland extracts prepared daily from female Dermacentor andersoni stiles during the course of engorgement. Percentage of suppression of Con A responsiveness was similar for both B. indicus and B. taurus cells. The overall responsiveness of B. indicus derived T cells is significantly greater than that of similar cells from B. taurus, when mean counts per minute of methyl-tritiated-thymidine incorporation were compared for both groups. Cells of B. indicus origin were 34.5% more reactive. In vitro responsiveness of the same cell populations to LPS were significantly enhanced by the presence of tick salivary gland extracts. B. indicus lymphocyte reactivity to LPS was significantly greater (42.9%) than that of similar B. taurus cells in the absence of salivary gland extracts. B. indicus and B. taurus macrophage elaboration of IL-1 were suppressed in a similar manner by tick salivary gland extracts prepared on days 5-9 of engorgement. B. indicus macrophages produced more IL-1 than similar cells of B. taurus origin either in the presence (45.6%) or absence (43.0%) of LPS. Macrophages derived from both genetic backgrounds were significantly suppressed in their LPS induced production of TNF in the presence of tick salivary gland extracts collected on days 0-9 of engorgement. B. indicus might be able to develop more vigorous immune responses to foreign immunogens presented to the animal during tick feeding.

Tick-induced modulation of the host immune response.

The tick-host-pathogen interface is characterised by complex immunological interactions. Host immune responses to tick infestation and infection with tick-borne pathogens involve cytokines, antibodies, complement and T lymphocyte regulatory and effector pathways. A successful host-parasite relationship is a balance between limiting the parasite by host defenses and the ability of the parasite to modulate, evade or restrict the host response. Hosts acquire immunological based resistance to tick infestation, which reduces engorgement, production of ova and viability. Salivary glands of ixodid ticks produce a complex array of immunogens and pharmacologically active molecules. Tick salivary gland derived material can modulate host cytokine, antibody and cell mediated immune responses. Both immunoregulatory and immune effector pathways of the host are suppressed. Tick feeding impairs the ability to develop a primary immune response to a thymic dependent immunogen. Lymphocytes obtained from tick infested hosts are reduced in their ability to proliferate in vitro to T lymphocyte mitogens, while responses to B lymphocyte polyclonal activators are unaltered. Normal macrophages and lymphocytes were exposed to female tick salivary gland extracts prepared daily during the course of engorgement. All extracts reduced lymphocyte responses to T cell mitogens and enhanced in vitro proliferation in the presence of a B lymphocyte mitogen. Macrophage elaboration of tumour necrosis factor alpha and interleukin-1 are significantly reduced in a differential manner. Production of interleukin-2 and interferon-gamma by T lymphocytes is reduced. Tick modulation of the host immune response could enhance the ability of the arthropod to obtain a blood meal and facilitate pathogen transmission to an immunocompetent host.

Inhibition of lipid A- and lipopolysaccharide-induced cytokine secretion, B cell mitogenesis, and lethal shock by lipid A-specific murine monoclonal antibodies.

Three murine hybridomas secreting IgM monoclonal antibodies (MAbs) to lipid A (LA) of Salmonella minnesota R595 were generated. These MAbs serologically cross-reacted with LA and lipopolysaccharide (LPS) of unrelated gram-negative bacterial species. All three MAbs significantly suppressed the ability of LA and LPS from various gram-negative bacteria to induce tumor necrosis factor (TNF)-alpha (36%-67%) and interleukin-1 (30%-98%) in murine peritoneal macrophages and to stimulate B lymphocytes (37%-78%). Lipid A-induced TNF alpha production was also suppressed in mice (86%-88%). All three antibodies protected adrenalectomized mice against lethal shock induced by LA of S. minnesota R595. Optimal protection was achieved with one of the antibodies (MLA-1), if it was administered 2 h before injection of lipid A, and full protection persisted < or = 24 h. Moreover, MLA-1 was able to protect adrenalized or D(+)-galactosamine-sensitized mice against lethal shock induced by LPS derived from various gram-negative bacteria. This cross-protection could be predicted on the basis of serologic cross-reactivity and cross-neutralization by MLA-1 of the bioactivity of the heterologous LA or LPS in vitro.

Modulation of host-immune responses by ticks (Acari: Ixodidae): effect of salivary gland extracts on host macrophages and lymphocyte cytokine production.

Ixodid tick infestation induces host acquired resistance, which involves immunoglobulin cell-mediated and complement-dependent effector pathways. Ticks have developed countermeasures to modulate host antiarthropod responses. Ixodid-mediated host immunomodulation results in vitro in reduced responsiveness to T-lymphocyte mitogens for cells obtained from infested hosts and impaired antibody responses to a thymic dependent antigen. Salivary gland extracts from days 0-9 of engorgement from unmated, female Dermacentor andersoni Stiles suppressed lymphocyte proliferative responses (LPS) to the T-cell mitogen Con A up to 68.4%, whereas responsiveness to E. coli LPS was enhanced. Cytokines assessed in this study included interleukin-1, IL-1, and tumor necrosis factor (TNF) alpha produced by macrophages, and interleukin-2, IL-2, and gamma interferon (IFN-G) secreted by T-lymphocytes. Salivary gland extracts prepared from tissues obtained on days 0-5 of engorgement suppressed IL-1 elaboration from 89.8% on day 0 through 37.5% on day 6. Levels of TNF were reduced from 40.7 to 94.6% throughout the course of the study. Production of IL-2 was suppressed by 14.1-31.9%, and IFN-G was reduced by 8.7-57.0%. Reduced IL-1 levels during the early phases of feeding indicated reduced host ability to activate T-lymphocytes and provide costimulatory, differentiation, and development signals for B-cells. Both IL-1 and TNF are endogenous pyrogens and activate polymorphonuclear leukocytes. Activities of TNF and IFN-G include antiviral properties and induction of expression of class I and II major histocompatibility complex molecules, which are critical components in the recognition of antigen by T-lymphocytes. The autocrine role of IL-2 in proliferation of T-lymphocytes is central to the development of immune reactivity involving T-cell regulation or effector functions or both. Reductions in cytokine levels would suppress immune responses directed toward immunogens introduced into the host during the course of tick feeding. These results indicates that immunomodulation of the host during tick feeding facilitates engorgement and pathogen transmission.

Neuro-hormonal host defence in endotoxin shock.

The sensitivity (LD100) of mice to lipopolysaccharide (LPS) endotoxin and to its toxic moiety, lipid A (LA), increased 500-fold after adrenalectomy (ADX). Inhibition of glucocorticoid synthesis in intact mice by metyrapone had a similar, though less dramatic, sensitizing effect to LPS. In ADX mice, the serum level of tumor necrosis factor-alpha (TNF) was 40-60 times higher than that in controls at 2 h after LPS/LA treatment. In intact mice the serum corticosterone level fell 1 h after lipid A injection to below detectable levels, which was followed by a brisk increase reaching the peak level of 48-50 micrograms/100 ml at 2 h. Both TNF production and the lethal effect of PLS/LA could be inhibited in ADX mice by glucocorticoid treatment. Plasma prolactin was increased significantly 1 h after endotoxin administration in both intact and ADX animals.

Development and characterization of ouabain-resistant human fusion partners.

The ouabain-resistant mutant cell lines, HOA-1 and HOA-20 were developed from WI-L2-729-HF2 by cloning with increasing concentration of ouabain. Both parent and mutant cell lines were resistant to base analogues, 6-thioguanine (6-TG) and 8-azaguanine (8-AG) to the level of 20 micrograms/ml in the culture medium. The parent cell line WI-L2-729-HF2 was highly sensitive to ouabain, whereas HOA-1 and HOA-20 were resistant to ouabain to the level of 1 microM and 20 microM, respectively. However, all the cell lines were sensitive to HAT-selective medium which is essential for hybrid selection after fusion. All three lymphoblastoid cell lines were positive for Epstein-Barr virus nuclear antigen (EBNA), secreted TNF-beta (lymphotoxin) without any external stimulation, secreted trace amounts of IgG(kappa), which was also present in their cytoplasm and had IgM(kappa) as surface bound immunoglobulin. They also expressed the CD20, CD71 (transferrin receptor) as surface antigens. In addition to these antigens, HOA-20 also expressed CD38 antigen. The karyotype analysis of these cell lines revealed modal chromosomal numbers ranging from 40 to 47. The HLA-A, -B and -C antigens expressed by WI-L2-729-HF2 and its mutants HOA-1 and HOA-20 were identical. Both the HOA-1 and HOA-20 mutants were found suitable for the generation of hybrids after fusion with EBV-transformed human B-lymphocytes.

Human--human hybridomas secreting lipid A reactive monoclonal antibodies.

Five human-human hybridoma cell lines secreting monoclonal antibodies (mAbs) against lipid A (LA) were produced by cell fusion of Epstein-Barr virus (EBV) transformed human peripheral blood lymphocytes and a human lymphoblastoid cell line KR-4. All these mAbs were isotyped as IgM(kappa) and reacted with lipopolysaccharides (LPS) and LA of various gram-negative bacteria. Whereas the binding of only four of the five mAbs to solid-phase LA was blocked by polymyxin-B sulphate, the mitogenic effect of LPS and LA on murine B lymphocytes was inhibited by all five mAbs. These results demonstrate that the human immune system recognizes at least two common epitopes in lipid A of various gram-negative bacteria.