Editing ELISA (section)

==Principle==
As an analytical biochemistry assay and a "wet lab" technique, ELISA involves detection of an [[analyte]] (i.e., the specific substance whose presence is being quantitatively or qualitatively analyzed) in a liquid sample by a method that continues to use liquid reagents during the [[analysis]] (i.e., controlled sequence of biochemical reactions that will generate a signal which can be easily quantified and interpreted as a measure of the amount of analyte in the sample) that stays liquid and remains inside a reaction chamber or well needed to keep the reactants contained.<ref name="MsagatiFood17">{{cite book |url=https://books.google.com/books?id=P2Q6DwAAQBAJ&pg=PT229 |title=Food Forensics and Toxicology |last=Msagati |first=T.A. |publisher=John Wiley & Sons |year=2017 |page=PT229 |isbn=9781119101383}}</ref><ref name="CrowtherELISA95">{{cite book |chapter-url=https://books.google.com/books?id=AodkPkz_7NEC&pg=PA35 |chapter=Chapter 2: Basic Principles of ELISA |title=ELISA: Theory and Practice |last=Crowther |first=J.R. |series=Methods in Molecular Biology |publisher=Humana Press |year=1995 |volume=42 |pages=35–62 |doi=10.1385/0-89603-279-5:1 |pmid=7655571 |isbn=0896032795}}</ref> This is in contrast to "dry lab" techniques that use dry strips. Even if the sample is liquid (e.g., a measured small drop), the final detection step in "dry" analysis involves reading of a dried strip by methods such as [[reflectometry]] and does not need a reaction containment chamber to prevent spillover or mixing between samples.<ref name="SonntagDry93">{{cite book |chapter-url=https://books.google.com/books?id=ZW0UWoZNhpEC&pg=PA1 |chapter=Chapter 1: Introduction to dry chemistry |title=Dry Chemistry: Analysis with carrier-bound reagents |last=Sonntag |first=O. |editor-last=van der Vliet |editor-first=P.C. |series=Laboratory Techniques in Biochemistry and Molecular Biology |volume=25 |pages=1–6 |year=1993 |isbn=9780080887364}}</ref> 

As a heterogenous assay, ELISA separates some components of the analytical reaction mixture by adsorbing certain components onto a solid phase which is physically immobilized. In ELISA, a liquid sample is added onto a stationary solid phase with special binding properties and is followed by multiple liquid reagents that are sequentially added, incubated, and washed, followed by some optical change (e.g., color development by the product of an enzymatic reaction) in the final liquid in the well from which the quantity of the analyte is measured. The quantitative "reading" is usually based on detection of intensity of transmitted light by [[spectrophotometry]], which involves quantitation of transmission of some specific wavelength of light through the liquid (as well as the transparent bottom of the well in the multiple-well plate format).<ref name="MsagatiFood17" /><ref name="CrowtherELISA95" /> The sensitivity of detection depends on amplification of the signal during the analytic reactions. Since enzyme reactions are very well known amplification processes, the signal is generated by enzymes which are linked to the detection reagents in fixed proportions to allow accurate quantification, and thus the name "enzyme-linked".<ref name="NielsenFood17">{{cite book |url=https://books.google.com/books?id=_u4mDwAAQBAJ&pg=PA492 |title=Food Analysis |last1=Hsieh |first1=Y.-H.P. |last2=Rao |first2=Qinchun |editor-last=Nielsen |editor-first=S. Suzanne |publisher=Springer |pages=491–98 |year=2017 |isbn=9783319457765}}</ref>

The analyte is also called the ligand because it will specifically bind or ligate to a detection reagent, thus ELISA falls under the bigger category of [[ligand binding assays]].<ref name="MsagatiFood17" /> The ligand-specific binding reagent is "immobilized", i.e., usually coated and dried onto the transparent bottom and sometimes also side wall of a well<ref name="SchasfoortHand17">{{cite book |title=Handbook of Surface Plasmon Resonance |last=Schasfoort |first=R.B.M. |publisher=Royal Society of Chemistry |edition=2nd |page=296 |year=2017 |isbn=9781782627302}}</ref> (the stationary "solid phase"/"solid substrate" here as opposed to solid microparticle/beads that can be washed away), which is usually constructed as a multiple-well plate known as the "ELISA plate". Conventionally, like other forms of [[immunoassay]]s, the specificity of [[antigen]]-[[antibody]] type reaction is used because it is easy to raise an antibody specifically against an antigen in bulk as a reagent. Alternatively, if the analyte itself is an antibody, its target antigen can be used as the binding reagent.<ref name="ElgertImmuno09">{{cite book |url=https://books.google.com/books?id=gpNPZFGDPzgC&pg=PA149 |title=Immunology: Understanding the Immune System |last=Elgert |first=K.D. |publisher=John Wiley & Sons |pages=149–50 |year=2009 |isbn=9780470081570}}</ref>