Your search keyword '"Cell Adhesion Molecules isolation & purification"' showing total 11 results

1. Quality of recombinant protein determines the amount of autoreactivity detected against the tumor-associated epithelial cell adhesion molecule antigen: low frequency of antibodies against the natural protein.

Author

Schmetzer O, Moldenhauer G, Riesenberg R, Pires JR, Schlag P, and Pezzutto A

Subjects

Animals, Antibodies, Neoplasm biosynthesis, Antibodies, Neoplasm blood, Antigens, Neoplasm isolation & purification, Autoantibodies biosynthesis, Autoantigens isolation & purification, Baculoviridae genetics, Baculoviridae immunology, Biomarkers, Tumor isolation & purification, Biomarkers, Tumor standards, Breast Neoplasms immunology, Cell Adhesion Molecules isolation & purification, Cell Adhesion Molecules standards, Cell Line, Colorectal Neoplasms immunology, Dose-Response Relationship, Immunologic, Drosophila melanogaster genetics, Drosophila melanogaster immunology, Drug Contamination, Epithelial Cell Adhesion Molecule, Humans, Immunoglobulin G biosynthesis, Immunoglobulin G blood, Protein Denaturation, Protein Folding, Quality Control, Recombinant Proteins isolation & purification, Stomach Neoplasms immunology, Antigens, Neoplasm immunology, Autoantibodies blood, Autoantigens immunology, Biomarkers, Tumor immunology, Cell Adhesion Molecules immunology, Recombinant Proteins immunology, Recombinant Proteins standards

Abstract

The human epithelial cell adhesion molecule (EpCAM) is expressed on normal epithelial cells and is overexpressed in most carcinomas. EpCAM-targeted immunotherapy has been tried in several clinical studies. High titers of autoantibodies against EpCAM have been reported by different authors. We have generated large amounts of purified protein in S2 Drosophila cells (S2-EpCAM) with a purity of >96%. In contrast, the protein produced in baculovirus-dependent systems (baculo-EpCAM) that has been used in previous studies shows a purity of 79%. (1)H nuclear magnetic resonance spectrum of S2-EpCAM is typical of folded protein, whereas the baculo-EpCAM sample shows a spectrum corresponding to a partially unfolded protein. Using S2-EpCAM, denatured S2-EpCAM, and baculo-EpCAM, we measured EpCAM Abs of different isotypes in the serum of healthy controls and cancer patients. We found Ab titers against EpCAM in a much lower percentage of sera as published previously, and support the hypothesis that Ab reactivity in some published studies might be due to reactivity against denatured protein, to contaminating proteins in the baculovirus preparations, and to reactivity with BSA. Tetanus toxoid-reactive IgG Abs are present in 1000-fold higher titers compared with EpCAM-reactive Abs. Only IgA Abs were found in higher proportions and in higher concentrations than tetanus toxoid-specific Abs. Our study shows that EpCAM only rarely induces autoantibodies against native protein and emphasizes the importance of using extremely purified Ag preparations when evaluating Abs against tumor-associated Ags.

Published

2005

2. Characterization of a pattern recognition protein, a masquerade-like protein, in the freshwater crayfish Pacifastacus leniusculus.

Author

Lee SY and Söderhäll K

Subjects

Amino Acid Sequence, Animals, Astacoidea enzymology, Astacoidea microbiology, Bacterial Adhesion, Cell Adhesion Molecules isolation & purification, Cell Adhesion Molecules metabolism, Cell Adhesion Molecules physiology, Escherichia coli physiology, Hemocytes chemistry, Hemocytes enzymology, Immunoblotting, Molecular Sequence Data, Protein Binding, Serine Endopeptidases isolation & purification, Serine Endopeptidases metabolism, Serine Endopeptidases physiology, Astacoidea chemistry, Cell Adhesion Molecules chemistry, Drosophila Proteins, Insect Proteins chemistry, Pattern Recognition, Visual physiology, Serine Endopeptidases chemistry

Abstract

A multifunctional masquerade-like protein has been isolated, purified, and characterized from hemocytes of the freshwater crayfish, Pacifastacus leniusculus. It was isolated by its Escherichia coli binding property, and it binds to formaldehyde-treated Gram-negative bacteria as well as to yeast, Saccharomyces cerevisiae, whereas it does not bind to formaldehyde-fixed Gram-positive bacteria. The intact masquerade (mas)-like protein is present in crayfish hemocytes as a heterodimer composed of two subunits with molecular masses of 134 and 129 kDa. Under reducing conditions the molecular masses of the intact proteins are not changed. After binding to bacteria or yeast cell walls, the mas-like protein is processed by a proteolytic enzyme. The 134 kDa of the processed protein yields four subunits of 65, 47, 33, and 29 kDa, and the 129-kDa protein results in four subunits of 63, 47, 33, and 29 kDa in 10% SDS-PAGE under reducing conditions. The 33-kDa protein could be purified by immunoaffinity chromatography using an Ab to the C-terminal part of the mas-like protein. This subunit of the mas-like protein has cell adhesion activity, whereas the two intact proteins, 134 and 129 kDa, have binding activity to LPSs, glucans, Gram-negative bacteria, and yeast. E. coli coated with the mas-like protein were more rapidly cleared in crayfish than only E. coli, suggesting this protein is an opsonin. Therefore, the cell adhesion and opsonic activities of the mas-like protein suggest that it plays a role as an innate immune protein.

Published

2001

3. A novel glycosylphosphatidyl inositol-anchored protein on human leukocytes: a possible role for regulation of neutrophil adherence and migration.

Author

Suzuki K, Watanabe T, Sakurai S, Ohtake K, Kinoshita T, Araki A, Fujita T, Takei H, Takeda Y, Sato Y, Yamashita T, Araki Y, and Sendo F

Subjects

Actins blood, Adjuvants, Immunologic physiology, Amidohydrolases, Amino Acid Sequence, Animals, Antibodies, Monoclonal blood, Antibodies, Monoclonal physiology, Base Sequence, Binding Sites, Antibody, Binding, Competitive immunology, CD18 Antigens blood, Cell Adhesion immunology, Cell Adhesion Molecules genetics, Cell Adhesion Molecules immunology, Complement C3b metabolism, GPI-Linked Proteins, Humans, Hydrolases, Membrane Glycoproteins genetics, Membrane Glycoproteins immunology, Mice, Molecular Sequence Data, Sequence Homology, Amino Acid, Cell Adhesion Molecules isolation & purification, Cell Movement immunology, Glycosylphosphatidylinositols blood, Membrane Glycoproteins blood, Neutrophils immunology

Abstract

We report here a novel glycosylphosphatidyl-inositol (GPI)-anchored glycoprotein on human leukocytes. Treatment of neutrophils with a mAb (3H9) to this molecule sequentially up-regulates and down-regulates beta2 integrin-dependent adhesion of these cells as well as their transendothelial migration in vitro. In addition, this mAb simultaneously modulates the avidity of beta2 integrin for its ligand, iC3b, with kinetics similar to those observed in 3H9 modulation of neutrophil adherence. This mAb also induces beta2 integrin-dependent cytoskeletal remodeling. This novel GPI-anchored protein (GPI-80) is highly homologous with Vanin-1, a recently reported GPI-anchored protein that is expressed on perivascular thymic stromal cells and is involved in thymus homing in mice. The finding that both GPI-80 and Vanin-1 are 40% homologous with human biotinidase suggests the existence of a biotinidase superfamily of molecules that may be involved in the regulation of leukocyte trafficking.

Published

1999

4. Isolation, structural characterization, and chromosomal mapping of the mouse vascular adhesion protein-1 gene and promoter.

Author

Bono P, Salmi M, Smith DJ, Leppänen I, Horelli-Kuitunen N, Palotie A, and Jalkanen S

Subjects

Amine Oxidase (Copper-Containing) isolation & purification, Amino Acid Sequence, Animals, Base Sequence, Blotting, Southern, Cell Adhesion Molecules isolation & purification, Codon, Initiator, Exons, Genome, Introns, Mice, Mice, Inbred Strains, Molecular Sequence Data, Regulatory Sequences, Nucleic Acid, Sequence Analysis, DNA, Sialoglycoproteins chemistry, Sialoglycoproteins genetics, Sialoglycoproteins isolation & purification, Transcription, Genetic, Amine Oxidase (Copper-Containing) chemistry, Amine Oxidase (Copper-Containing) genetics, Cell Adhesion Molecules chemistry, Cell Adhesion Molecules genetics, Chromosome Mapping, Promoter Regions, Genetic

Abstract

Vascular adhesion protein-1 (VAP-1) is an endothelial cell adhesion molecule which mediates lymphocyte binding to endothelial cells. The cloning of a mouse VAP-1 (mVAP-1) cDNA revealed that mVAP-1 is a novel 110/220 kDa transmembrane molecule with significant identity to copper-containing amine oxidases. In this work the nucleotide sequence and primary structure of the mVAP-1 gene was determined and the promoter region was structurally characterized. The isolated approximately 14.4-kb mVAP-1 gene consists of 4 exons and 3 introns. Primer extension analysis and 5' rapid amplification of cDNA ends revealed multiple transcription initiation sites in different tissues suggesting that the mVAP-1 transcription is differently regulated in different tissues. Analysis of the sequence immediately upstream of the detected transcription initiation sites showed no canonical TATA or CCAAT elements, but putative regulatory elements were found close to the detected transcription start sites. The cloning of the mVAP-1 gene reveals the first insight into the genomic organization of murine amine oxidases and will, by targeted disruption of the gene, allow us to understand better the importance of VAP-1 in leukocyte trafficking and monoamine oxidase activity for the function of the immune system.

Published

1998

5. Comparison of E-selectin-binding glycoprotein ligands on human lymphocytes, neutrophils, and bovine gamma delta T cells.

Author

Jones WM, Watts GM, Robinson MK, Vestweber D, and Jutila MA

Subjects

Animals, Antigens, Surface blood, Blotting, Western, Cattle, Cell Adhesion Molecules isolation & purification, E-Selectin isolation & purification, Epitopes, T-Lymphocyte blood, Flow Cytometry, Glycoproteins isolation & purification, Humans, L-Selectin physiology, Ligands, Membrane Glycoproteins physiology, Precipitin Tests, Protein Binding immunology, Receptors, Fibroblast Growth Factor physiology, Sialoglycoproteins, Cell Adhesion Molecules metabolism, E-Selectin blood, Glycoproteins blood, Neutrophils metabolism, Receptors, Antigen, T-Cell, gamma-delta blood, Receptors, Lymphocyte Homing metabolism, T-Lymphocyte Subsets metabolism

Abstract

We compared E-selectin-binding cell surface ligands on bovine gamma delta T cells and human leukocytes using an E-selectin/Ig chimera. The chimera worked well in flow cytometric studies and showed that bovine gamma delta T cells were the only lymphocyte population in newborn animals that bound E-selectin chimera. Furthermore, the chimera blocked gamma delta T cell rolling on E-selectin. Chimera reacted with four potential glycoprotein ligands of 180, 200, 250, and 300 kDa in Western blot analysis of gamma delta T cell detergent lysates, and it specifically precipitated at least two of these E-selectin ligands (200 and 250 kDa) from lysates of cell surface biotinylated gamma delta T cells. Preclearing bovine gamma delta lysates of GD3.5 Ag and workshop cluster 1 did not abrogate E-selectin ligand precipitation, suggesting that these surface markers do not represent E-selectin ligands. Human neutrophils possessed three E-selectin-binding ligands of approximately 80 to 90, 130, and 230 kDa, while human lymphocytes variably possessed three ligands of 120, approximately 220 to 240, and 260 kDa. Cross-precipitation experiments confirmed the results of others that neutrophil L-selectin serves as the 80 to 90-kDa E-selectin ligand. The human lymphocyte approximately 220 to 240-kDa and 260-kDa ligands may be analogous to the bovine gamma delta T cell molecules, whereas the 120-kDa is unique to human cells. The identities of the human and bovine lymphocyte E-selectin ligands are unknown. Finally, E-selectin ligand-1 apparently may have a minimal role, if any, in lymphocyte/E-selectin interactions, since a polyclonal anti-E-selectin ligand-1 serum stained a minimal number of cutaneous lymphocyte-associated Ag-positive human lymphocytes and bovine gamma delta T cells.

Published

1997

6. Soluble E-selectin is found in supernatants of activated endothelial cells and is elevated in the serum of patients with septic shock.

Author

Newman W, Beall LD, Carson CW, Hunder GG, Graben N, Randhawa ZI, Gopal TV, Wiener-Kronish J, and Matthay MA

Subjects

Adult, Base Sequence, Cell Adhesion Molecules blood, Cell Adhesion Molecules isolation & purification, Chromatography, Gel, E-Selectin, Endothelium, Vascular chemistry, Enzyme-Linked Immunosorbent Assay, Female, Humans, Interleukin-1 pharmacology, Male, Middle Aged, Molecular Sequence Data, Sepsis blood, Cell Adhesion Molecules analysis, Endothelium, Vascular metabolism, Shock, Septic blood

Abstract

A quantitative sandwich ELISA for E-selectin in the fluid phase (soluble E-selectin, sEs) has been developed that is sensitive to 100 pg/ml. The assay shows no reactivity with either L- or P-selectins. We have used this to determine the fate of E-selectin after cell-surface expression and to test whether levels measured in vivo may represent the state of endothelial activation. E-selectin was first detectable in supernatants of IL-1-stimulated endothelial cells at 24 h, and increased slowly up until 72 h. However, over this time period the total E-selectin detectable in the system (cells plus supernatants) declined dramatically. 125I-surface-labeled endothelial cells cultured for 24 h show an E-selectin of reduced m.w. in the supernatant, indicating that the molecule is shed from the surface. The shed form also appears to be slightly smaller than the intact membrane form as determined from immunoprecipitation and molecular sieving studies. In addition, the cytoplasmic domain of the molecule found in supernatants of activated endothelial cells and in serum is not intact as determined by loss of reactivity with an antipeptide antibody specific for the cytoplasmic domain. We have examined the sera of 71 normal individuals. Without exception, sEs was found in serum in the range of 0.13 to 2.8 ng/ml, suggesting that even in the absence of overt inflammatory processes E-selectin is being synthesized and released into the bloodstream. In addition, bacteremic patients with hypotension, but not those without, showed markedly elevated sEs values. As determined by cell-binding studies, the blood-derived form of E-selectin is biologically active.

Published

1993

7. Regulation of locomotion and cell-cell contact area by the LFA-1 and ICAM-1 adhesion receptors.

Author

Dustin ML, Carpen O, and Springer TA

Subjects

B-Lymphocytes physiology, Cell Adhesion Molecules isolation & purification, Cell Line, Humans, Intercellular Adhesion Molecule-1, Lymphocyte Function-Associated Antigen-1 isolation & purification, Microscopy, Fluorescence, Cell Adhesion immunology, Cell Adhesion Molecules physiology, Cell Communication immunology, Cell Movement immunology, Lymphocyte Function-Associated Antigen-1 physiology

Abstract

We demonstrate complementary differences in the behavior of B lymphoblastoid cells adhering to LFA-1 or its counter-receptor ICAM-1. The interaction of B lymphoblastoid cells with glass-supported planar bilayers bearing LFA-1 or ICAM-1 was observed by time-lapse video microscopy, and the distribution of adhesion receptors on cells interacting with the planar bilayers was studied by immunofluorescence microscopy. B lymphoblasts formed a large contact area and crawled rapidly (up to 25 microns/min) on planar bilayers bearing ICAM-1. In contrast, these cells attached to planar bilayers bearing LFA-1 through a fixed point about which the cells actively pivoted, using a single stalk-like projection. Phorbol ester-stimulated lymphoblasts, which adhere more strongly to ICAM-1-bearing substrates than unstimulated lymphoblasts, were still capable of locomotion on ICAM-1. Phorbol ester stimulation of B lymphoblasts on planar bilayers bearing LFA-1 promoted a rapid conversion from "stalk" attachment to symmetrical spreading of the cell on the substrate. Cellular LFA-1 remained uniformly distributed on the cell surface during interaction with bilayers bearing purified ICAM-1 as determined by immunofluorescence. In contrast, ICAM-1 was concentrated in the stalk-like structure through which the unstimulated B lymphoblasts adhered to LFA-1 in planar bilayers, but ICAM-1 immunofluorescence became more uniformly distributed over the cell surface within minutes of phorbol ester addition. Neither LFA-1 or ICAM-1 colocalized with the prominent staining of filamentous actin in the ruffling membrane regions. Interaction through cell surface LFA-1 and ICAM-1, 2, or 3 promotes different cellular morphologies and behaviors, the correlation of which with previously observed patterns of lymphocyte interaction with different cell types is discussed.

Published

1992

8. Leukocyte integrin P150,95 (CD11c/CD18) functions as an adhesion molecule binding to a counter-receptor on stimulated endothelium.

Author

Stacker SA and Springer TA

Subjects

Animals, Antibodies, Monoclonal, Antibody Specificity, Chromatography, Affinity, Epitopes immunology, Humans, In Vitro Techniques, Integrin alphaXbeta2 isolation & purification, Integrin alphaXbeta2 metabolism, Lymphocyte Function-Associated Antigen-1 physiology, Macrophage-1 Antigen physiology, Precipitin Tests, Cell Adhesion Molecules isolation & purification, Endothelium, Vascular metabolism, Integrin alphaXbeta2 physiology

Abstract

p150,95 is a member of the beta 2 family of integrins, which includes both LFA-1 and Mac-1. These molecules are known to play a role in the adhesion of lymphocytes, granulocytes, and monocytes to various cell types including vascular endothelium. p150,95 is presumed to have an adhesive function because of its structural relationship to the other beta 2 integrins and the ability of anti-p150,95 mAb to inhibit some myeloid cell interactions with tumor cells, endothelial cells, and other substrates. In an endeavor to demonstrate directly that p150,95 can act as an adhesion molecule, we raised a mAb (CBRp150/4G1) to the alpha subunit of p150,95, which allows for the purification of functional intact p150,95 heterodimers. The antibody was selected by using a high pH elution ELISA. The assay was designed to select for antibodies directed to the alpha-chain of p150,95, which could be readily dissociated from p150,95 under conditions of high pH and 2 mM MgCl2. p150,95 purified under these conditions with CBRp150/4G1-Sepharose could be immunoprecipitated by using antibodies to the alpha- and beta-chains of p150,95 indicating that the structural integrity of the heterodimer was preserved during purification and elution. Elution in the absence of divalent cations yielded primarily dissociated alpha and beta subunits. Other antibodies previously made to p150,95 alpha-chain such as SHCL3 were greatly reduced in their efficiency of yielding intact heterodimer under these conditions. Mapping of the epitopes by using chimeric molecules of p150,95/Mac-1 revealed that antibodies that react with the divalent cation sites of p150,95 are inferior for the purification of intact p150,95. The adhesive capacity of p150,95 was demonstrated by the specific binding of 18-h rIL-1 beta or LPS-stimulated endothelial cells to purified p150,95 absorbed to plastic microtiter plates. These results indicate that p150,95 can function independently as an adhesion molecule and that it can interact with a counter-receptor on stimulated endothelium.

Published

1991

9. Identification of a new cell surface glycoprotein with accessory function in murine T cell responses.

Author

Golde WT, McDuffie M, Kappler J, and Marrack P

Subjects

Amidohydrolases pharmacology, Animals, Antibodies, Monoclonal immunology, Antigen-Presenting Cells immunology, Antigens, Differentiation metabolism, Antigens, Differentiation, T-Lymphocyte analysis, Concanavalin A pharmacology, Flow Cytometry, Interleukin-2 biosynthesis, Ligands, Lymphocyte Activation, Lymphocyte Cooperation, Lymphocyte Culture Test, Mixed, Lymphocyte Function-Associated Antigen-1, Mice, Molecular Weight, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase, Receptors, Leukocyte-Adhesion metabolism, Antigens, Surface analysis, Cell Adhesion Molecules isolation & purification, Glycoproteins analysis, T-Lymphocytes immunology

Abstract

T cell binding to target cells involves not only the TCR and its MHC-bound ligand, but also a collection of additional proteins on both the T cell and its target. In an attempt to identify new molecules involved in this binding, mAb were raised against APC, and screened for their abilities to inhibit T cell recognition of Ag plus MHC on B cells. Six antibodies were identified that inhibited this reaction and that bound a cell-surface glycoprotein (Lgp55), with core polypeptide Mr 30,000 and a glycosylated Mr of approximately 55,000 depending upon the cell source. The properties of Lgp55 were consistent with it being the mouse homologue of a recently identified human ligand (intercellular adhesion molecule-2) for lymphocyte functional Ag-1 because the proteins are of comparable Mr, and antibody to Lgp55, like anti-lymphocyte functional antigen-1, blocks T cell recognition of Ag presented by B cells, but not of Ag presented by mouse fibroblasts.

Published

1990

10. Isolation of the murine intercellular adhesion molecule 1 (ICAM-1) gene. ICAM-1 enhances antigen-specific T cell activation.

Author

Siu G, Hedrick SM, and Brian AA

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cell Adhesion Molecules immunology, Cell Adhesion Molecules isolation & purification, Cloning, Molecular, DNA isolation & purification, Epitopes genetics, Epitopes isolation & purification, Humans, Mice, Molecular Sequence Data, Sequence Homology, Nucleic Acid, Tissue Distribution, Cell Adhesion Molecules genetics, Epitopes immunology, Genes, Lymphocyte Activation, T-Lymphocytes immunology

Abstract

Cell adhesion molecules in the immune system are believed to play an important role in lymphocyte-target cell conjugate formation. One such molecule, intercellular adhesion molecule 1 (ICAM-1), is important in the function, aggregation, and adherence of leukocytes. Here, we report the isolation and characterization of the murine ICAM-1 gene. We report that the murine ICAM-1 gene is a member of the Ig gene superfamily, has limited homology to its human counterpart, and is expressed in cells of lymphocytic and myeloid lineages. Transfection of the ICAM-1 cDNA into MHC class II-transfected fibroblasts leads to enhancement of the Ag-specific T cell response when the transfectants are used as APC.

Published

1989

11. Molecular cloning and expression of Pgp-1. The mouse homolog of the human H-CAM (Hermes) lymphocyte homing receptor.

Author

Zhou DF, Ding JF, Picker LJ, Bargatze RF, Butcher EC, and Goeddel DV

Subjects

Amino Acid Sequence, Animals, Antigens, Ly genetics, Antigens, Ly isolation & purification, Blotting, Western, Cell Adhesion Molecules isolation & purification, Cell Line, Cloning, Molecular, Cricetinae, Cricetulus, DNA isolation & purification, Female, Humans, Membrane Glycoproteins genetics, Membrane Glycoproteins isolation & purification, Mice, Molecular Sequence Data, Ovary, Receptors, Lymphocyte Homing, Base Sequence, Cell Adhesion Molecules genetics, Receptors, Immunologic genetics, Sequence Homology, Nucleic Acid

Abstract

Mouse phagocytic glycoprotein-1 (Pgp-1; Ly-24) is a 95-kDa glycoprotein of unknown function that has served as an important T cell/leukocyte differentiation marker. Recent work has suggested that it may be related to a human 85- to 95-kDa glycoprotein (termed variously the Hermes Ag/lymphocyte homing receptor, ECMRIII, P80, and CD44) that is involved in lymphocyte binding to high endothelial venules in the process of lymphocyte homing, and has been implicated in other cell adhesion events. The widespread expression of this molecular class in diverse organ systems suggests a broad role in cellular adhesion, and has led to the unifying designation homing-cellular adhesion molecule (H-CAM). By using human H-CAM cDNA probes, we have isolated a full-length cDNA for the mouse homolog. Comparison of the human and mouse sequences reveals that an N-terminal domain homologous to cartilage proteoglycan core and link proteins, as well as the C-terminal transmembrane and cytoplasmic sequences, are highly conserved (89% and 86% identity, respectively). In contrast, a proximal extracellular domain thought to serve as a target for O-glycosylation and chondroitin sulfate attachment has undergone substantial divergence (only 42% identity). Transient expression of the cDNA in CHO cells followed by immunologic staining confirms that this mouse H-CAM cDNA encodes Pgp-1.1, one of two known Pgp-1 alloantigens.

Published

1989