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“NeuroELISA” kits are sandwich ELISAs (enzyme-linked immunosorbent assays). The kits are specifically validated and designed for fast, accurate and sensitive amyloid beta, tau and α-synuclein protein quantitation. These ready-to-use neurobiology ELISA kits enable measurements of protein from a variety of biological samples including serum, plasma and CSF (cerebrospinal fluid). For more information visit our Neurobiology ELISA Page.
We offer a large menu of Thermo Scientific Pierce and Novex neurobiology ELISA kits. These kits are manufactured to help ensure excellent quality and reproducibility. The kits meet quality-controlled specifications for criteria such as sensitivity, dynamic range, precision, specificity, recovery and lot-to-lot consistency. See our ELISA Selection Tool to find a kit to help with your research needs.
The ELISA method is a benchmark for quantitation of antigens. ELISAs are adaptable to high-throughput screening because results are rapid, consistent and relatively easy to analyze. The best results have been obtained with the sandwich format, utilizing highly purified, pre-matched capture and detector antibodies. The resulting signal provides data which is very sensitive and highly specific.
Neuro-specific ELISA protocols (Figure 1) begin with a capture antibody, specific for a protein of interest, coated onto the wells of microplates. Samples, including a standard containing protein of interest, control specimens and unknowns, are pipetted into wells. During the first incubation, the protein antigen binds to the capture antibody. After washing, a detection antibody is added to the wells, this antibody binds to the immobilized protein captured during the first incubation. After removal of excess detection antibody, an enzyme-linked (i.e. HRP) secondary antibody is added and binds to the detection antibody. After a third incubation and washing to remove the excess secondary antibody, a substrate solution is added and is converted by the enzyme to a detectable form (color signal.) The intensity of this colored product is directly proportional to the concentration of antigen present in the original specimen. Thermo Scientific Pierce and Novex neurobiology ELISA kits have been designed to enable specific detection of phosphorylation, offer great specificity and correlate well to western blot data.
Figure 1. Scheme of a typical neurobiology protocol. Our ready-to-use Neurobiology ELISA kits come with standard, detection antibody, HRP conjugate, chromogenic substrate and stop solution to complete all steps listed above.
Note: The protocol provided is representative of most neurobiology ready-to-use ELISA kits for measurement of neuroproteins. Protocols for individual kits may differ. Depending on the protein of interest, antibodies, buffers or substrates being used, this general protocol may need to be optimized. For more information see Overview of ELISA and ELISA Development and Optimization.
Run time: 4 hours — 30 minutes hands-on time.
Note: A standard curve must be run with each assay for quantification.
Note: If using an Antibody Pair Kit, to build your own ELISA, you will need to coat the capture antibody on to a 96-well microplate yourself. For this process you will need: a 96-well microplate, capture antibody, and blocking buffer (usually BSA or milk diluted in PBS). You will follow these steps before starting the above protocol:
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Thermo Scientific Pierce and Novex neurobiology ELISA kits are highly tested and validated. Below is data from our most popular kits. For more information about our selection of neurobiology ELISA kits please visit our Neurobiology ELISA page.
Figure 2. Tau (total) ELISA Kit, Human. Using the above protocol samples were serially diluted and run using Tau (total) ELISA Kit, Human. Parallelism between natural and recombinant (standard) human tau protein was demonstrated. | Figure 3. Amyloid beta 42 ELISA Kit, Mouse. Using the above protocol samples were spiked into standard diluent buffer and run using Amyloid beta 42 ELISA Kit, Mouse. Parallelism between amyloid beta standard and cell culture supernatant is demonstrated. Cell culture supernatant used came from Neuro2a (mouse neuroblastoma) cells. |
For Research Use Only. Not for use in diagnostic procedures.