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Immunofluorescent analysis of a section of adult mouse cerebellar dentate nucleus stained with chicken pAb to neuron specific enolase (NSE), CPCA-NSE, dilution 1:3,000 in red. The section was costained with rabbit pAb to GFAP, RPCA-GFAP, dilution 1:5,000 in green. The blue is Hoechst staining of nuclear DNA. Following transcardial perfusion of mouse with 4% paraformaldehyde, brain was post fixed for 24 hours, cut to 45μM, and free-floating sections were stained with above antibodies. CPCA-NSE antibody detects NSE protein heavily expressed in the cytoplasm and dendrites of dentate neurons while the GFAP antibody stains the network of astroglial cells.

Western blot analysis of different tissue and cell lysates using chicken pAb to neuron specific enolase (NSE), CPCA-NSE, dilution 1:5,000 in green: [1] protein standard (red), [2] rat brain, [3] mouse brain, [4] cow brain and [5] SH-SY5Y cells. The strong band at about 47kDa corresponds to the NSE protein.

Chicken Polyclonal Antibody to NSE
Cat# CPCA-NSE

$120.00 – $800.00

Neuron specific enolase (NSE) is an enzyme which catalyzes the conversion of 2-phosphoglycerate to phosphoenolpyruvate in the glycolytic pathway, and also the reverse reaction in gluconeogenesis. It is one of three mammalian enolases, which are also known as ENO1, ENO2, and ENO3 or alternately as α, β and γ-enolase. The three enolases are related in protein sequence (see here), and have different cell type specific expression patterns, so that antibodies to them are useful cell type specific markers. NSE is also known as enolase 2 or γ-enolase and is heavily expressed in neuronal cells. Enolase 1 is also known as α-enolase and as non-neuronal enolase. The third enolase, enolase 3 or β-enolase, is expressed in muscle cells. Perhaps not surprisingly, since neurons require a great deal of energy, they are very rich in glycolytic enzymes such a GAPDH and NSE. Antibodies to this protein are therefore useful to identify neuronal cell bodies, and also developing neuronal lineage and neuroendocrine cells. Release of NSE from damaged neurons into CSF and blood has also been used as a biomarker of neuronal injury, and elevated NSE levels in blood and tissues are seen associated with various kinds of neuroendocrine derived tumors (1,2).
The CPCA-NSE antibody was made against full length recombinant human NSE expressed in and purified from E. coli. It can be used to trace NSE and to identify neuronal cells in cell culture and sectioned material, and it also works for IHC. As shown under our “Additional data” tag this antibody is an excellent marker of neuroendocrine cells in the pancreas. We also supply an alternate polyclonal antibody to NSE made in rabbit, RPCA-NSE. Mouse select image at left for larger view.

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SKU: cpca-nse Categories: Cell Structure Marker, Cell Type Marker, Chicken Polyclonal Antibodies, Developmental Marker, Immunohistochemistry Verified
  • Overview
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  • Data Sheets
Name: Chicken polyclonal to neuron specific enolase
Immunogen: Recombinant full length human NSE expressed in and purified from E. coli.
HGNC Name: ENO2
UniProt: P09104
Molecular Weight: 47kDa
Host: Chicken
Isotype:
Species Cross-Reactivity: Human, rat, mouse
RRID: AB_2861180
Format: Concentrated IgY preparation in PBS plus 0.02% NaN3
Applications: WB, IF/ICC, IHC
Recommended Dilutions: WB: 1:5,000-1:10,000. IF/ICC 1:500-1:1,000. IHC: 1:10,000
Storage: Store at 4°C. For longer term storage freeze at -20°C

A sequence alignment of the 3 human enolase molecules can be downloaded from here.

Chromogenic Immunostaining of a formalin fixed paraffin embedded rat cerebral cortex section with chicken pAb to neuron specific enolase (NSE), CPCA-NSE, dilution 1:10,000, detected in DAB (brown) following the ABC method. Hematoxylin (blue) was used as the counterstain. The NSE protein is localized to the cytoplasm of most neurons, with the exception of Purkinje cells.

Chromogenic Immunostaining of a formalin fixed paraffin embedded human pancreas section with chicken pAb to neuron specific enolase (NSE), CPCA-NSE, dilution 1:10,000, detected in DAB (brown) following the ABC method. Hematoxylin (blue) was used as the counterstain. The NSE antibody robustly stains the neuroendocrine cells of pancreatic islets.

1. Begaz T, Kyriacou DN, Segal J, Bazarian JJ. Serum biochemical markers for post-concussion syndrome in patients with mild traumatic brain injury. J. Neurotrauma 23:1201-10 (2006).

2. Isgrò MA, Bottoni P, Scatena R. Neuron-Specific Enolase as a Biomarker: Biochemical and Clinical Aspects. Adv. Exp. Med. Biol. 867:125-43 (2015).

3. Shaw G, et al. Preferential transformation of human neuronal cells by human adenoviruses and the origin of HEK 293 cells. FASEB J. 16:869-71 (2002).

Download Datasheet PDFMSDS Datasheet PDF

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EnCor Biotechnology Inc.
4949 SW 41st Boulevard, Ste 40
Gainesville
Florida 32608 USA

Phone: (352) 372 7022
Fax: (352) 372 7066
E-mail: [email protected]

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