Steps of an ELISA

Vocabulary:
Antibody
Primary antibody

Antigen
Secondary antibody

ELISA

Lesson Summary:
Student match diagrams with text descriptions to understand the steps of an ELISA.
A common test used to detect if a patient has been exposed to dengue virus is called
an ELISA (enzyme linked immunosorbant assay). This test takes advantage of the
interactions between antigens and antibodies. Often compared to a lock and key, an
antigen/antibody interaction is very specific.

Student Learning Objectives:

The student will be able to...
1. Sequence steps of an ELISA test
2. Define ELISA
3. Explain the use of an ELISA to aid in disease diagnosis
4. Describe antigen/antibody interaction
5. Diagram antigen/antibody interaction

2
? KEY QUESTION(S):
What is an ELISA? How
is it used as a diagnostic
test?

TIME ESTIMATE:
15 45 minutes depending on prior knowledge
LEARNING STYLES:
Visual, kinesthetic and
auditory

Standards:
SC.912.L.14.52 SC.912.L.16.10 SC.912.L.18.1

Materials:
Steps of an ELISA cards, cut (laminate for repeated use)
Steps of an ELISA student worksheet, per student pair (laminate for repeated use)

Background Information:
The ELISA has been used as a diagnostic tool in medicine and plant pathology, as
well as a quality-control check in various industries. In simple terms, in ELISA, an
unknown amount of antigen is affixed to a surface, and then a specific antibody is
applied over the surface so that it can bind to the antigen. This antibody is linked
to an enzyme, and, in the final step, a substance containing the enzymes substrate
is added. The subsequent reaction produces a detectable signal, most commonly a
color change in the substrate.
Performing an ELISA involves at least one antibody with specificity for a particular
antigen. The sample with an unknown amount of antigen is immobilized on a solid
support (usually a polystyrene microtiter plate) either non-specifically (via adsorption
to the surface) or specifically (via capture by another antibody specific to the same
antigen, in a sandwich ELISA). After the antigen is immobilized, the detection
antibody is added, forming a complex with the antigen. The detection antibody can
be covalently linked to an enzyme, or can itself be detected by a secondary antibody
that is linked to an enzyme through bioconjugation. Between each step, the plate is
typically washed with a mild detergent solution to remove any proteins or antibodies
that are not specifically bound. After the final wash step, the plate is developed
by adding an enzymatic substrate to produce a visible signal, which indicates the
quantity of antigen in the sample.
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Advance Preparation:

Project the image of antigens and antibodies.

Teaching tip: Make this into a file folder game. Affix the Steps of an ELISA student
worksheet to the inside left and right sides of a file folder. Laminate for repeated use.
Color copy the ELISA cards, laminate, and cut. Using small pieces of Velcro, place one
side on the ELISA cards and the other in the center of each step on the worksheet.

Procedure and Discussion Questions with Time Estimates:

1. Review or introduce the following key points about antibodies and antigens:
Antigens are foreign proteins which cause the immune system to generate
antibodies.
Specific antibodies are produced for each antigen. They bind like a lock and key.
There are different antibodies produced by the human immune system (IgG,
IgM, IgE, etc) but all have the same basic starting structure: a Y. At the top of the
Y is the part that recognizes a specific antigen.
The part of the antigen that binds with the antibody is referred to as the epitope.
In this picture, it is the gray parts.
Show the students that the tops of the antibody Y fits with certain epitopes on
the antigens. Some antigens have multiple epitopes, so they are recognized by
different antibodies (kind of like a back-up system).
Tell students scientists have developed diagnostic assays that utilize the unique
and specific binding properties of antibodies and antigens.
Introduce the idea that antibodies can serve as antigens as well and in
diagnostic assays we create antibodies that recognize other antibodies as
antigens or a protein which it is specific for.
Primary antibodies recognize the original antigen we are testing against.
Secondary antibodies recognize the first (primary) antibody. Using both increases
sensitivity.
2. Arrange students in pairs.
3. Distribute Steps of an ELISA cards and student worksheets to each pair.
4. Tell them to follow the directions on the worksheet.
5. (5-10 minutes) Allow student pairs to complete activity.
6. Review the steps together, clarifying as needed.
7. Show the video to reinforce how an ELISA is performed.
http://www.youtube.com/watch?v=RRbuz3VQ100&feature=related

Assessment Suggestions:
Instructor can visually observe correct completion of the activity.

Resources/References:
ELISA video: http://www.youtube.com/watch?v=RRbuz3VQ100&feature=related

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STUDENT WORKSHEET

Steps of an ELISA
A common test used to detect if a patient has been exposed to a virus such as HIV, Dengue, or West Nile
is called an ELISA (Enzyme Linked ImmunoSorbant Assay). This test takes advantage of the interactions
between antigens and antibodies. Often compared to a lock and key, an antigen/antibody interaction is
very specific. ELISA tests usually take place in plastic plates containing wells, or depressions.
Match the statements and images below to sequence the steps of an ELISA test.

Virus proteins (antigens) are added

to wells of a 96-well plate.

The antigens bind to the plastic,

coating the bottom of the wells.

The primary antibody is added to the well.

In the case of the dengue ELISA,
the primary antibodies (IgM) are from
the patients serum sample.

Excess antibody is washed away, leaving

only antibodies bound to the antigens
behind. This wash removes excess
antibodies that are unbound and prevents
non-specific binding.

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STUDENT WORKSHEET

A secondary antibody is added to the wells.

This antibody recognizes the patient
IgM antibodies, bound to the antigens.
The secondary antibody also has a
colorimetric tag attached.

Excess secondary antibody is washed away,

leaving only secondary antibodies,
bound to the patient IgM antibodies.
This wash removes excess antibodies
that are unbound.

A substrate is added to the wells.

Bound secondary antibody containing a

colorimetric tag will cause a color change
when exposed to the substrate. A color
change indicates a positive reaction.

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T E A C H E R PA G E S

Make one set of eight cards for each group. Cut along dotted lines to separate into eight cards, each
representing a step in the ELISA reaction.

23

T E A C H E R PA G E S

Steps of an ELISA
A common test used to detect if a patient has been exposed to a virus such as HIV, Dengue, or West Nile
is called an ELISA (Enzyme Linked ImmunoSorbant Assay). This test takes advantage of the interactions
between antigens and antibodies. Often compared to a lock and key, an antigen/antibody interaction is
very specific. ELISA tests usually take place in plastic plates containing wells, or depressions.
Match the statements and images below to sequence the steps of an ELISA test.

Virus proteins (antigens) are added

to wells of a 96-well plate.

The antigens bind to the plastic,

coating the bottom of the wells.

The primary antibody is added to the well.

In the case of the dengue ELISA,
the primary antibodies (IgM) are from
the patients serum sample.

Excess antibody is washed away, leaving

only antibodies bound to the antigens
behind. This wash removes excess
antibodies that are unbound and prevents
non-specific binding.

24

T E A C H E R PA G E S

A secondary antibody is added to the wells.

This antibody recognizes the patient
IgM antibodies, bound to the antigens.
The secondary antibody also has a
colorimetric tag attached.

Excess secondary antibody is washed away,

leaving only secondary antibodies,
bound to the patient IgM antibodies.
This wash removes excess antibodies
that are unbound.

A substrate is added to the wells.

Bound secondary antibody containing a

colorimetric tag will cause a color change
when exposed to the substrate. A color
change indicates a positive reaction.

25

T E A C H E R PA G E S

Antibody

Antigens

Antigen
Antigen-binding fragment

Antibody

TalkingGlossaryofGeneticTerms

NATIONALHUMANGENOMERESEARCHINSTITUTE
NATIONALINSTITUTESOFHEALTH|genome.gov

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IllustrationbyDarrylLeja,NHGRI