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COORDINATION OF CLASSICAL AND 
ALTERNATIVE METHOD OF COMPLEMENT 
SYSTEM 
DEVU SYAM
Important effector in both innate and acquired immunity. 
Discovered in 1894 by Jules bordet as a heat labile component of 
the normal plasma which complement the antibacterial activity of the 
antibody. 
The term “complement” was coined by Paul Ehrlich: “the activity of 
blood serum that completes the action of antibody”. 
It consist of more than 30 distinct serum proteins which act as 
cascade. 
Synthesized by liver hepatocytes, blood monocytes, tissue 
macrophages and the epithelial cells of the gastrointestinal and 
genitourinary tracts. 
Circulate in serum as zymogens.
Four important functions: 
•Lysis of cells, bacteria and viruses. 
•Opsonization, which promotes the phagocytosis of 
particulate antigens. 
•Activation of inflammatory response. 
•Immune clearance, which removes immune complexes 
from the circulation and deposits them in the spleen and 
liver.
C1(C1q, C1r, C1s ) 
C2(C2a, C2b) 
C3(C3a, C3b) 
C4(C4a, C4b) 
C5(C5a, C5b) 
C6 
C7 
C8 
C9 
Factor B 
Factor D 
DAF, CD55 
CR1, CD35 
Factor H 
Factor I
NOMENCLATURE 
Designated by numerals : C1-C9 
By letter symbols: factor D, factor B etc 
Smaller fragments resulting from cleavage of a component is 
designated “a” and larger fragment designated “b” except for C2 
Those complexes that have enzymatic activity are designated by 
a bar over the number or symbol.
1-classical pathway which is activated by Ab bound 
to Ag 
2- the lectin pathway activated by carbohydrates 
3-Alternative pathway activated in the presence of 
various microbial pathogen
CLASSICAL PATHWAY 
Begins with the formation of antigen-antibody 
complex. 
IgM and IgG are involved. 
Conformational change in the Fc portion expose 
binding site for C1 component. 
C1 consist of C1q and two molecules each of C1r and 
C1s, held together in a complex (C1qr2s2) stabilized by 
Ca2+ ions.
C4b2a cuts C3 into two major fragments: 
C3b is the main effector molecule of the complement system. 
It coat the pathogen surface. 
Macrophages and neutrophils have receptors for C3b and can 
bind the C3b-coated cell or particle preparatory to 
phagocytosis. 
This effect qualifies C3b as an opsonin 
C3a, the small fragment is released into the surrounding fluids. 
It can bind to receptors on basophils and mast cells triggering 
them to release their vasoactive contents (e.g., histamine). 
Because of the role of these materials in anaphylaxis, C3a is 
called an anaphylatoxin.
A single C3 convertase molecule can generate over 200 
molecules of C3b, resulting in tremendous amplification at 
this step of the sequence. 
Many C3b molecules bind to the microbial surface. 
A labile internal thioester bond in C3 is activated as C3b is 
formed, allowing the C3b fragment to bind to free hydroxyl 
or amino groups on the cell membrane.
C5a is the most anaphylatoxine. 
C5b initiate the assembly of the terminal complement 
component. 
C5b, which serves as the anchor for the assembly of a single 
molecule each of 
•C6 
•C7 and 
•C8 
The resulting complex C5b•6•7•8 guides the polymerization of 
as many as 18 molecules of C9 into a tube inserted into the lipid 
bilayer of the plasma membrane. This tube forms a channel 
allowing the passage of ions and small molecules. Water enters 
the cell by osmosis and the cell lyses
The complement system can also be triggered without antigen-antibody 
complexes. 
Hydrolysis of C3 initiates alternative pathway. C3 is abundant in 
plasma. 
C3b is produced at a significant rate by spontaneous cleavage 
(trickover) through spontaneous hydrolysis of the thioester in the C3 to 
form C3b(H2O), allowing binding of factor B. 
factor D plasma protease cleave factor B (Bb $ Ba) to form 
C3b(H2O)Bb a fluid-phase C3 convertase, and can cleave C3 to C3a 
and C3b. 
This results in the formation of alternative pathway C3 convertase, 
C3bBb.
C3 convertase enzyme is stabilized by properdin or factor P.
INFLAMMATION 
many of the released fragments help develop an inflammatory 
response. 
C3a, C4a, C5a- anaphylotoxins bind to receptors on mast cells 
and basophils; degranulation, smooth muscle contraction; capillary 
dilation; fluid influx. 
C5a is also effective chemoattractants that initiate accumulation 
of complement and phagocytic cells to the site of infection or 
antigen-presenting cells to lymph nodes. C5a play key role in 
increasing migration and adherence of neutrophils and monocytes 
to vessels walls
Regulation of complement system 
Because it is nonspecific, several regulatory mechanisms are 
involved (otherwise there would be a lot of “collateral 
damage”). 
Many components are very labile. 
Many regulatory proteins block activity through binding to 
target.
Complement system
Complement system
Complement system

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Complement system

  • 1. COORDINATION OF CLASSICAL AND ALTERNATIVE METHOD OF COMPLEMENT SYSTEM DEVU SYAM
  • 2. Important effector in both innate and acquired immunity. Discovered in 1894 by Jules bordet as a heat labile component of the normal plasma which complement the antibacterial activity of the antibody. The term “complement” was coined by Paul Ehrlich: “the activity of blood serum that completes the action of antibody”. It consist of more than 30 distinct serum proteins which act as cascade. Synthesized by liver hepatocytes, blood monocytes, tissue macrophages and the epithelial cells of the gastrointestinal and genitourinary tracts. Circulate in serum as zymogens.
  • 3. Four important functions: •Lysis of cells, bacteria and viruses. •Opsonization, which promotes the phagocytosis of particulate antigens. •Activation of inflammatory response. •Immune clearance, which removes immune complexes from the circulation and deposits them in the spleen and liver.
  • 4. C1(C1q, C1r, C1s ) C2(C2a, C2b) C3(C3a, C3b) C4(C4a, C4b) C5(C5a, C5b) C6 C7 C8 C9 Factor B Factor D DAF, CD55 CR1, CD35 Factor H Factor I
  • 5. NOMENCLATURE Designated by numerals : C1-C9 By letter symbols: factor D, factor B etc Smaller fragments resulting from cleavage of a component is designated “a” and larger fragment designated “b” except for C2 Those complexes that have enzymatic activity are designated by a bar over the number or symbol.
  • 6. 1-classical pathway which is activated by Ab bound to Ag 2- the lectin pathway activated by carbohydrates 3-Alternative pathway activated in the presence of various microbial pathogen
  • 7.
  • 8. CLASSICAL PATHWAY Begins with the formation of antigen-antibody complex. IgM and IgG are involved. Conformational change in the Fc portion expose binding site for C1 component. C1 consist of C1q and two molecules each of C1r and C1s, held together in a complex (C1qr2s2) stabilized by Ca2+ ions.
  • 9.
  • 10.
  • 11.
  • 12.
  • 13. C4b2a cuts C3 into two major fragments: C3b is the main effector molecule of the complement system. It coat the pathogen surface. Macrophages and neutrophils have receptors for C3b and can bind the C3b-coated cell or particle preparatory to phagocytosis. This effect qualifies C3b as an opsonin C3a, the small fragment is released into the surrounding fluids. It can bind to receptors on basophils and mast cells triggering them to release their vasoactive contents (e.g., histamine). Because of the role of these materials in anaphylaxis, C3a is called an anaphylatoxin.
  • 14. A single C3 convertase molecule can generate over 200 molecules of C3b, resulting in tremendous amplification at this step of the sequence. Many C3b molecules bind to the microbial surface. A labile internal thioester bond in C3 is activated as C3b is formed, allowing the C3b fragment to bind to free hydroxyl or amino groups on the cell membrane.
  • 15.
  • 16.
  • 17. C5a is the most anaphylatoxine. C5b initiate the assembly of the terminal complement component. C5b, which serves as the anchor for the assembly of a single molecule each of •C6 •C7 and •C8 The resulting complex C5b•6•7•8 guides the polymerization of as many as 18 molecules of C9 into a tube inserted into the lipid bilayer of the plasma membrane. This tube forms a channel allowing the passage of ions and small molecules. Water enters the cell by osmosis and the cell lyses
  • 18.
  • 19.
  • 20. The complement system can also be triggered without antigen-antibody complexes. Hydrolysis of C3 initiates alternative pathway. C3 is abundant in plasma. C3b is produced at a significant rate by spontaneous cleavage (trickover) through spontaneous hydrolysis of the thioester in the C3 to form C3b(H2O), allowing binding of factor B. factor D plasma protease cleave factor B (Bb $ Ba) to form C3b(H2O)Bb a fluid-phase C3 convertase, and can cleave C3 to C3a and C3b. This results in the formation of alternative pathway C3 convertase, C3bBb.
  • 21.
  • 22.
  • 23. C3 convertase enzyme is stabilized by properdin or factor P.
  • 24.
  • 25.
  • 26. INFLAMMATION many of the released fragments help develop an inflammatory response. C3a, C4a, C5a- anaphylotoxins bind to receptors on mast cells and basophils; degranulation, smooth muscle contraction; capillary dilation; fluid influx. C5a is also effective chemoattractants that initiate accumulation of complement and phagocytic cells to the site of infection or antigen-presenting cells to lymph nodes. C5a play key role in increasing migration and adherence of neutrophils and monocytes to vessels walls
  • 27.
  • 28. Regulation of complement system Because it is nonspecific, several regulatory mechanisms are involved (otherwise there would be a lot of “collateral damage”). Many components are very labile. Many regulatory proteins block activity through binding to target.