EnzyChrom™ Nitric Oxide Synthase Assay Kit

SKU:BHT15600197
Suppliers
BioAssay Systems
BioAssay Systems
Details Products
Overview
Click light‑blue chips for details
EnzyChrom Nitric Oxide Synthase Assay Kit is designed for quantitative determination of nitric oxide synthase (NOS) activity and screen for NOS inhibitor. It uses OD540 nm readout; suited to biological; typical assay time 40 min; detection limit 0.25 U/L.
Detection method Colorimetric (OD 540 nm)
Sample type Biological
Species All species
Procedure 40 min
Detection limit 0.25 U/L
Options selector
Catalog no. Size
ENOS-100 100 Tests
Available Options

Select the variant that best fits your experiment. Availability and lead time may vary by option.

  • Options: Size: 100 Tests
  • Lead time: varies by selected option; please contact us for current fulfillment timing.
  • Storage: -20°C — Store at -20°C (freezer). Avoid repeated freeze-thaw cycles.
  • Shipping: cold-chain shipment (typically with ice packs).
  • Upon receipt: store at the recommended temperature as soon as possible.
  • Sales terms and conditions: Please review prior to ordering.
Field Specification
Mfr No ENOS-100
Assay Time
  • 40 min
Detection Method
  • Colorimetric (OD 540 nm)
Product Type
  • Assay Kits
  • Enzyme Activity
Sample Type(s) Biological
Shipping Cold pack (ICE) — Ships on ice (cold pack included). Store immediately upon receipt.
Species All
Storage -20°C — Store at -20°C (freezer). Avoid repeated freeze-thaw cycles.

Overview

For quantitative determination of nitric oxide synthase (NOS) activity and screen for NOS inhibitor. The assay uses OD540nm for signal readout. Compatible sample input includes Biological. Typical stated assay timing is 40 min.

Key elements and design rationale

  • Readout format: OD540nm supports plate-based signal acquisition and consistent comparison across matched samples.
  • Sample compatibility: The stated sample scope includes Biological, which is useful when aligning matrix type with calibration and control design.
  • Analytical range context: The supplied specifications include a stated detection limit of 0.25 U/L for interpreting low-signal samples.
  • Feature emphasis: Sensitive and accurate. Detection range 0.25 – 25 U/L in a 96-well plate.

Additional feature notes highlight Rapid and reliable. Can be completed in 40 min if the reduction of NO 3 – to NO 2 – is performed at 60°C. Available format information for this listing includes 100 Tests.

Biological background

This product is centered on measurement of nitric oxide synthase within the matrices described for the assay. In practice, datasets from this type of format are typically interpreted by comparing relative signal, activity, or abundance across matched control and experimental groups rather than relying on a single value in isolation. Careful alignment of sample matrix, incubation window, and calibration strategy is important when comparing results across plates, operators, or study days.

More details

Nitric oxide (NO) is a reactive radical that plays an important role in many key physiological functions. NO, an oxidation product of arginine by nitric oxide synthase (NOS), is involved in host defense and development, activation of regulatory proteins, and direct covalent interaction with functional biomolecules. Simple, direct, and non-radioactive procedures for measuring NOS are becoming popular in Research and Drug Discovery. BioAssay Systems EnzyChrom™ Nitric Oxide Synthase Assay Kit involves two steps: a NOS reaction step during which NO is produced followed by an NO detection step. Since the NO generated by NOS is rapidly oxidized to nitrite and nitrate, the NO production is measured following the reduction of nitrate to nitrite using an improved Griess method. The procedure is simple and the time required for sample pretreatment and assay is reduced to as short as 40 min.

Detection method

Colorimetric (OD 540 nm).

Detection limit and analytical sensitivity

Reported detection limit: 0.25 U/L.

Procedures and timing

Stated procedure or timing information: 40 min.

Research relevance and current trends

  • Plate-based quantification and side-by-side group comparison remain central use cases for this assay format.
  • The product notes emphasize multi-sample throughput, making it relevant for screening-oriented and larger batch comparison studies.
  • The description supports intervention-focused study designs in which researchers compare baseline and perturbed conditions.

Common research applications

  • Quantify nitric oxide synthase in biological by OD540 nm readout.
  • Compare treatment or phenotype groups using matched biological handling.
  • Monitor time-course or pre/post changes in biological across study conditions.

Interpretation is usually strongest when signal changes are assessed alongside matrix-matched controls, replicate agreement, and the assay's stated analytical window.

Notes for experimental interpretation

  • Matrix composition, background signal, and sample handling can influence apparent response; compare like-with-like whenever possible.
  • Use appropriate blanks, controls, and replicate wells to distinguish biological differences from plate, reagent, or handling variability.

For laboratories requiring additional technical capacity, we provide scientific support services including assay execution, method guidance, product sourcing, and customization to align the assay with specific experimental objectives. If you need assistance selecting the appropriate kit configuration, adapting the workflow to your application, or identifying related research services, please click Talk to a Scientist, email support@biohippo.com, or review our Research Services; a member of our scientific team will follow up with recommendations tailored to your study.

The effects of calorie restriction and exercise on age-related alterations in corpus cavernosum

Macit, C et al (2020). The effects of calorie restriction and exercise on age-related alterations in corpus cavernosum. Frontiers in Physiology, 11. Assay: Nitric Oxide Synthase in rat tissue.

Minocycline Protection against Paraquat Toxicity in Drosophila melanogaster

Bonilla, E., Medina-Leendertz, S., Mora, M., Vielma, J. R., Atencio-Bracho, L., Bravo, Y. & Arcaya, J. L. (2017). Minocycline Protection against Paraquat Toxicity in Drosophila melanogaster. Toxicology International, 24(1), 65-73. Assay: Nitric oxide synthase in mice brain tissue.

Pleiotropic effects of linagliptin monotherapy on levels of nitric oxide, nitric oxide synthase, and superoxide dismutase in hemodialysis patients with diabetes

Kimura, K. et al (2016). Pleiotropic effects of linagliptin monotherapy on levels of nitric oxide, nitric oxide synthase, and superoxide dismutase in hemodialysis patients with diabetes. The Showa University Journal of Medical Sciences, 28(1), 9-17. Assay: Nitric oxide synthase in angus steer serum.

The role of BATF2 in LPS/IFNgamma polarized macrophages

Gehman, MA (2015). The role of BATF2 in LPS/IFNgamma polarized macrophages. Theses and Dissertations-Microbiology, Immunology, and Molecular Genetics 10: 1-205. Assay: Nitric oxide synthase in mice macrophages.

Amelioration of lead- and cadmium-induced rat tracheal hypercontraction by linalool and eugenol

Hiba S et al (2014). Amelioration of lead- and cadmium-induced rat tracheal hypercontraction by linalool and eugenol. Toxicological & Environmental Chemistry 96(2): 307-317. Assay: Nitric oxide synthase in rat tissue.

Amelioration of lead- and cadmium-induced rat tracheal hypercontraction by linalool and eugenol

Shabir, H et al (2014). Amelioration of lead- and cadmium-induced rat tracheal hypercontraction by linalool and eugenol. Tox. & Environ. Chem. 96(2):307-317 Assay: Nitric oxide synthase in rat tissue.

Amelioration of lead- and cadmium-induced rat tracheal hypercontraction by linalool and eugenol

Shabir, H et al (2014). Amelioration of lead- and cadmium-induced rat tracheal hypercontraction by linalool and eugenol. Tox. & Environ. Chem. 96(2):307-317 Assay: Nitric Oxide Synthase in rat tissue.

Hydrogen sulfide promotes nitric oxide production in corpus cavernosum by enhancing expression of endothelial nitric oxide synthase

Meng, JP (2013). Hydrogen sulfide promotes nitric oxide production in corpus cavernosum by enhancing expression of endothelial nitric oxide synthase. International journal of impotence research 25.3: 86-90. Assay: Nitric oxide synthase in rat Corpus Cavernosum Tissue.

Get a Quote

Please use this form for bulk quantity requests or customized products.

Contact Information

Product Information

Try Celltrypse Free – Request Your Sample Today

Experience the power of Celltrypse™, c-LEcta's innovative enzyme solution for gentle and efficient cell dissociation. Request your free sample and discover a superior alternative for your cell culture workflows.

Try Celltrypse Free – Request Your Sample Today

Try Celltrypse Free – Request Your Sample Today

Experience the power of Celltrypse™, c-LEcta's innovative enzyme solution for gentle and efficient cell dissociation. Request your free sample and discover a superior alternative for your cell culture workflows.

Try Celltrypse Free – Request Your Sample Today