Mouse Lipocalin-2/NGAL ELISA Kit PicoKine®

SKU:BHE21000659
Overview
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Mouse Lipocalin-2/NGAL (LCN2) PicoKine® Quick ELISA kit is designed for quantitative detection of Lipocalin-2/NGAL. Suitable for cell culture supernatants, serum, plasma (heparin, EDTA) and urine. Optimized for a streamlined sandwich ELISA workflow with high signal-to-noise and reproducible results. Reported sensitivity: <10 pg/ml.
Target LCN2
Reactivity Mouse
Sample Type(s) cell culture supernatants, serum, plasma (heparin, EDTA) and urine.
Assay Type Sandwich ELISA
Sensitivity <10 pg/ml
Detection Range 78 pg/ml - 5,000 pg/ml
Assay Time ~3.5 hours
Options selector
Catalog no. Size
EK0854 96 wells/kit, with removable strips.
Available Options

Select from the available variant options shown for this product. Availability and lead time may vary by option.

  • Options: Size: 96 wells/kit, with removable strips..
  • Lead time: items “in stock at manufacturer” typically ship in 5–7 business days.
  • Storage: Store at 4℃ for 6 months, at -20℃ for 12 months. Avoid multiple freeze-thaw cycles (Ships with gel ice, can store for up to 3 days in room temperature. Freeze upon receiving.); cold-chain shipment (typically with ice packs) is expected.
  • Please ensure someone is available to receive temperature-sensitive deliveries promptly.
  • Sales terms and conditions: Please review prior to ordering.
Field Specification
Mfr No EK0854
Alternative Names Neutrophil gelatinase-associated lipocalin;NGAL;Lipocalin-2;SV-40-induced 24P3 protein;Siderocalin LCN2;p25;Lcn2;
Assay Time
  • ~3.5 hours
Assay Type
  • Sandwich ELISA
Detection Range 78 pg/ml - 5,000 pg/ml
Expression System
  • NS0
Gene ID 16819
Immunogen Expression system for standard: NS0; Immunogen sequence: Q21-N200
Product Type
  • ELISA Kits
  • PicoKine® ELISA Kitss
Reactivity
  • Mouse
Sample Type(s) cell culture supernatants, serum, plasma (heparin, EDTA) and urine.
Sensitivity <10 pg/ml
Storage Store at 4℃ for 6 months, at -20℃ for 12 months. Avoid multiple freeze-thaw cycles (Ships with gel ice, can store for up to 3 days in room temperature. Freeze upon receiving.)
Target LCN2
UniProt # P11672

Background

Also known as: Neutrophil gelatinase-associated lipocalin, NGAL, Lipocalin-2, SV-40-induced 24P3 protein, Siderocalin LCN2, p25, Lcn2.

Mouse Lipocalin-2/NGAL (LCN2) is widely studied as a molecular readout in experimental models where changes in protein abundance reflect underlying biology. This target is frequently investigated in Molecular & Cellular Biology research contexts. Cytokines and chemokines act as soluble messengers that coordinate immune cell activation, trafficking, and effector functions. Their concentrations can change rapidly in response to infection, tissue injury, or immune stimulation.

Biological function and signaling context

In immune signaling networks, cytokine production is often induced by pattern-recognition pathways and inflammatory transcriptional programs, while feedback regulators can dampen responses to restore homeostasis. Chemokine gradients guide leukocyte migration, influencing which cell populations accumulate at a site and how long they persist.

Why it matters in research

  • Immune activation readout: Shifts in abundance can reflect pathway engagement and cellular activation state.
  • Microenvironment profiling: Levels can help characterize inflammatory tone in tissues or biofluids.
  • Response monitoring: Time-course measurements support interpretation of stimulus, treatment, or infection models.

Disease and translational relevance

Many cytokines and chemokines are reported to associate with inflammatory, autoimmune, infectious, and oncology-related processes. In research settings, interpreting changes benefits from pairing this analyte with complementary markers (e.g., upstream triggers, downstream effectors, and cell-type indicators) and considering matrix effects.

Sample data

Concentration (pg/ml)078156312625125025005000
O.D.0.0170.0730.1230.2270.3760.7171.3552.128

Intra/inter assay consistency

Intra-Assay PrecisionInter-Assay Precision
Sample123123
n161616242424
Mean (pg/ml)14178525881308172606
Standard deviation6.238.46113.877.5454.73161.57
CV (%)4.4%4.9%4.4%5.8%6.7%6.2%

Kit components

Description|Quantity Pre-coated 96-well strip microplate|1 Standard|2 vials Biotinylated antibody (100x)|100ul Avidin-Biotin-Peroxidase Complex (100x)|100ul Sample Diluent|30ml Antibody Diluent|12ml Avidin-Biotin-Peroxidase Diluent|12ml Color Developing Reagent (TMB)|10ml Stop Solution|10ml Wash Buffer (25x)|20ml Adhesive plate sealers|4

Materials required but not provided

  • Microplate Reader capable of reading absorbance at 450nm.
  • Incubator.
  • Automated plate washer (optional).
  • Pipettes and pipette tips capable of precisely dispensing 0.5 µl through 1 ml volumes of aqueous solutions.
  • Multichannel pipettes are recommended for large amount of samples.
  • Deionized or distilled water.
  • 500ml graduated cylinders.
  • Test tubes for dilution.
How many samples can I run per plate?
Each PicoKine® kit (96-well format) typically accommodates a 7-point standard curve in duplicate, 2 non-specific binding wells, and up to 39 unknown samples in duplicate. Exact capacity may vary by kit — refer to the datasheet.
What sample dilution should I use?
Boster recommends performing a pilot study first: run serial dilutions of your samples (e.g. 1:2, 1:4, 1:8, 1:16) to identify the range that falls within the standard curve. This is important because sample matrix and protein expression levels vary significantly by experiment.
Why is my signal weak or absent?
The most common causes are: (1) target protein below the kit's detection limit — try concentrating samples or reducing dilution; (2) reagents not at room temperature before use; (3) insufficient incubation time; (4) expired or contaminated reagents. See Boster's full ELISA troubleshooting guide at bosterbio.com/protocol-and-troubleshooting/picokine-elisa-troubleshooting.
Why is my background signal high?
High background is typically caused by insufficient washing (ensure thorough plate draining after each wash step), excess antibody concentration, or contaminated TMB substrate. Increase the number of wash cycles or reduce antibody concentration. Always use fresh substrate solution.
Are the kit components sterile?
Components are bottled using aseptic techniques and heat-treated vials, but are not guaranteed sterile. If your experiment requires sterile material, filter through a 0.2 µm membrane designed for biological fluids before use.
How do I analyze my ELISA results?
Plot absorbance (OD 450 nm) against standard concentrations and fit a 4-parameter logistic (4PL) or sigmoidal curve. Read unknown sample concentrations from the curve. Boster provides a free online ELISA data analysis tool at bosterbio.com/biology-research-tools/elisa-data-analysis-online.
How should I store samples before running the assay?
Aliquot samples before freezing to avoid repeated freeze-thaw cycles, which can degrade the target protein. Store aliquots at -80°C for long-term use. Serum and plasma should be collected, processed, and stored under consistent conditions to minimise pre-analytical variability.
What positive and negative controls should I include?
Include a positive control (a sample known to contain the target protein at a measurable level) and a negative control (sample matrix without the target, or a sample from a species the kit does not cross-react with). Running controls in every assay validates the assay performance and flags plate-to-plate variability.

Can’t Find What You’re Looking For? We can help you source the best match or customize an ELISA solution for your study. Options may include alternative target synonyms, different species reactivity, sample type/matrix compatibility (serum/plasma/lysate/supernatant), assay format (sandwich/competitive), sensitivity/range, detection chemistry (colorimetric/fluorescent/chemiluminescent), plate format (pre-coated/uncoated, strips vs full plate), and bulk or custom packaging. Click Talk to a Scientist to submit a request form, email us at support@biohippo.com, or explore our Research Services for additional support. Our team will be in contact with you shortly.

  1. Jin et al. (2025). Single-Cell RNA Sequencing Analysis Reveals the Role of Macrophage-Mediated CD44–AKT–CCL2 Pathways in Renal Tubule Injur…. Research.
  2. Fan et al. (2025). S-nitrosoglutathione inhibits pyroptosis of kidney tubular epithelial cells in sepsis via the SIRT3/SOD2/mtROS signaling…. RENAL FAILURE.
  3. Liping et al. (2025). Narciclasine attenuates sepsis-associated acute kidney injury through the ESR1/S100A11 axis. FUNCTIONAL & INTEGRATIVE GENOMICS.
  4. Ting et al. (2022). Astrocytic phagocytosis contributes to demyelination after focal cortical ischemia in mice. Nature Communications.
  5. Chen et al. (2020). Ischemic postconditioning attenuates acute kidney injury following intestinal ischemia-reperfusion through Nrf2-regulate…. FASEB JOURNAL.
  6. Qianqian et al. (2019). Lipocalin 2 Protects Against Escherichia coli Infection by Modulating Neutrophil and Macrophage Function. Frontiers in Immunology.
  7. Gupta et al. (2019). Gut IgA abundance in adult life is a major determinant of resistance to dextran sodium sulfate-colitis and can compensat…. IMMUNOLOGY.
  8. Zhang et al. (2019). A Multifunctional Nanotherapy for Targeted Treatment of Colon Cancer by Simultaneously Regulating Tumor Microenvironment. Theranostics.
  9. Pei et al. (2018). Protective role of fenofibrate in sepsis-induced acute kidney injury in BALB/c mice. RSC Advances.
  10. Tani et al. (2015). AB0166 The Effect of a Treatment with Allogenic Mesenchimal Stromal Cells (MSCS) on Urinary Biomarkers in a Mouse Model …. ANNALS OF THE RHEUMATIC DISEASES.
  11. Sun et al. (2013). Protective Effect of Ginsenoside Rb1 against Intestinal Ischemia-Reperfusion Induced Acute Renal Injury in Mice. PLoS One.
  12. Gu et al. (2025). Chronic Low-Dose Cadmium Exposure Disrupts Gut Microbiota and Lipid Metabolism to Induce Liver Injury. FOOD AND CHEMICAL TOXICOLOGY.
  13. Huang et al. (2025). Lipocalin-2 regulates astrocyte-oligodendrocyte interaction to drive post-stroke secondary demyelination. Cell Reports.
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