Presentation is loading. Please wait.

Presentation is loading. Please wait.

Chapter 12 - Immunological methods

Published byRebecca Malone Modified over 11 years ago

Similar presentations

Presentation on theme: "Chapter 12 - Immunological methods"— Presentation transcript:

1 Chapter 12 - Immunological methods
Objectives Be able to define the terms antibody and antigen. Understand the structure of an IgG antibody. Be able to give a brief description of the production of polyclonal and monoclonal antibodies, and antiglobulins. Be able to describe measurement of antibody-antigen complexes (immunofluorescence, direct and indirect ELISA. Be able to describe competitive ELISA and its application to measuring chemical contaminats. Be able to give a brief description of affinity chromotography, western blotting and immunoprecipitation.

2 Antigen Antibody Virus particles Macrophage B-cell T-cell
antigen-presenting molecule T-cell Antibody

3 There are five classes of antibodies, we will focus on the IgG class.

4 The B cells can make a unique antibody for each antigen presented
The B cells can make a unique antibody for each antigen presented. It is estimated that there is the potential to produce up to 1 x 1010 structurally different IgG antibodies.

5 Production of antibodies
Polyclonal antibodies – a mix of many different antibodies that recognize different determinants on an antigen. This mix makes standardization of assays difficult.

6 Production of antibodies
2. Monoclonal antibodies – a myeloma cell is fused with an antibody-producing cell to create a hybridoma cell capable of producing a single antibody. This is a more expensive process than producing polyclonals but is the cornerstone for a variety of drug/hormone/chemical assays that are routinely available.

7 7

8 Production of antibodies
3. Antiglobulins – these are antibodies to an antibody. The use of fluorescently or chemically-labeled antiglobulins makes it easy to detect antibodies in assays like ELISA (see later).

9 + self

10 Detection of the antibody-antigen complex
Direct or indirect immunofluorescence Direct ELISA (detects antigen) useful for - environmental samples - medicine drug testing hormone testing 3. Indirect ELISA (detects antibody) useful for - Treponema palladium (syphilis) - Feline leukemia virus - HIV Advantages of ELISA: cheap sensitive rapid

11 Giardia (left) and Cryptosporidium (right)– Fluorescent Antibody Staining
H.D.A. Lindquist, USEPA

12 Direct ELISA steps Indirect ELISA Steps of the ELISA assay
1) coat wells with Ab 1) coat wells with Ag 2) add sample (Ag) to each well 2) add sample (Ab) to each well 3) incubate and wash 3) incubate and wash 4) add enzyme-linked Ab 4) add enzyme-linked Ab 5) incubate and wash 5) incubate and wash 6) perform enzyme assay and measure color 6) perform enzyme assay and measure color

13 In the 1970’s, the first antibodies against pesticides were developed
In the 1970’s, the first antibodies against pesticides were developed. Using these antibodies, the ELISA assay was modified and developed for use in monitoring chemical contaminants in the environment. The technology has been further refined to the point that commercial kits are now available for detection of many different contaminants. Immunoassay kits available for: Pesticides Atrazine 2,4-D Metolachlor Paraquat Aldicarb Carbaryl Carbofuan Procymidone Alachlor Inorganics Other organic contaminants PCP (pentachlorophenol) PCB (polychlorinated biphenyls) BTEX (benzene, toluene, ethylbenzene) PAH (polyaromatic hydrocarbons) TNT nitrate cadmium lead mercury calcium cobalt nickel zinc Detection limits Water – low ug/L (ppb) Soil – high ug/L to low mg/L (ppb – ppm)

14 These kits are based on the competitive ELISA reaction.
Immunoassay for chemical contaminants 1. sample containing 2,4-D is extracted 2,4-D -Ab 2. enzyme-linked 2,4-D is added 2,4-D 3. antibody-linked magnetic beads are added -Ab 4. a magnetic field is applied beads are collected the enzyme substrate is added and color is produced depending on the amount of enzyme linked to the beads

15 Advantages of Immunoassays:
Assay sensitivity is in the low ug/L (ppb) Assay is rapid Assay is easy to perform Assay is cost-effect ($20/sample) Accepted by EPA Assay is portable Disadvantages of Immunoassays: cross reaction – an antibody may cross react with similar structures. This is a problem with PAHs and with the BTEX compounds. So usually, BTEX are measured as a combination. can be difficult to analyze multiple solutes

Download ppt "Chapter 12 - Immunological methods"

Similar presentations

Serological tests (Antigen antibody interactions)

Serological tests (Antigen antibody interactions)
ANTIGEN ANTIBODY REACTION

ANTIGEN ANTIBODY REACTION
Research Techniques Made Simple: Enzyme Immunoassay and ELISA

Research Techniques Made Simple: Enzyme Immunoassay and ELISA
Antibodies Analytical Techniques Utilizing Antibodies: flow cytometry

Antibodies Analytical Techniques Utilizing Antibodies: flow cytometry
Enzyme Linked Immunosorbent Assay

Enzyme Linked Immunosorbent Assay
If you would like to use any of the material presented in this slide show, please contact me, before doing so. Some of the material presented here may.

If you would like to use any of the material presented in this slide show, please contact me, before doing so. Some of the material presented here may.
Measurement of Immune function:. Detect antigens and / or antibodies. Immunological tests rely upon: ability of antibodies to aggregate particulate antigens.

Measurement of Immune function:. Detect antigens and / or antibodies. Immunological tests rely upon: ability of antibodies to aggregate particulate antigens.
In the name of God. Summer School Influenza Unit, Pasteur Institute of Iran summer 2012.

In the name of God. Summer School Influenza Unit, Pasteur Institute of Iran summer 2012.
ELISA Enzyme Linked Immunosorbent Assay. Definitions  Antibodies (also known as immunoglobulins abbreviated Ig) are gamma globulin proteins that are.

ELISA Enzyme Linked Immunosorbent Assay. Definitions  Antibodies (also known as immunoglobulins abbreviated Ig) are gamma globulin proteins that are.
AB+AG reactions Detect Identify Quantitate antigen or antibody Disadvantage: Cross reaction -similar or common epitope.

AB+AG reactions Detect Identify Quantitate antigen or antibody Disadvantage: Cross reaction -similar or common epitope.
Part Three Basic Test Methods

Part Three Basic Test Methods
Immune Testing.

Immune Testing.
LOCALIZING MOLECULES. 1. WHAT MOLECULES? LOCALIZING MOLECULES 1. WHAT MOLECULES? 2. WITH RESPECT TO WHAT?

LOCALIZING MOLECULES. 1. WHAT MOLECULES? LOCALIZING MOLECULES 1. WHAT MOLECULES? 2. WITH RESPECT TO WHAT?
Immunolabeling Technique

Immunolabeling Technique
© 2004 Wadsworth – Thomson Learning Immunology Tutorial Introduction & Course outline By: Moh’d J. Al Khatatneh.

© 2004 Wadsworth – Thomson Learning Immunology Tutorial Introduction & Course outline By: Moh’d J. Al Khatatneh.
Introduction to Immunoassays

Introduction to Immunoassays
Enzyme-linked Immunosorbent Assay

Enzyme-linked Immunosorbent Assay
Experimental systems in Immunology Sadegh Babashah, PhD Department of Molecular Genetics, Faculty of Biological Sciences, Tarbiat Modares University.

Experimental systems in Immunology Sadegh Babashah, PhD Department of Molecular Genetics, Faculty of Biological Sciences, Tarbiat Modares University.
What is a monoclonal antibody?.  An antibody that recognizes a single epitope  It is made by fusing B cells with myeloma cells to produce a hybridoma.

What is a monoclonal antibody?.  An antibody that recognizes a single epitope  It is made by fusing B cells with myeloma cells to produce a hybridoma.
LOCALIZATION OF A MOLECULE - placing in space and or time. -Answering where and/when.

LOCALIZATION OF A MOLECULE - placing in space and or time. -Answering where and/when.

Similar presentations

Ads by Google