Background to ELISA

Related articles

Loading Control Antibody Guide

Knockout-validated primary antibodies

Polyclonal antibodies

Goat polyclonal antibodies

Monoclonal antibodies

Rabbit monoclonal antibodies

Secondary antibodies resources

Alexa Fluor secondary antibodies

Biotinylated secondary antibodies

DyLight secondary antibodies

Gold-labelled secondary antibodies

FITC secondary antibodies

HRP secondary antibodies

Products related to novel coronavirus research

TMPRSS2 and COVID-19

ACE2 and SARS-COV-2 research

CD marker antibodies

Protein Tag antibodies

Bradford immunoassay protocol

Antibody types and structure

Antibody purification methods

How to prepare Phosphate Buffered Saline (PBS)

How to use UniProt

Flow Cytometry introduction

Flow Cytometry (FC) protocol

How to design a flow cytometry panel

The Flow Cytometer

Flow Cytometry Gating

Fluorescent Markers

Isoclonic Controls

Isotype Controls

Flow Cytometry Optimisation

When to use Flow Cytometry?

Multicolour Panels

Western blot introduction

SDS-PAGE

Western Blot Protocol

Western Blot Troubleshooting

BSA vs Non-fat milk

Protein loading techniques

Calculating the Rf values

Bradford assay

Knockout Validation

Enhancing Detection of Low-Abundance Proteins

PVDF vs Nitrocellulose

9 tips for detecting phosphorylation events using a Western Blot

Western Blotting with Tissue Lysates

Immunodetection

Blotting, gels and samples:

Antibodies and epitope tags

Immunoprecipitation

Western blot membrane stripping protocol

Data analysis

Immunohistochemistry introduction

Immunohistochemistry and Immunocytochemistry

Immunohistochemistry protocol

Immunohistochemistry troubleshooter

Chromogenic and Fluorescent detection

Preparing paraffin-embedded and frozen samples for Immunohistochemistry

Immunofluorescence introduction

Immunofluorescence guide

Immunofluorescence assay protocol

ELISA introduction

Types of ELISA

Background to ELISA

Choosing the right ELISA kit

ELISPOT assay protocol

Competitive ELISA assay protocol

Direct ELISA assay protocol

Indirect ELISA assay protocol

Sandwich ELISA assay protocol

ELISA components

ELISA troubleshooting

Matched antibody pair

ELISA assay spectrophotometry

Measuring analyte concentration using serial dilutions and standard curve

What is ELISA?

Enzyme-linked immunosorbent assay (ELISA) is a laboratory technique, via which antigens can be detected in biological samples. Similar to the rest of the immunoassays, this technique also relies on specific antibodies to detect the antigen of interest. This detection consists of specific antigen-antibody interactions.

ELISA principles:

During the ELISA assay, the antigen is fixed to a solid surface, either directly or with the help of a capture antibody. Following the antigen immobilization, a detection antibody, which has been conjugated with a suitable molecule for a detection is added. This molecule can be a fluorophore or an enzyme.

 

 

The greatest advantage of this assay is its high specificity and sensitivity. ELISAs can easily detect antigens at the picogram level under the right conditions. Carrying out the experiment is relatively simple, thanks to the protocols that are supplied with the kits.

 

 

The main disadvantage of this assay is that the readout must be obtained in a short time, because the detection is based on the enzyme and substrate reactions. The information that can be obtained about the antigen is quite limited, because it solely relies on the amount of it present in the sample.

Types of ELISA detection:

ELISA uses the enzymatic label for production of a detectable signal, which is directly correlating to the antibody-antigen binding. Several types of enzymes and substrates can be used in this assay, leading to different methods being incorporated.

 

 

The major difference is that in direct ELISA only one antibody is used, compared to two that are needed for indirect ELISA.

Direct detection:

When performing direct detection, the antibody is conjugated to the detection enzyme, which is both cost and time effective. The downside to this method is that the antibody reactivity can be altered, due to the attached enzyme. Also, the enzyme labelled antibody has to be different for every target antigen.

Indirect detection:

In this type of detection, the antibodies are coupled with biotin and then a streptavidin-conjugated step is performed. Using unlabelled primary antibodies combined with either enzyme or biotinylated secondaries is also possible.