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Agglutination

It is an Ag-Ab reaction in which the antigen is bound to a surface

when the Ab react with the Ag thatBound to its original surface we call it

Direct agglutination

when the Ab react with the Ag thatBound to artificial surface we call it

Indirect agglutination

Agglutination

Coomb’s test (Antiglobulin test or AGT)

o immune-mediated hemolytic anemia.o Hemolytic disease of the newborn

(ABO, Rh)

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o identify antibodies present in a patient's serum prior before blood transfusion.

o Blood transfusion preparation.o Antenatal antibody screening.

Agglutination

Latex agglutination

Agglutination

Latex agglutination: Lancefield grouping for streptococci

Agglutination

Co-agglutination

 Aggregation of “particulate antigens” bound with agglutinins of more than one specificity.

Example: coagglutination staphylococcus aureus protein A for serotyping strains ofStreptococcus pneumoniae,

Agglutination

Haemagglutination

Haemagglutination inhibition

o Example: Influenza virus

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o Heterophiles antibodies tests (Monospot test, Paul – Bunnell test):o  agglutination of the horse RBCs by heterophile antibodies in patient's serum for rapid diagnosis of EBV infectious mononucleosis.

o Cold agglutnin test:o Cold agglutinins are antibodies made by the immune system in response to infection having the ability to agglutinate RBC in Low temperature. E.g. Mycoplasma pneumoniae

o Weil felix test:o  it is agglutination test for the diagnosis of rickettsial infections.o based on the presence of antigenic “cross-reaction” between Rickettsia and certain serotypes of  Proteus 

o VDRL: screening for syphilis caused by treponema pallidum.

o Widal test: standard tube agglutination test for salmonella typhi.

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Precipitation

o It is a reaction in which the Ab interact with a free soluble Ag .

o At the optimum concentration ,positive reaction form a precipitin line

Complete identity

Precipitation: Ouchterlony, agar diffusion test

Non identity Partial identity

o This is precipitation reaction to test identity between two antigens or between two antibodies

Double immunodiffusion

Precipitation: Ouchterlony, agar diffusion test

Non identity Partial identity

Complete identity

o This is precipitation reaction to test identity between two antigens or between two antibodies

Double immunodiffusion

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Negative control (non Toxogenic)

Test organism

Positive control (Toxogenic)

Precipitin lines

o an Antigen (toxin), antibody (antitoxin) reaction.o +ve reaction produce a precipitin lines. (precipitation reaction)o Used to identify the toxogenic corynebacterium diphtherae

Precipitation

AgMg/ml

Diameter /mm

SampleDiameter

Sampleconcentration

o This is precipitation reaction to test presence of entire subclass of immunoglobulin by applying specific antiglobulin forming a precipitation rings.

Single radial immunodiffusion

Precipitation

o This is method to separate the serum by electrophoresis.o Create a trench containing specific anti serum.o Diffusion of both serum and anti serum forming a precipitin

lines Counter immuno-electrophoresis

Western bloto technique used to detect specific proteins in the given sample.

o  It uses ”gel electrophoresis” to separate proteins (or polypeptide) and are then transferred to a membrane.

o  (nitrocellulose) where they are stained with labled antibodies specific to the target protein.

Sample ABTest Ag Enzym linked Ab Enzyme substrate

Western blot

Immunofluorescenceo Antibodies containing fluorescent dye react with

serum (either Ag or Specific Ab)..

o Positive reaction is shown under fluorescent microscope.

Toxin antitoxin Neutralization

The toxin( hemolysin) sample (serum) Ab RBC lysed with the toxin

o Testing the presence of the antitoxin in the serum.

o If they are present the toxin will be neutralized .RBCs not lysed.

o If there is no antitoxin the toxin will lyse the RBCs

The toxin( hemolysin) sample (serum) Ab RBC lysed with the toxin

Toxin antitoxin Neutralization invitro example Anti-streptolysin O ASO

Schick’s test:

o Testing immunity of the patient against diphtheria.o 0.2 ml of the diphtheria toxin in the test forearm and 0.2 ml of inactivated diphtheria toxin (by heat ) in the control forearm.

Complement fixation test (CFT)

o Preparing sensitized complement & two systems:

o System1:o Containg serum sample &

prepared antigeno System 2 (indicator system):

o containing sensitized sheep RBCs & Ab to sheep RBCs.

o In +ve reaction the serum containing Ab will react with the Ag the complement will be consumed by system 1 (RBCs will not be lysed)..

o In –ve reaction where there is no Ab in the serum so the complement will consumed by system 2 (RBCs will be lysed).

Test A g S ample A B complement S heep RB C A b to sheep RB C

Sample ABTest Ag complement Ab to sheep RBCSheep RBC

Radioimmunoassay

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Enzyme Linked Immuno-Sorbent Assay (E.L.I.S.A)

S ample A BA g Enzym linked A b Enzyme substrate

o This a solid phase reaction through which the serum antibody will be captured to the wells using capture Ag.

o An Antihuman globulin conjugate containing chromogenic enzyme will react with the sample Ab.

o Adding enzyme substrate will produce colour on the well.

o So +ve test is manifested by presenece of colour , in –ve test there is no colour.Indirect E.l.I.S.A

Sample ABAg Enzym linked Ab Enzyme substrate

Enzyme Linked Immuno-Sorbent Assay (E.L.I.S.A)

o This a solid phase reaction through which the serum antibody will be captured to the wells using capture Ag.

o The conjugate here is directed to the Ag i.e. the sample and conjugate will compete each other.

o Adding enzyme substrate will not produce colour on the well.

o So +ve reaction is manifested by no colour , -ve reaction there is a colour.Competitive E.l.I.S.A

S ample A BA g Enzym linked A b Enzyme substrate

Sample ABAg Enzym linked Ab Enzyme substrate

Enzyme Linked Immuno-Sorbent Assay (E.L.I.S.A)

o This a solid phase reaction through which the serum antigen will be captured to the wells using capture Ab.

o The conjugate here is directed to the Ag i.e. the Ag will be sandwiched between capture & test Abs

o Adding enzyme substrate will produce colour on the well.

o So +ve test is manifested by presenece of colour , in –ve test there is no colour.Sandwich E.l.I.S.A

A BSample A g Enzym linked A b Enzyme subst rate

ABSample Ag Enzym linked Ab Enzyme substrate

Enzyme Linked Immuno-Sorbent Assay (E.L.I.S.A)

Spectrophotometer

Flowcytometry o  is a biophysical laser based technology employed in cell counting, cell marker detection, allowing synchronized analysis of the physical and chemical characteristics of up to thousands of particles per second.

o Example: used in the diagnosis  blood cancers, and CD4 cell counting in AIDS patients

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Immunochromatography

o rapid and easy.o Antigen-antibody immune

complexes flow through a region and encounter antibody against them, resulting in a visible coloured line

o E.g Used in rapid diagnosis of Malaria

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