IgG Suppresses Antibody Responses in Mice Lacking C1q,C3, Complement Receptors 1 and 2, or IgG Fc-Receptors

Antigen-specific IgG antibodies, passively administered to mice or humans together with large particulate antigens like erythrocytes, can completely suppress the antibody response against the antigen. This is used clinically in Rhesus prophylaxis, where administration of IgG anti-RhD prevents RhD-negative women from becoming immunized against RhD-positive fetal erythrocytes aquired transplacentally. The mechanisms by which IgG suppresses antibody responses are poorly understood. We have here addressed whether complement or Fc-receptors for IgG (FcγRs) are required for IgG-mediated suppression. IgG, specific for sheep red blood cells (SRBC), was administered to mice together with SRBC and the antibody responses analyzed. IgG was able to suppress early IgM- as well as longterm IgG-responses in wildtype mice equally well as in mice lacking FcγRIIB (FcγRIIB knockout mice) or FcγRI, III, and IV (FcRγ knockout mice). Moreover, IgG was able to suppress early IgM responses equally well in mice lacking C1q (C1qA knockout mice), C3 (C3 knockout mice), or complement receptors 1 and 2 (Cr2 knockout mice) as in wildtype mice. Owing to the previously described severely impaired IgG responses in the complement deficient mice, it was difficult to assess whether passively administered IgG further decreased their IgG response. In conclusion, Fc-receptor binding or complement-activation by IgG does not seem to be required for its ability to suppress antibody responses to xenogeneic erythrocytes.     

Influence of Complement on the Neutralization of Murine Cytomegalovirus by Rabbit Antibody

Antiserum against murine cytomegalovirus produced in the rabbit contained complement (C')-requiring neutralizing (CRN) antibody. The proportion of CRN was extremely high (up to 98%) during the early portion of an immunization procedure, whereas the antisera produced late had a much lower proportion that required C'. The antiserum produced was specific for MCMV with or without C'.     

Thymus-independent Step in the Immune Response to Sheep Erythrocytes

THE nature of the T and B cell interaction in the response to erythrocyte antigens¹ has been an area of intense interest recently. Perhaps because of the influences of molecular biology, there has been a tendency to invoke specific mechanisms such as informational RNA and thymus specific immunoglobulins as mediators of this synergism. But once it was demonstrated that antigen specific receptors of immunoglobulin nature were on the surface of immune competent cells², it was possible to approach the problem more simply; that is from the viewpoint of control of protein synthesis and/or release of proteins from the cell surface. This communication outlines recent evidence concerning the role of non-specific mitogens in the control of antibody precursor (B cells) and antibody secreting cells.     

Functional Compensation between Cholecystokinin-1 and -2 Receptors in Murine Paraventricular Nucleus Neurons

Cholecystokinin (CCK) and its receptor subtypes CCK-1 and -2 have diverse homeostatic functions. CCK-1 and -2 receptors share a common phosphatidylinositol signaling pathway, yet little is known regarding their possible functional coupling. We focused on CCK-mediated Ca²⁺ signaling in parvocellular paraventricular nucleus (PVN) cells, which control satiety and other autonomic functions. Analysis of mouse hypothalamic slices demonstrated that the general CCK receptor agonist CCK-8s (10 nm) triggered Ca²⁺ transients most significantly in the posterior subregion of the PVN (PaPo). This 10 nm CCK-8s-induced response was absent in CCK-1 receptor knock-out (CCK1R^−/−) slices, showing that the response is mediated by CCK-1 receptors. CCK-8s concentrations higher than 30 nm triggered a Ca²⁺ rise similarly in wild-type and CCK1R^−/− slices. The large CCK-8s (100 nm)-induced Ca²⁺ responses in CCK1R^−/− slices were blocked by a CCK-2 receptor antagonist (CI-988), whereas those in wild-type slices required a mixture of CI-988 and lorglumide (a CCK-1 receptor antagonist) for complete antagonism. Therefore, CCK-1 and -2 receptors may function synergistically in single PaPo neurons and deletion of CCK-1 receptors may facilitate CCK-2 receptor signaling. This hypothesis was supported by results of real-time RT-PCR, immunofluorescence double labeling and Western blotting assays, which indicated CCK-2 receptor overexpression in PaPo neurons of CCK1R^−/− mice. Furthermore, behavioral studies showed that intraperitoneal injections of lorglumide up-regulated food accesses in wild-type but not in CCK1R^−/− mice, whereas CI-988 injections up-regulated food accesses in CCK1R^−/− but not in wild-type mice. Compensatory CCK signaling via CCK-2 receptors in CCK1R^−/− mice shed light on currently controversial satiety-controlling mechanisms.     

Response of Mouse T and B Lymphocytes to Sheep Erythrocytes

THE primary immune response of mice to sheep red blood cells (SRBC) involves two types of lymphocytes: the antibody-forming cell series, whose precursors are found in bone marrow (B cells) and cooperating or “helper” cells of uncertain function whose precursors are found in the thymus (T cells)¹. Within 24 h of an intravenous injection of SRBC, an increase of haemolytic antibody plaque-forming cells (p.f.c.) occurs in the spleen, reaching a peak 5 days later. Part, but not all, of this increase is due to division among the B cells². T cells in the spleen also undergo a wave of mitosis, detectable from the second to the fifth day³.     

Dose-Dependent Induction of Murine Th1/Th2 Responses to Sheep Red Blood Cells Occurs in Two Steps: Antigen Presentation during Second Encounter Is Decisive

The differentiation of CD4 T cells into Th1 and Th2 cells in vivo is difficult to analyze since it is influenced by many factors such as genetic background of the mice, nature of antigen, and adjuvant. In this study, we used a well-established model, which allows inducing Th1 or Th2 cells simply by low (LD, 10⁵) or high dose (HD, 10⁹) injection of sheep red blood cells (SRBC) into C57BL/6 mice. Signature cytokine mRNA expression was determined in specific splenic compartments after isolation by laser-microdissection. LD immunization with SRBC induced T cell proliferation in the splenic T cell zone but no Th1 differentiation. A second administration of SRBC into the skin rapidly generated Th1 cells. In contrast, HD immunization with SRBC induced both T cell proliferation and immediate Th2 differentiation. In addition, splenic marginal zone and B cell zone were activated indicating B cells as antigen presenting cells. Interestingly, disruption of the splenic architecture, in particular of the marginal zone, abolished Th2 differentiation and led to the generation of Th1 cells, confirming that antigen presentation by B cells directs Th2 polarization. Only in its absence Th1 cells develop. Therefore, B cells might be promising targets in order to therapeutically modulate the T cell response.     

Automated Technique for the Detection of Hemagglutinins to Sheep Erythrocytes

The Technicon autoanalyzer system used for the detection of homologous human hemagglutinins has been modified for the detection of hemagglutinins to sheep red blood cells. Antibody quantitation was obtained by plotting the optical density (OD) readings of peak heights of a serially diluted reference serum versus the serum dilutions. When the OD of the peak height of an unknown sample fell within the linear portion of the plot, a direct determination of the antibody titer was made. If the OD of the sample fell outside the linear portion, dilutions of the sample were carried out until a direct reading could be made. Assay by this method of at least 140 samples was possible within a day. Titers obtained with the autoanalyzer agreed very closely with those obtained by manual titration.     

Glucocorticoid Receptors in Murine Erythroleukaemic Cells

Abstract

Glucocorticoid receptors in murine erythroleukaemic cells were studied in relation to hexamethylene bisacetamide (HMBA) induced differentiation. Specific binding of dexamethasone was measured. A single class of saturable, high affinity binding sites was demonstrated in intact cells; with cell homogenates or fractions binding was low and could not be reliably quantified. Receptor binding in whole cell suspensions was lower in cells which had been treated with HMBA (36.5 ⁺- 8.2 pmol/g protein) than in untreated controls (87.9 ⁺- 23.6 pmol/g protein); dissociation constants were similar in treated (2.7 nM) and untreated cells (2.5 nM). Dexamethasone, hydrocortisone, corticosterone and progesterone competed with tritium-labelled dexamethasone for receptor binding sites; cortisone, deoxycorticosterone and oestradiol had little effect.     

Induction of Allergic Responses to Peanut Allergen in Sheep

Peanut allergy is the leading cause of deaths due to food-induced anaphylaxis but despite continued research, there are currently no specific treatments available. Challenge testing is limited in patients due to the high risk of adverse reactions, emphasising the need for an appropriate animal model. In the present study we examine the induction of allergic responses in a sheep model for peanut allergy. Sheep were sensitised with peanut (PN) extract and in separate injections with ovalbumin (OVA) or house dust mite (HDM) extract. Serum PN-specific IgE responses were detected in 40–50% of immunised sheep, while only 10% (1 of 10 sheep) showed detectable OVA-specific IgE. All PN-allergic sheep tested showed an Ara h 1-specific IgE response, while four out of five allergic sheep showed an Ara h 2-specific IgE response. Animals with high serum IgE levels to HDM were also PN IgE-positive. Of the PN-sensitised animals with high PN-specific IgE, 80% also showed an immediate hypersensitivity reaction following an intradermal PN injection. This new large animal model of peanut allergy may provide a useful tool for future investigations of allergen-associated immune mechanisms and specific immunotherapy.     

Differential Activation of Dual Signaling Responses by Human H1 and H2 Histamine Receptors

Abstract

Stimulation of human H₁ and H₂‐histamine receptors (HRs) primarily activates signaling pathways to increase intracellular calcium [Ca²⁺]_i and cyclic AMP (cAMP), respectively. Activation of H₂‐HR in human embryonic kidney (HEK) cells by histamine and dimaprit increases both cAMP formation and [Ca²⁺]_i, as determined by cAMP‐scintillation proximity assays and fluorescence imaging plate reader (FLIPR) assays. In HEK cells expressing relatively high levels of H₂‐HR (B_max = 26 pmol/mg protein), histamine and dimaprit are full agonists in eliciting cAMP responses with pEC₅₀ values of 9.30 and 7.72 that are 1000‐fold more potent than their respective pEC₅₀ values of 6.13 and 4.91 for increasing [Ca²⁺]_i. The agonist potencies decrease for both responses at lower H₂‐HR density (5 pmol/mg protein) and dimaprit exhibits partial agonist behavior for the [Ca²⁺]_i response. The inverse agonists ranitidine and cimetidine more potently inhibit cAMP production in the higher expressing H₂‐HR line. Histamine also activated both signaling pathways via human H₁‐HRs highly expressed (B_max = 17 pmol/mg protein) in HEK cells, with a 1000‐fold greater potency for [Ca²⁺]_i vs. cAMP responses (pEC₅₀ = 7.86 and 4.82, respectively). These studies demonstrate a markedly different potency for activation of multiple signaling pathways by H₁‐ and H₂‐HRs that may contribute to the selectivity of histamine responses in vivo.     

Effects of Silicate Polymers on Erythrocytes in Presence and Absence of Complement

The effects of silicates upon erythrocytes depend upon the degree of polymerization. Monomeric silicate does not appear to be taken up by red cells. Polymerized silicates are taken up and bound tightly. In the presence of small polymeric forms erythrocytes are lysed by complement. Larger polymers are bound to erythrocytes but do not sensitize to complement hemolysis. Larger polymers, however, are directly toxic and cause hemolysis in the absence of complement. Red cells exposed to complement-active polymers show characteristic alteration in morphology with the assumption of irregular bell shapes. Larger polymers cause the cells to become spherical before spontaneous rupture occurs. Large polymers cause erythrocyte agglutination but this is minimal or absent with small complement-active polymers. Complement-active polymers cause little or no change in osmotic fragility. Increase in mechanical fragility is a sensitive indication of the presence of larger, agglutinating polymers. The conversion of pneumococci from Gram positivity to negativity appears to be caused principally by complement-active polymers. Possible implications of polymer size and complement activity are discussed in relation to production of silicotic lesions by silica-containing ores.     

Restoration of the Immune Response to Sheep Erythrocytes by a Serum Factor

THE immune response of CBA mice to sheep erythrocytes (SRBC) is known to be thymus-dependent because strain members thymectomized during the first few hours of life exhibit a marked inability to respond to this antigen^1,2. Experiments with isoantisera suggested that a cell to cell interaction is involved in this response. Thymus cells per se do not develop into haemolytic plaque-forming cells, but in some, so far obscure, way they cause cells of bone marrow origin to become producers of haemolytic plaques^2,3. A study of spleen cells from neonatally thymectomized (NNT) mice in a tissue culture system indicated that the decreased responsiveness to SRBC is also expressed in vitro. In that case 15×10⁶ NNT spleen cells produced only 500 haemolytic plaques when assayed on day 4 of culture. But when 15×10⁶ thymus cells were added to identical cultures of NNT spleen cells at inception, the number of haemolytic plaque forming cells increased to 2,300 (ref. 4). When an equivalent number of thymus cells alone were incubated with SRBC there was no response.     

Serum and Egg Antibody Responses in Chickens to Escherichia coli

The effects of Freund’s adjuvants on antibody production in chickens against E. coli whole cells were examined. The levels of anti-E. coli IgG antibodies in serum were higher when Freund’s complete (FCA) or incomplete adjuvant (FIA) was administered than that without adjuvant. Production of antibodies recognizing E. coli cells and their lipopolysaccharide was enhanced by FIA, while both FIA and FCA enhanced production of antibodies recognizing outer membrane components. In contrast, serum IgM antibody levels were higher when no adjuvant was used. Anti-E. coli IgG antibodies in serum were efficiently transferred to egg yolk, giving antibody activity in egg yolk similar to that in serum. However, anti-E. coli IgM antibodies were not detected in the egg, suggesting that egg (white) IgM was not influenced by antigenic stimulation of the humoral immune system. Antimicrobial activity of the egg yolk IgG was highest when the bacteria antigen was injected with FIA.     

Use of Formalinized Sheep Erythrocytes in the Rubella Hemagglutination-Inhibition Test

Rubella antibody determination by the hemagglutination-inhibition test was effectively simplified by substitution of formalinized sheep red blood cells for avian erythrocytes.     

小鼠念珠菌感染模型和抗感染免疫

目前,临床相关的小鼠念珠菌感染疾病模型种类日益增多.与早期小鼠念珠菌感染模型相比,近期感染模型与临床上免疫抑制机会性念珠菌感染患者的感染方式、感染的发展进程、临床表现、靶器官临床病理组织学特征更相近.建立了特定免疫缺陷小鼠(如转基因/基因敲除小鼠等);感染源从白色念珠菌转向非白念珠菌(如近平滑念珠菌、光滑念珠菌等);感染方式从局部口腔-消化道感染逐步转变为血源性深部多器官组织感染.特定模型的建立更深入地探讨了宿主-念珠菌感染源之间相互的免疫机制.细胞介导的免疫反应在宿主抗念珠菌感染免疫反应中占主导,吞噬细胞直接杀伤真菌;细胞分化为Th1和Th2型细胞,分泌相关细胞因子进行免疫调控.体液免疫中一些保护性抗体也具有一定的保护作用.