Serological Tests PDF

Summary

This document provides an overview of serological tests, including ELISA, Immunofluorescence, Immunoperoxidase, and Radioimmunoassay. It explains the principles and procedures involved, as well as the applications of these methods.

Full Transcript

‫ميحرلا نمحرلا هللا مسب‬
Serological
tests
Presented by
Abeer Mohamed
Assistant lecturer at Microbiology department
 Antigen

▪ Means any substance, which when
introduced into body stimulate the
immune system to produce immune
response specific to the injected
substance and no to un-related materials.
 Antibody

Specific to
Fab Microbe

Specific to
FC species & (in
same Ab)
Labelling Antibody

Enzyme or
Fluoresence
isothiocynate
 Antigen- antibody reactions

❖ Are serological reactions and are
used as serological diagnostic tests
for the identification of infectious
disease.
 Serological tests
Used to detect and measure antigen –antibody reaction
Primary binding Secondary Tertiary binding
test binding test test

Immunofluorescence
Neutralization
ELISA and Precipitation
Agglutination test
Immunoperoxidase test

Radioimmunoassay
Complement
Fixation test
 Primary binding test

Tests that directly measure the binding of antigen and antibody
 Enzyme-linked
immunosorbent assay
(ELISA)
Principle:
1.ELISA is a serological test in which
the antigen-antibody reaction is
detected by labeling the antibody by an
enzyme (horseradish peroxidase and
alkaline phosphatase).
2.The enzymatic activity is detected by
addition of substrate which destructed into
certain a color detected by ELISA reader
(Spectrophotometer device)

3.The intensity of the developed color is
proportional to the amount of the antibody
or antigen.
4. Performed in wells of polystyrene plates
which used to absorb Ag or Ab (Microtiter plate)

5.Types of ELISA according to the solid surface
used:

- Cell ELISA: performed in wells of microtiter
plate.

- Dot ELISA: performed on high protein
binding paper (nitrocellulose membrane).
Dot ELISA
Cell ELISA
 Types of ELISA assays:

Direct ELISA: Indirect ELISA: Sandwich
antigen antibody ELISA: antigen
detection detection. detection
 Direct ELISA: antigen detection Substrate
Any free
Conjugated 1ry Ab
Ab washed
away
Fetal
5.Washing PBS
Ag
2.Washing PBS
3-5 times
bovine 3-5 times

serum
1.Incase of uncoated 3.Add fetal bovine 4.Add 6.Add substrate and
plate load Ag serum or casein conjugated 1ry incubated in dark place
(Sample) to well of (blocking substance) Ab with enzyme 15 min at room temp
microtiter plate and To allow Ab attached to and incubated which converted by
incubate overnight at Ag not to wall of wells 37 °C for 1hr. enzyme into detectable
4°C for complete substance then add
absorption to wells stop solution H2SO4
wall then measure colour
by ELISA reader
Advantages of direct ELISA: Disadvantages of direct ELISA:
Fewer steps. (Ag, labeled Ab) The direct labeling of primary
Quick results. antibodies for every Ag (expensive)
 Indirect ELISA: antibody detection& Secondary
quantitively determined. Ab
Any free
1ry Ab
washed
away

Fetal Washing PBS 3-5
2.Washing PBS times
Ag 3-5 times bovine
serum
1. Ag (known) coated 3.Add fetal bovine 4.Add serum or 5.Add
to well of microtiter serum or casein sample contain conjugated 2ry
plate and incubate (blocking substance) primary Ab Ab that binds to
overnight at 4°C for To allow Ab attached to (unknown) the primary Ab
complete absorption to Ag not to wall of wells unconjugated
wells wall and incubated
37 °C for 1hr.
 Substrate

Unbounded
2ry Ab
washed
away

Washing PBS 3-5
times

6.Add substrate so enzyme
hydrolyzed substrate to
form colored product then
measure by ELIZA reader
(the amount of colored
end product is directly
proportional to Ab
Advantages of indirect ELISA: Disadvantages of indirect ELISA:
-Cross-reactivity might occur with the
Highly sensitive and more flexible
secondary antibody, resulting in
than direct ELISA due to use 2ry Ab
nonspecific signal.
-An extra incubation step is required
in the procedure.
 Used for antigen detection but
Sandwich ELISA: the target antigen must contain at
antigen detection least two antigenic sites
(epitopes).
 Protein A one of cell wall
of Staphlyococoous
consider as receptor for FC
Unbounded Substrate
1ry Ab
washed
Ag away
Washing
Washing PBS 3-5 PBS 3-5
Washing PBS 3-5
times times
Ab times

1. Primary Ab (known) 2. Sample contain 4. Add detection 6.Add 8.substrate
added to coat well of suspected Ag is antibody (specific to a enzyme- so enzyme
microtiter plate and added to well, different epitope on conjugated hydrolyzed
incubate overnight at then incubation the antigen) and secondary substrate to
4°C for complete ex.37 °C for 1 hr allowed to react antibody is form colored
absorption to wells added and product
wall or already coated allowed to then
plate react. measure by
ELIZA reader
Reading ELISA results:

Qualitative result (especially for antibody detection) is determined by naked
eye as a simple colour change.

Quantitative result (antibody detection) is determined by measuring the
intensity of colour in a spectrometer (ELISA reader) or by testing dilutions of the
test serum and determining the highest dilution that shows a colour change.
 Dot ELISA

Dotted Ag allowed to dry at room temp

Nitrocellulose membrane floated with reference serum
containing specific Ab then incubated at room temp for 2hr

Washing 3 times by buffer

Immersed in pool contain antispecies serum (2ry Ab)
conjugated with peroxidase enzyme incubate 37C/2hr
Blue dot
Immersed in substrate working for 15 min at room temp in dark positive
place ,stop reaction by washing
 Immunofluorescence (IF)
fluorescent antibody test
(FAT)

Principle:
❑The intracellular location of antigen could
be determined in the infected cell cultures,
impression smears or thin frozen sections of
infected tissues by using specific antibodies
prelabeled with fluorescent dye (fluorescene
isothiocyanate).
Two types of fluorescent
antibody test

Direct Indirect
 Direct IF

Detection of
Ag within cell

Detection of
Identify Ag
location

In nucleus In cytoplasm
Procedure of the direct method:

1. Acetone-fixed tissue or smear containing
(Ag) (unknown or suspected) is fixed on a slide,
then incubated with the fluorescence antibody.

2.Wash (3 times by PBS) to remove unbounded
antibody

3. Examined by dark field illumination under a
microscope with UV light source
Result
The antigen particles that
bounded with labeled antibody
gives yellow-green fluorescence
 Indirect IF

Detection of Ab

Needed

Primary Secondary
unlabeled labeled
antibody antibody
Procedure of the indirect method:
1. Acetone-fixed tissue or smear is treated with (unlabeled
primary Ab) then incubated for 30 min at room temp

2.Wash (3 times by PBS) to remove unbounded antibody

3. A fluorescent labeled antibody (Secondary Ab) then
incubated for 30 min at room temp

4. Wash

5. Examined by fluorescence microscope
 Points of Direct IF Indirect IF
difference
For Detection Ag Detection Ab
Labeled Ab Primary Secondary
Steps 2-steps 3-steps
Time Rapid Slow
Advantage Rapid Conjugated Ab for
each species
Disadvantage Conjugated Ab for each Ag Slow

Specificity Less specific More specific
Disadvantages of immunofluorescence staining:
▪ High cost of fluorescent microscope and reagents.
▪ The need of well-trained person.
 Immunoperoxidase test (IP)

Principle:

The intracellular location of antigen could be determined in the
infected cell cultures, impression smears or thin frozen sections
of infected tissues by using specific antibodies prelabeled with
enzymes (peroxidases).
Immunoperoxidase (IP) staining

It is an alternative method for IF test.

Its procedures and principles are similar to those of IF test, but the
antibody is conjugated to peroxidase enzyme.

In the presence of appropriate substrate, the enzyme forms a colored
insoluble precipitate appear as yellowish-brown dots in the cytoplasm or
nucleus of the infected cell.
Advantages of IP staining in comparison with IF
staining:
Requires an ordinary light microscope.
Produces morphologically clearer, non-fading and
permanent preparation.
Disadvantages of IP staining:
▪ The presence of endogenous peroxidase enzyme in the cells
of many tissues, particularly leukocytes, may induce false
positive result with IP staining.
▪ This problem can be overcomed by destruction of the
endogenous peroxidase before staining by treatment of the
tissue sections with hydrogen peroxide.
Endogenous
peroxidase
Points of difference IP ELISA

Physical nature of Ag Ag in paraffine embedded Ag is free in fluid as saliva,
tissue section, fixed on In tissue homogenate,
slide, monolayer of filtrate
infected cell culture,
impression smear of
lymph node
Labeling Peroxidase enzyme Alkaline phosphatase
enzyme

Result of hydrolyzed Insoluble granules so Soluble color
substrate detect location of Ag
either in nucleus or
cytoplasm
Read Light microscope ELISA reader
 Same idea as ELISA but different label:
Radioactive isotope (instead of enzyme)
Measurement of Degree of radioactivity
(instead of degree of colour change)
As sensitive as ELISA
C. Radioimmunoassay Disadvantage: Hazards of radioactivity
(RIA) Applications:
Measurement of biological substances
(Ags) (e.g. drugs, hormones, tumour
markers)
Measurement of antibodies
Thanks for your attention