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Query: UMLS:C0026764 (
multiple myeloma
)
36,148
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
We constructed a recombinant gene encoding an immunoglobulin (Ig) heavy chain consisting of the variable region from the phosphorylcholine (PC)-specific secreting
myeloma
MOPC167 and the epsilon constant region from SJL mice. This gene, cloned into the shuttle vector pSV2gpt, was transfected into J558L
myeloma
cells, and stable transformants that expressed the epsilon gene were cloned. The
IgE
heavy chain in these transformants is associated with the endogenous lambda light chain and is secreted as an intact
IgE
molecule. However, the secreted
IgE
does not bind to PC conjugated to bovine serum albumin (PC-BSA). The MOPC167 kappa chain gene was cloned into the shuttle vector pSV2neo and was transfected into the epsilon heavy-chain transformant. Stable transformants were cloned that expressed both the epsilon heavy chain and the kappa light chain.
IgE
secreted from such a transformant was shown to bind to PC-BSA. Both types of secreted recombinant
IgE
bound to rat basophilic leukemia (RBL) cells, but only the
IgE
produced by the cell line transformed with the MOPC167 kappa gene could be cross-linked with PC-BSA to cause serotonin release.
...
PMID:Expression of a recombinant murine IgE in transfected myeloma cells. 243 Oct 59
In an attempt to block the interactions between
IgE
and its receptor on mast cells (Fc epsilon R), we have established anti-Fc epsilon R monoclonal antibodies (mAb) by fusion of
myeloma
cells with mouse splenocytes immunized with irradiated rat basophilic leukemia (RBL) cells. Two anti-Fc epsilon R mAb were obtained (denoted 4.7 and 5.14) that could specifically bind to RBL and mast cells. This binding could be inhibited by
IgE
. The mAb and their F(ab')2 fragments inhibited 125I-
IgE
binding to RBL cell and triggered cell degranulation. The Fab' fragments, on the other hand, could only inhibit
IgE
binding but did not stimulate cell degranulation. Furthermore, these monovalent fragments inhibited RBL and mast cell degranulation induced by
IgE
-antigen complexes both in vitro and in vivo in the passive cutaneous anaphylaxis reaction. The number of mAb 4.7 and 5.14 molecules bound per RBL cells was similar to that of
IgE
; nevertheless, mAb 4.7 and 5.14 recognized different epitopes on the
IgE
receptor. Immunoprecipitation and immunoblotting analysis demonstrated that the mAb reacted with the alpha-subunit of the Fc epsilon R. Our findings establish the anti-Fc epsilon R mAb as a useful reagent for the isolation and characterization of the Fc epsilon R's alpha-subunit and the monomeric (Fab') for blocking the
IgE
-Fc epsilon R interactions.
...
PMID:Monoclonal antibodies specific to the alpha-subunit of the mast cell's Fc epsilon R block IgE binding and trigger histamine release. 243 3
Nasal lavage fluids from unstimulated individuals contain a histamine-releasing factor (HRF) similar to those which we have previously described from macrophages, platelets, and from blister fluids obtained during the late cutaneous reaction. The nasal HRF was partially purified by ion-exchange chromatography and gel filtration. Although some m.w. heterogeneity was observed, the majority of the HRF eluted at an apparent m.w. range of 15,000 to 30,000. This partially purified HRF induced histamine release from basophils of certain individuals. Histamine release occurred via a mechanism which is
IgE
-dependent in that: basophils desensitized by exposure to anti-
IgE
in the absence of calcium no longer respond to HRF, and desensitization with HRF reduces responsiveness to anti-
IgE
; and removal of
IgE
from the basophil surface by using lactic acid renders cells unresponsive to HRF. We have further defined this
IgE
dependence and have shown that the reason that only selected basophil donors respond to HRF is due to a previously unrecognized, functional heterogeneity of
IgE
. Thus, passive sensitization using sera from responders restored the responsiveness of acid-stripped basophils and conferred responsiveness to basophils of a nonresponder with naturally unoccupied
IgE
receptors. Sera from nonresponders failed to do this even though similar numbers of
IgE
molecules were put onto the basophil surface in each case. This property of responder sera was due to
IgE
because both heating sera at 56 degrees C for 2 hr and passage of sera over anti-
IgE
-Sepharose (which removes greater than 90% of the
IgE
) markedly reduced the ability of sera to induce responsiveness, and because an excess of either purified
IgE
myeloma
or purified penicillin-specific
IgE
antibody from a nonresponder competitively inhibited the ability of
IgE
from responder sera to induce responsiveness to HRF. We conclude that nasal lavage fluids contain an HRF which induces basophil histamine release in a specific,
IgE
-dependent fashion but only from individuals with the appropriate type of
IgE
. Because we have shown that basophils are recruited into the nose during the late-phase reaction, we suggest that nasal HRF may induce these cells to release histamine and other mediators which could contribute to the symptomatology of the late-phase reaction.
...
PMID:Studies of IgE-dependent histamine releasing factors: heterogeneity of IgE. 243 89
IgE
-anti-
IgE
complexes were formed by preincubation of a human
myeloma
IgE
with a monoclonal anti-human
IgE
antibody at different concentrations. Binding of
IgE
onto the anti-
IgE
inhibited the histamine release capacity of anti-
IgE
from basophils. The
IgE
cell-binding capacity was altered by the
IgE
/anti-
IgE
ratio in the preincubation buffer. Heating of the complexes gave a partial recovery of the anti-
IgE
degranulation capacity, suggesting that the monoclonal anti-
IgE
is specific for an epitope present on the D epsilon 2 domain.
...
PMID:Monoclonal anti-human IgE: histamine release capacity and effect on in vitro sensitization of human basophils. 244 Feb 72
Leucocytes from human peripheral blood were acid eluted and sensitized in vitro with increasing concentrations of radiolabelled
myeloma
IgE
. This sensitization step was performed with or without 30%
IgE
depleted serum. After the
IgE
binding, cells were washed and submitted to a challenge with monoclonal anti-
IgE
for the determination of the cellular sensitivity and reactivity in a histamine release assay. A sample of each of the sensitized cells was analyzed for its radioactivity and the number of basophils quantified, thus allowing the determination of the mean number of
IgE
molecules per basophil. Raising the
IgE
concentrations in the sensitization procedure led to an increase of the
IgE
on the basophil membrane, and to a concomitant elevation of the cell sensitivity. The presence of serum during the binding of
IgE
onto the cells lowers slightly the binding of
IgE
to the basophils but decreases strongly the cellular reactivity.
...
PMID:Basophil sensitivity and reactivity to monoclonal anti-human IgE after in vitro sensitization with human myeloma IgE. 244 Feb 73
An
IgE
immunotoxin consisting of rat
IgE
myeloma
protein, IR 162, conjugated via the heterobifunctional linking agent N-succinimidyl-3-(2-pyridyldithio)propionate to intact ricin was synthesized and evaluated. The capacity of this
IgE
-immunotoxin to bind to rat basophilic leukemia cells (RBL cells) and to inhibit RBL cell incorporation of [3H]leucine was assessed. The
IgE
-intact ricin conjugate sensitized RBL cells for histamine release after treatment with anti-
IgE
with a time-course of sensitization and dose-response equivalent to native
IgE
. Intact ricin and
IgE
-intact ricin were both cytotoxic to RBL cells as assessed by [3H]leucine incorporation. Lactose (50 mM) competed with intact ricin binding and toxicity such that more than 100 ng/ml ricin (8 times its IC50 in the absence of lactose) was required for ricin to kill RBL cells in the presence of lactose. Lactose (50 mM) was not able to fully inhibit 1-100 ng/ml
IgE
-ricin immunotoxin killing of RBL cells. Saturation of RBL cell
IgE
receptors by preincubation with
IgE
totally inhibited
IgE
-intact ricin-induced toxicity, in the presence of lactose, indicating that toxicity required
IgE
Fc receptor binding.
...
PMID:IgE-immunotoxins. I. IgE-intact ricin. 244 11
An IgG type of antibody directed against
IgE
has been studied in serum from healthy and allergic individuals. The technique used is based on a solid phase paper radioimmunoassay in which the discs were sensitized with purified
IgE
myeloma
. After incubation with patients' serum, human IgG labeled with iodine 125 was added. The anti-
IgE
antibodies were partially blocked by endogenous
IgE
in the serum and heating the serum samples at 56 degrees C disrupted the immune complexes (ie, IgG-aIgE:
IgE
), thereby increasing the detectable levels of IgG anti-
IgE
. The specificity of anti-
IgE
autoantibody was confirmed by both competitive inhibition and absorption experiments, using IgG, IgM, IgA,
IgE
, and rabbit anti-human IgG. Significantly raised levels of anti-
IgE
autoantibody were found in patients suffering from atopic disorders in comparison to the controls. These observations may suggest that the anti-
IgE
autoantibody could play a certain role in the modulation of
IgE
-mediated immune system and the pathogenesis of atopic diseases.
...
PMID:IgG autoantibody to IgE in atopic patients. 244 12
Immunotoxins--toxins covalently conjugated to specific antibodies--have been studied as possible agents in the treatment of cancer. The avid binding of
IgE
antibodies to FcR on mast cells and basophils suggested the possible use of an
IgE
-immunotoxin in the treatment of malignant mastocytosis or as a method to generate mast cell-depleted animals for study. To this end, the effect of a covalent conjugate of rat
myeloma
IgE
and ricin A chain on rat cutaneous mast cells was examined in vivo.
IgE
-ricin A chain was capable of binding to and sensitizing cutaneous mast cells in vivo as indicated by a bluing response to intracutaneous anti-ricin A chain.
IgE
-ricin A chain, given either as a single dose or, even more effectively, as two split doses, significantly reduced cutaneous histamine content for 6 to 8 days. Neither a mixture of
IgE
and ricin A chain that were not conjugated nor the induction of cutaneous mast cell degranulation with anti-
IgE
affected cutaneous histamine levels. Therefore,
IgE
-ricin A chain produces a prolonged depletion of cutaneous histamine levels.
...
PMID:IgE immunotoxins. Effect of an IgE-ricin A chain conjugate on rat skin histamine content. 244 77
The effect of KB-2413 on
IgE
-mediated histamine and LTC4 release from leukocytes obtained from asthmatic patients who were sensitive to mites, and from human lung tissues passively sensitized with
IgE
myeloma
serum was studied. KB-2413 inhibited the
IgE
-mediated chemical mediator release concentration dependently at a range of 10(-4) to 3 x 10(-3) M. KB-2413 did not enhance histamine release at a higher concentration unlike ketotifen. These findings suggest that the inhibitory effect of KB-2413 on the release of chemical mediators contributes to the anti-allergic activity of this compound.
...
PMID:Inhibition of chemical mediator release from human leukocytes and lung in vitro by a novel antiallergic agent, KB-2413. 244 88
Receptors for
IgE
(Fc epsilon R) on rat bone marrow-derived macrophages (BMDM phi) were demonstrated by a rosette assay employing trinitrophenyl-coated ox erythrocytes (EoTNP) sensitized with mouse
IgE
anti-dinitrophenyl monoclonal antibody (EoTNP-
IgE
). Virtually all BMDM phi emerging from bone marrow cells cultured for 1 week in the presence of mouse L929 cell supernatant, with partially purified murine CSF-1 or recombinant murine GM-CSF, formed
IgE
rosettes. To study the effect of interferons (IFNs) on Fc epsilon R expression, 1-week-old rat BMDM phi were incubated with murine recombinant IFN-gamma, purified IFN-alpha or IFN-beta, and were tested for their capacity to bind and ingest EoTNP sensitized suboptimally with
IgE
. A marked increase in the percentage of cells forming
IgE
rosettes or phagocytosing EoTNP-
IgE
was noted after 8-72 hr incubation of BMDM phi with 0.1-1000 U/ml of IFNs. At similar concentrations IFN-gamma and IFN-beta triggered EoTNP-
IgE
binding or ingestion more efficiently than IFN-alpha. The enhancing effect was blocked by the respective anti-IFN antibodies, cycloheximide or actinomycin D but not by mitomycin C. The
IgE
rosette formation and
IgE
-mediated phagocytosis were dose-dependently inhibited by native rat
IgE
but not by heat-denaturated
IgE
myeloma
protein IR162 or monomeric rabbit IgG. Our results demonstrate that rat BMDM phi express constitutively Fc epsilon R, and that murine IFNs augment Fc epsilon R-mediated binding and ingestion in a time- and dose-dependent manner. This effect probably reflects an increase in the number of Fc epsilon R per cell, as a result of de novo synthesis of Fc epsilon R.
...
PMID:Augmentation of IgE receptor expression and IgE receptor-mediated phagocytosis of rat bone marrow-derived macrophages by murine interferons. 245 Aug 38
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