Multiplex immunoassays enable the detection of multiple different analytes in the same sample. A well-designed multiplex assay could mean that only one vial of blood might need to be drawn from a patient instead of 8 or more vials. Therefore, one multiplex test can answer multiple questions at the same time. Immunoassays capitalize upon the specific affinity between antibody and antigen. Some immunoassays use antigen as the probe in order to detect the binding of antibody target, while other immunoassays use antibody probes in order to detect antigen targets. Most immunoassays are single-plex, meaning that they can only be used to detect one antibody-antigen pair at a time; this is generally the case with most ELISA (Enzyme Linked ImmunoSorbent Assay) tests. The idea of a multiplex ELISA is attractive, and it mostly indicates a type of multiplex immunoassay that relies upon antibody-antigen binding events. The traditional ELISA is single-plex, and requires multiple binding and washing steps as well as an enzymatic system that produces a colorimetric or chemiluminiscent label as a quantitative readout of target concentration in a sample.
Sonication of cells is an essential first step to any protein purification process. Sonication is used to break apart the cell membrane, which releases all proteins into solution. Once the intracellular and transmembrane proteins are free, they can be enriched by protein purification methods. One very useful method is biomagnetic protein purification. This process uses superparamagnetic beads to isolate specific target proteins. The superparamagnetic beads are coated with proteins that specifically bind to the proteins of interest, and a magnetic separation rack attracts the beads. The remaining cellular debris is washed away and replaced by a protein isolation buffer that keeps the proteins stable until further analysis can be performed.
Cellular assays form the backbone of basic research and drug discovery. A cell culture is the perfect environment in which to collect information about normal and abnormal growth, and to test novel drug compounds safely in a controlled environment. An assay in biology is carefully designed to test a single variable. Once a standard protocol for a cellular assay is established, it is highly consistent, so the chances of having confounding variables is low. This streamlines experiments and makes it easy to analyze data and draw conclusions.
A magneto elisa is a combination of magnetic bead separation and Enzyme Linked ImmunoSorbent Assay (ELISA) for analyte detection. The magnetic bead separation helps to enrich the target population from complex media such as serum or whole blood prior to quantitative detection via ELISA. This works particularly well for cell separation and detection. One example where a magneto ELISA was used, was to detect CD4+ T-cells from whole blood of HIV patients. An accurate count of CD4+ T-cells is imperative in the treatment and management of HIV and detection of AIDS development.
Proteomics is the study of the protein in an organism. Protein is a fundamental building block of life, and proteins are the workhorses within and between cells. Biochemical pathways are built out of enzymes and ligands—without them nothing would be accomplished; plants wouldn’t produce glucose, animals wouldn’t be able to digest food, the immune system would cease to exist, and all other biological processes would grind to a halt. The fundamental importance of proteins for life makes them an important topic of study. The first step in understanding protein structure and function is to extract them. Protein extraction is the process of isolating and purifying protein from samples of whole tissue, cell cultures, or biological fluids. The protein extraction protocol used is tailored to match the starting material and the end goals of the assay. Considering the goal of the experiment is extremely important when developing a protein extraction protocol because certain buffer choices (such as high salt, high detergent formulations) can ruin an experiment when higher order protein structure and function needs to be preserved.
Cell lysis is the first step of breaking the cell membrane that enables further study of the proteins, nucleic acids, and other molecules inside of cells. When cell lysis is successful, the undamaged contents of the cell escape through the damaged cell membrane. These contents are then separated out of the mixed sample and used for further study. The methods used for separation of the lysed cell contents are dependent on the goal of the study. Careful investigation of these inner workings can reveal disease patterns, improve our understanding of normal cellular function, and elucidate biochemical pathways and therapeutic targets. Protein isolation is different from nucleic acid separation, and the reagents used vary drastically. There are a few ways to lyse the cell membrane; these include mechanical disruption, liquid homogenization, freeze/thaw cycles, manual griding, and the use of detergents. Sonication cell lysis is an example of mechanical disruption used for releasing the contents of cells.
Flow cytometry, or fluorescent activated cell sorting (FACS) has become a fundamental method for analyzing and collecting cell populations. Flow cytometry tells you the percentage of cells in a particular population that have the characteristics that you are interested in. These characteristics are defined by the array of surface proteins on each cell. The principle of flow cytometry involves labeling cell surface proteins with fluorophores and using lasers to record the fluorescent profile of a population of cells; these cells can also be sorted and isolated into enriched populations during the FACS process. The results of flow cytometry are read by the technicians and scientists performing the assay, and are typically displayed as two-dimensional dot plots with color density information included for greater detail and dynamic range.
A lateral flow immunoassay is an easy-to-use and inexpensive paper-based device used to detect the presence of specific protein in fluid. The basic immunoassay works by taking advantage of the lock-and-key specificity of antibodies and their corresponding antigens. In the case of a lateral flow immunoassay the capture antibodies are printed onto a paper strip and the liquid moves across it via capillary action. The presence of the target antigen is detected by a colorimetric change on the strip of paper, which also makes the lateral flow assay an example of immunochromatography. The principle component of most immunochromatography devices is usually gold nanoparticles or an enzyme-conjugated bead; the gold nanoparticles have a red hue, and enzyme conjugated beads produce a colorful product when a substrate is introduced into the system. In both instances a positive test result is visible to the naked eye. Most lateral flow immunoassays are qualitative tests, which means that a color change on the test line indicates a positive result while the lack of color indicates a negative result. There is a significant amount of research invested in the development of quantitative lateral flow immunoassays in which numerical analysis of protein concentration is possible.
An antigen is a substance that is capable of stimulating an immune response and activating white blood cells to produce antibodies. Antigens can be proteins or sugars that are located on the outer surfaces of cells. All cells have antigens including the ones inside the body, bacteria, and even viruses. The antibodies produced by the immune system are custom-fitted to the antigen that initially stimulated the immune response. The antibodies have an antigen recognition site (paratope) that has highly specific affinity for a region on the antigen called the epitope.
Nanobeads have applications ranging from basic science research to clinical imaging and targeted drug delivery. Nanobeads are composites of nanoparticles. Nanoparticles are defined as being less than 100 nanometers in diameter while nanobeads are usually around 50 to 200 nanometers in diameter. There are also microbeads, but these are much larger and have diameters of at least 1000 nanometers, or 1 micrometer, which is close to the size of a cell. Animal cells range from 10 to 30 micrometers in diameter. The size of nanobeads is very important to their function; partly because they are so much smaller than a cell, which enables them to be used for cell labeling and isolation. In the case of magnetic nanobeads, the nanometer size imparts the paramagnetic property that is so valuable for biomagnetic separation, clinical imaging (contrast enhanced magnetic resonance (MRI)), and therapeutics such as magnetic hyperthermia for targeted tumor destruction.