TNF-{alpha} regulates IL-4-induced Fc{varepsilon}RII/CD23 gene expression and soluble Fc{varepsilon}RII release by human monocytes

We examined the regulatory effects of TNF- on IL-4-induced geneexpression of the low-affinity receptor for IgE (FcRII/CD23)in human monocytes and IL-4-induced soluble FcRII (sFcRII) releasefrom monocytes. IL-4-induced FcRII expression on the surfaceof monocytes was reduced by TNF- as early as 1 day after cultureand the effect of TNF- increased with prolonged culture. Thepresent analysis was designed to examine whether or not TNF-could suppress IL-4-induced FcRII mRNA expression and enhancedIL-4-induced sFcRII release. The addition of TNF- to monocytecultures with IL-4 significantly reduced FcRII expression onthe surface of monocytes and significantly increased sFcRIIrelease from monocytes. Over time, there was an inverse relationshipbetween the disappearance of cell surface FcRII and the appearanceof sFcRII in culture supernatants. FcRII mRNA expression inmonocytes cultured with IL-4 was not affected by TNF- when examinedat 6 h after cultivation. When the cells were cultured withTNF- for more than 24 h, however, TNF- down-regulated IL-4-inducedFcRII mRNA levels. This correlated with the kinetics of down-regulationof IL-4-induced FCRII expression on the surface of monocytesby TNF-. These results suggest that TNF-dependent reductionof IL-4-;induced FcRII expression on the surface of monocytesresulted, at least in part, from the suppression of FcRII mRNAexpression and the enhancement of sFcRII release.     

The level of tumor necrosis factor-{alpha} producing cells in the spinal cord correlates with the degree of Theiler's murine encephalomyelitis virus-induced demyelinating disease

The levels of tumor necrosis factor (TNF)- producing cells wereanalyzed in mice with Theller's murine encephalomyelitis virus-induceddemyelinating disease (TMEV-IDD). Using an ELISPOT assay, wedemonstrate an increase in TNF- producing cells in the spinalcords of TMEV-infected SJL/J mice, especially at an active diseasestage. The numbers of TNF- producing cells were extremely highin susceptible SJL/J mice compared with the numbers in resistantBALB/c and C57BL/6 mice. TNF- producing cells were also immunohistochemicallyidentified in active lesions of TMEV-IDD at acute as well aschronic stages. The percentage of TNF- producing cells comparedwith the total number of cells isolated from spinal cords washigher in TMEV-infected SJL/J mice than resistant BALB/c andC57BL/6 mice. Correspondingly, the level of TNF- was much higherin the culture supernatants of both infiltrating cells in thespinal cords and spleen cells from clinically affected animalsthan that from similarly treated resistant mice. Treatment ofvirus-infected mice with a mAb specific for TNF- at the beginningof the onset of disease suppressed the development of the demyelinatingdisease. These findings suggest that TNF- may play an importantrole in the pathogenicity of TMEV-IDD.     

Nickel and skin irritants up-regulate tumor necrosis factor-{alpha} mRNA in keratinocytes by different but potentially synergistic mechanisms

A critical role of tumor necrosis factor (TNF)- in irritantcontact dermatitis and in the challenge phase of allergic contactdermatitis has recently been demonstrated in vivo. As in situhybridization studies have indicated that keratinocytes werethe cellular source of TNF- in these reactions, we studied themechanisms of TNF- mRNA induction in keratinocytes by agentsthat induce contact dermatitis. Murine Ia^–;/CD3^–epidermal cells were stimulated with phorbol myristate acetate(PMA), dimethylsulfoxide (DMSO), sodium dodecyl sulfate (SDS)and NiSO₄, all of which up-regulated epidermal cell TNF- mRNAproduction. In contrast, trinitrobenzenesulfonic acid and trinitrochlorobenzenedid not significantly up-regulate TNF- mRNA. These results wereconfirmed with murine keratinocyte cell lines. In keratinocytestransfected with a chloramphenicol acetyltransferase constructcontaining the –1059 to +138 base pair TNF- promoter,increased promoter activity was observed upon stimulation withPMA and DMSO. In addition, PMA stimulation did not affect thestability of TNF- mRNA. The PMA- but also the DMSO- and SDSinducedup-regulation of TNF- mRNA was abolished by an inhibitor ofprotein kinase C (PKC). In contrast, NISO4 up-regulated TNF-mRNA by a PKC-independent mechanism, did not increase TNF- promoteractivity, but markedly increased the stability of the TNF- mRNA.Co-stimulation with PMA and NISO₄ induced a marked increasein TNF-a mRNA over that obtained with each agent alone. Thus,whereas PKC-dependent irritants act by up-regulating TNF- promoteractivity, nickel acts via post-transcrlptional regulation. Ourresults, also establish that some irritants and irritant sensitizersdirectly induce TNF- in keratinocytes without intermediate Langerhanscell derived signals.     

Soluble human high-affinity receptor for IgE abrogates the IgE-mediated allergic reaction

The high-affinity receptor for IgE (FcRI) has a tetrameric structurecomposed of one, one ß, and two disulfide-linked subunits, of which the subunit binds IgE with high affinity.A recombinant soluble form of the ectodomain of the human FcRIsubunit (rsFcRI) was recently generated by gene engineeringand was verified to bind IgE with an affinity as high as thatof native FcRI on the cell surface. rsFcRI was prepared on alarge scale in order to analyze its biological function. rsFcRIcompletely inhibited IgE binding to the cell surface, resultingin abrogation of the chemical mediator release from RBL-2H3cells. Furthermore it completely abolished the passive cutaneousanaphylaxis (PCA) response by trapping IgE specifically whenitwas administered into rats prior to IgE sensltizatlon. Evenafter IgE sensitizatlon, treatment of rsFcRI substantially reducedthe PCA response. It was finally shown that rsFcRI inhibitedIgE binding to human peripheral blood basophils and the histaminerelease from them. In this paper we address the ability of rsFcRIto specifically prevent the IgE-mediated allergic reaction.     

Double-stranded RNA and bacterial lipopolysaccharide enhance sensitivit to TNF-{alpha}-mediated cell death

The effect of double-stranded RNA (dsRNA) and bacterial lipopolysaccharideon the sensitivity to tumor necrosis factor (TNF)--medlatedcell death was studied In an In vitro system. Since secretionof TNF- Is a part of the early host response to viral and bacterialinfection, we examined whether mimicking the Infection withviral and bacterial products could affect the response of cellsto TNF-. Incubation of WEHI 164 fibrosarcoma cells with dsRNAor lipopolysaccharide (LPS) significantly increased their sensitivityto TNF--mediated lysis and to TNF-secreting inflammatory T cell-mediatedlysis. Thus, these products could induce Increased sensitivityto TNF- In cells In an inflammatory focus, possibly contributingto selective elimination of Infected but not healthy cells bythis non-specific cytokine. Additionally, our data show thatboth dsRNA and LPS, as well as TNF- Itself, rapidly Induce nuclearfactor-xB (NF-*B), a DNA-bindlng protein Implicated In regulationof gene expression. We suggest that NF-xB could regulate genescrucial for the induction of cell death by TNF-.     

Growth inhibition of Mycobacterium bovis by IFN-{gamma} stimulated macrophages: regulation by endogenous tumor necrosis factor-{alpha} and by IL-10

Murine bone marrow-derived macrophages (BMM) are able to inhibitthe intracellular growth of Mycobacterium bovis and Mycobacteriumtuberculosis H37Rv after activation with recomblnant (r) IFNand growth inhibition is mediated by reactive nitrogen intermediates(RNI) derived from L-arglnlne. We now demonstrate that tumornecrosis factor (TNF)- acts as an endogenous cofactor in theinduction of mycobacterial growth inhibition. TNF- was producedby BMM stimulated with rlFN- and infected with mycobacterla,and a specific antlserum to TNF- Inhibited rlFN--lnduced productionof RNI as well as growth inhibition of M. bovis. IL-10, a cytokinewhich suppresses antlmycobacterial macrophage functions, wasalso produced by BMM activated with hFN- and infected with M.bovis. IFN--induced production of TNF- and of reactive nitrogenintermediates as well as mycobacterial growth inhibition wereinhibited by exogenous IL-10, but only when given prior to IFN-stimulation. We conclude that the outcome of mycobacterial infectionis regulated by a coordinate interplay between IFN-, TNF- andIL-10.     

Antibody response elicited by T-dependent and T-independent antigens in gene targeted {kappa}-deficient mice

Animal models substantially contribute to the understandingof the pathogenesis of various human diseases, including thoseassociated with genetic defects. Our study investigated thecharacteristics of antibody responses elicited by T-dependentand T-independent antigens in mice rendered k-deficterrt bytargeted deletion of the J_kC_k gene segments. It is known thatin normal murine species the k repertoire dominates the antibodyrepertoire (k/ratio = 95:5). Our results indicate that the kgene deletion causes the alternative usage of 1 (93%) and 2(7%) light chains, confirming previous studies demonstratingthat in k-deficlent mice all B cells express IG receptors. Theanti-trinitrophenylbenzene (TUP) response in K–/–mice was compensated for by 1 and 2 bearing Igs. However, isoelectricfocusing analysis of anti-TNP antibodies showed a considerablymore restricted pattern of anti-TNP antibodies in K–/–as compared with antibodies in normal mice. No major differenceswere observed in the affinity for the hapten of or1 or 2 mAbsobtained from 129/Sv and K–/– mice. Furthermore,1 and 2 chains can reconstitute the expression of an Idiotype(460ld) borne on anti-TNP antibodies. The 460ld was detectedboth in polyclonal and monoclonal anti-TNP antibodies obtainedfrom K–/– mice. Our results clearly showed thatthe anti-TNP repertoire is compensated by the repertoire eventhough the latter is clonally restricted in K–/–mice.     

Ligand-induced autoregulation of IL-2 receptor {alpha} chain expression in murine T cell lines

The IL-2 receptor (IL-2R) is composed of three chains a, ßand . In mice, contrary to the human system, we have previouslydemonstrated that the IL-2Rß complex does not bindIL-2. Therefore, mouse IL-2 response is completely dependenton the expression of the IL-2R gene product. T cell clones expressingmouse IL-2Rß and the human IL-2R transgene have beenstudied. When cells are grown in IL-4, mouse IL-2R is not expressed.However, exposure to IL-2 leads to the expression of the endogenousmurine IL-2R subunit. The T cell line expressing mouse IL-2Rand human IL-2Rß can grow in IL-2 but does not expressendogenous murine IL-2 R. Transfection of these cells with thehuman IL-2R gene restores the capacity to induce murine IL-2R.This result demonstrates that IL-2-IL-2R interactions are requiredfor induction of IL-2R. The kinetics of induction and deinductionof murine IL-2R have been studied using clone 18.III. From negativecells, expression of murine IL-2R is a very slow phenomenon.From cells fully expressing IL-2R, deinduction is a two-stepprocess: after a rapid decrease of IL-2R the cells continueto express, for a long period of time, basal levels of murineIL-2R. When cells expressing basal levels of IL-2R are exposedto IL-2, induction of IL-2R is a very rapid phenomenon. Theautoregulatory loop formed by IL-2-IL-2R therefore displaysdifferent levels of functioning.     

Re-evaluation of the probabilities for productive rearrangements on the {kappa} and{lambda}loci

V-J rearrangements at Ig light chain (IgL) genes occur in restingsmall pre-B cells. In the absence of cell division, the probabilityof productive and rearrangements is proportional to the outputof ⁺ B and ⁺ B cells in bone marrow. The kinetics and probabilityof productive or rearrangements was assessed in three groupsof mice carrying two (wild-type), one or no intact Ig gene,and the following conclusion are drawn, and rearrangementsoccur independently at different kinetics, and rearrangementsare initiated at a time when rearrangements are stopping. Theprobability of productive and rearrangements per chromosomeis calculated to be –60 and –20% respectively. Thus,a gene can attempt rearrangements up to three times per chromosomeduring B cell development. These findings explain that the observedratio of ⁺ B/⁺ B cell production in wild-type mice is 95/5.     

Phenotypic and functional properties of murine {gamma}{delta} T cell clones derived from malaria immunized, {alpha}{beta} T cell-deficient mice

Six murine T cell clones expressing TCR were generated frommalaria immunized, ß T celldeficient mice. Phenotypiccharacterization of these clones has revealed that, in contrastto conventional ß T cells, there is a considerabledegree of heterogeneity among these clones with regard to theirsurface markers and their lymphokine profile. One clone wasfound to display significant anti-parasite activity in vivoupon adoptive transfer. We attempted to determine whether theprotective clone differs in one or more key characteristicsfrom the non-protective clones. Although no obvious patternpeculiar to the protective clone was observed, it appears thatmore than one parameter may, in combination, define a distinctprotective phenotype, and thus explain the functional differencebetween the protective and non-protective clones.     

Involvement of {alpha}1 and {alpha}4 integrins in gut mucosal injury of graft-versus-host disease

We have investigated the involvement of adhesion molecules inthe lymphocyte infiltration associated with acute intestinalgraft-versus-host disease (GVHD) induced by injection of C3Hlymph node cells into irradiated (C3H x DBA/2)F₁ mice. Firstwe analyzed the expression profile of adhesion molecules including1, 2, 4, 5, 6, L and ß7 integrins, CD44 and L-selectinof lymphocytes from lymph nodes and gut mucosa in normal mice.In normal mice, intraepithelial lymphocytes (IEL) and laminapropria lymphocytes (LPL) uniquely showed increased expressionof 1, 2 and ß7 integrins, and decreased expressionof L-selectin compared with that of lymphocytes of the lymphnodes and Peyer's patches. In mice with GVHD, IEL and LPL ofdonor lymph node cells origin underwent phenotyplc changes characterizedby the increased expression of 1, L and ß7 integrins,and the loss of L-selectin. The expression profile of adhesionmolecules on IEL and LPL of GVHD mice resembled that of normalmice except for the lack of 2 integrin. Treatment of GVHD micewith anti-1,-4 or-ß7 integrin antibody alone partiallyprevented the mucosal pathology of intestinal GVHD, whereasonly mice treated with anti-1 showed reduced donor lymphocyticinfiltration into the intestinal mucosa. In contrast, treatmentwith anti-L or anti-CD44 antibody did not affect the intestinalGVHD. Furthermore, dual blockade of both 1 and 4 integrins completelyinhibited the mucosal pathology and donor lymphocyte infiltrationof intestinal GVHD. These results indicate that 1 and 4 integrinsplay an important role in the pathology of intestinal GVHD.     

Requirements for cell surface expression of the human TCR/CD3 complex in non-T cells

The T-cell antigen receptor (TCR) consists of a glycoproteinheterodimer (/ß or /) which is non-covalently associatedwith at least four or five invariant polypeptides (CD3 ,,, ;and ). In T-cell variants lacking TCR ,ß or , it hasbeen shown that incomplete TCR/CD3 complexes are retained withinthe cell. To examine requirements for cell surface expressionof TCR/CD3, we transfected COS monkey kidney cells with cDNAsencoding TCR ,ß and CD3 , , and . We report thatcell surface appearance of TCR/CD3 on COS cells requires coordinateexpression of all six proteins. In the absence of the chain,subcomplexes comprising from two to five chains were readilydemonstrable In COS cells, but they failed to reach the cellsurface or to acquire N-llnked oligosaccharide side chains indicatingfailure to reach the medial Golgl. Pulse-chase, metabolic labellingof transfected COS cells showed that three chains (CD3 , CD3, and ) were stable while three (TCR , TCR ß and CD3) were rapidly degraded. In two- and three-chain co-transfectionsspecific intracellular subcomplexes were formed between TCR and CD3 , TCR and CD3 , or TCR ß and CD3 . Binarysubcomplexes having at least one stable chain (CD3 –TCRß) were stable while one formed by two unstable chains(TCR –CD3 ) was still degraded. Assembly of the TCR/CD3complex in COS cells thus appears centered around the metabolicallystable CD3 and CD3 proteins. Site-specific mutations of thenegatively-charged transmembrane amino acid of residues of theCD3 chains to alanines served to either abolish (for TCR –CD3 and TCR ß–CD3 ) or diminish (for TCR –CD3) these TCR-CD3 interactions. These mutations had no effect,however, on CD3–CD3 Interactions or upon synthesis, metabolism,or intracellular distributions of the CD3 proteins. The transmembranedomains of CD3 , , and thus appear to play a major role inassociations of CD3 with TCR chains.     

Composition of TCR-CD3 complex in human intestinal intraepithelial lymphocytes: lack of Fc{varepsilon}Rl{gamma} chain

Human intestinal intraepithelial lymphocytes (DEL) are a uniquepopulation of predominantly CD8ß⁺ TCRß⁺lymphocytes and, to a lesser extent, TCR⁺ lymphocytes that proliferatepoorly to anti-CD3 mitogenic signals but display significantcytolytic activity. Studies in mouse model systems have shownthat the chain of the high-CD3 affinity receptor for IgE (FcRl)may substitute for the chain in the TCR-CD3 complex of iIEL.This has suggested that the functional properties of these cellsmay be associated with an altered composition of the TCR-CD3complex. We therefore analyzed the TCR-CD3 complex of normalhuman iIEL. One-and two-dimensional non-reducing/reducing SDS-PAGEanalysis of CD3, CD3, CD3, and FcRr chain immunopreclpitatesof cell surface radiolabeled proteins with subunit-specificantibodies revealed a TCR-CD3 complex without associated FcRrchains. Thus, normal human NEL contain a TCR-CD3 complex thatconsists predominantly of , homodimers in association with theß TCR and CD3, and , similar to the majority of peripherallymphocytes. This indicates that the distinct properties ofhuman DEL are not associated with substitutions of the FcRlchain in the TCR-CD3 complex.     

Peripheral lymphoid development and function in TCR mutant mice

We describe the development and function of the peripheral lymphoidsystem of mutant mice rendered deficient in either ßor T cells via targeting of TCR genes In embryonic stem cells.In the spleen of ß T cell-deficient mice, T cellsdo not compensate in numbers for the lack of ß Tcells, but B cells do. ß T cell-deficient mice areunable to mount an antibody response to ovalbumln and do notreject skin allografts. Natural killer cell function is notimpaired in any of the mutant mice. TCR mutant mice will proveuseful in dissecting differential functions of ßand T cells in vivo.