BIOMAT Database Logo BIOMAT Database Logo

Activation of complement by an IgG molecule without a genetic hinge. 1993

O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Department of Biology, University of Oslo, Blindern, Norway.

The hinge region links the two Fab arms to the Fc portion of the IgG molecule. It mediates flexibility to the molecule and serves as a connecting structure between the two heavy chains. In addition it provides space between the Fab and Fc parts. All three properties have been proposed to be important for the ability of IgG to initiate complement activation leading to complement-mediated cell lysis (CML). Here we report the construction of a hinge-deleted mouse-human chimaeric IgG3 molecule with specificity for the hapten NIP (3-iodo-4-hydroxy-5-nitrophenacetyl), HM-1. HM-1 lacks the genetic hinge, but has an introduced cysteine between Ala 231 (EU numbering) and Pro 232 in the lower hinge encoded by the CH2 exon. The introduced cysteine forms a disulphide bond between the two heavy chains of the molecule. In CML, HM-1 shows a greater activity than IgG3 wild type. This is the first time an IgG molecule without a genetic hinge has been found to be active in CML. We conclude that the hinge functioning as a spacer is not a prerequisite for complement activation. Rather, its major role seems to be to connect the heavy chains to each other in the amino-terminal part of CH2. Because HM-1 is expected to have low Fab-Fc flexibility, this molecular feature is probably of no importance for complement activation.

UI MeSH Term Description Entries
D007074 Immunoglobulin G The major immunoglobulin isotype class in normal human serum. There are several isotype subclasses of IgG, for example, IgG1, IgG2A, and IgG2B. Gamma Globulin, 7S,IgG,IgG Antibody,Allerglobuline,IgG(T),IgG1,IgG2,IgG2A,IgG2B,IgG3,IgG4,Immunoglobulin GT,Polyglobin,7S Gamma Globulin,Antibody, IgG,GT, Immunoglobulin
D007127 Immunoglobulin Constant Regions The domains of the immunoglobulin molecules that are invariable in their amino acid sequence within any class or subclass of immunoglobulin. They confer biological as well as structural functions to immunoglobulins. One each on both the light chains and the heavy chains comprises the C-terminus half of the IMMUNOGLOBULIN FAB FRAGMENT and two or three of them make up the rest of the heavy chains (all of the IMMUNOGLOBULIN FC FRAGMENT) Ig Constant Regions,Immunoglobulin Constant Region,Constant Region, Ig,Constant Region, Immunoglobulin,Constant Regions, Ig,Constant Regions, Immunoglobulin,Regions, Ig Constant
D007143 Immunoglobulin Heavy Chains The largest of polypeptide chains comprising immunoglobulins. They contain 450 to 600 amino acid residues per chain, and have molecular weights of 51-72 kDa. Immunoglobulins, Heavy-Chain,Heavy-Chain Immunoglobulins,Ig Heavy Chains,Immunoglobulin Heavy Chain,Immunoglobulin Heavy Chain Subgroup VH-I,Immunoglobulin Heavy Chain Subgroup VH-III,Heavy Chain Immunoglobulins,Heavy Chain, Immunoglobulin,Heavy Chains, Ig,Heavy Chains, Immunoglobulin,Immunoglobulin Heavy Chain Subgroup VH I,Immunoglobulin Heavy Chain Subgroup VH III,Immunoglobulins, Heavy Chain
D008969 Molecular Sequence Data Descriptions of specific amino acid, carbohydrate, or nucleotide sequences which have appeared in the published literature and/or are deposited in and maintained by databanks such as GENBANK, European Molecular Biology Laboratory (EMBL), National Biomedical Research Foundation (NBRF), or other sequence repositories. Sequence Data, Molecular,Molecular Sequencing Data,Data, Molecular Sequence,Data, Molecular Sequencing,Sequencing Data, Molecular
D009592 Nitrohydroxyiodophenylacetate Also called 4-hydroxy-3-iodo-5-nitrophenylacetate. A haptenic determinant that can be radiolabeled and used as salts and derivatives for investigations of immunogenic specificity studies. NIP-Hapten,(4-Hydroxy-3-iodo-5-nitrophenyl)acetyl,(4-Hydroxy-5-iodo-3-nitrophenyl)acetyl,5-Iodo-4-hydroxy-3-nitrophenacetyl,Hydroxyiodonitrophenylacetate,NIP Acetyl Hapten,5 Iodo 4 hydroxy 3 nitrophenacetyl,Acetyl Hapten, NIP,Hapten, NIP Acetyl,NIP Hapten
D011993 Recombinant Fusion Proteins Recombinant proteins produced by the GENETIC TRANSLATION of fused genes formed by the combination of NUCLEIC ACID REGULATORY SEQUENCES of one or more genes with the protein coding sequences of one or more genes. Fusion Proteins, Recombinant,Recombinant Chimeric Protein,Recombinant Fusion Protein,Recombinant Hybrid Protein,Chimeric Proteins, Recombinant,Hybrid Proteins, Recombinant,Recombinant Chimeric Proteins,Recombinant Hybrid Proteins,Chimeric Protein, Recombinant,Fusion Protein, Recombinant,Hybrid Protein, Recombinant,Protein, Recombinant Chimeric,Protein, Recombinant Fusion,Protein, Recombinant Hybrid,Proteins, Recombinant Chimeric,Proteins, Recombinant Fusion,Proteins, Recombinant Hybrid
D002478 Cells, Cultured Cells propagated in vitro in special media conducive to their growth. Cultured cells are used to study developmental, morphologic, metabolic, physiologic, and genetic processes, among others. Cultured Cells,Cell, Cultured,Cultured Cell
D003001 Cloning, Molecular The insertion of recombinant DNA molecules from prokaryotic and/or eukaryotic sources into a replicating vehicle, such as a plasmid or virus vector, and the introduction of the resultant hybrid molecules into recipient cells without altering the viability of those cells. Molecular Cloning
D003167 Complement Activation The sequential activation of serum COMPLEMENT PROTEINS to create the COMPLEMENT MEMBRANE ATTACK COMPLEX. Factors initiating complement activation include ANTIGEN-ANTIBODY COMPLEXES, microbial ANTIGENS, or cell surface POLYSACCHARIDES. Activation, Complement,Activations, Complement,Complement Activations
D003545 Cysteine A thiol-containing non-essential amino acid that is oxidized to form CYSTINE. Cysteine Hydrochloride,Half-Cystine,L-Cysteine,Zinc Cysteinate,Half Cystine,L Cysteine

Related Publications

O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Complement activation by polymer binding IgG.
September 1984, Biomaterials,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Temperature dependent activation of the alternate complement pathway by an IgG cryoglobulin.
January 1979, American journal of hematology,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Complement activation by IgG immobilized on methylated silicon.
July 1996, Journal of biomedical materials research,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Human complement activation by self-associated IgG rheumatoid factors.
September 1982, Arthritis and rheumatism,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Insulin and IgG complexes. An immunologic bypass for complement activation.
August 1972, Diabetes,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Activation and inhibition of IgG mediated complement fixation by staphylococcal protein A.
August 1970, Clinical and experimental immunology,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Streptococcal protein H forms soluble complement-activating complexes with IgG, but inhibits complement activation by IgG-coated targets.
August 1997, The Journal of biological chemistry,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Enhancement of complement activation and cytolysis of human IgG3 by deletion of hinge exons.
November 1990, Scandinavian journal of immunology,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Staphylococcal protein A inhibits complement activation by interfering with IgG hexamer formation.
February 2021, Proceedings of the National Academy of Sciences of the United States of America,
O H Brekke, and T E Michaelsen, and R Sandin, and I Sandlie
Complement activation by human IgG antibodies to galactose-α-1,3-galactose.
September 2020, Immunology,
Copied contents to your clipboard!