| Field | Specification |
|---|---|
| Mfr No | |
| Alternative Names | L-selectin;CD62 antigen-like family member L;Leukocyte adhesion molecule 1;LAM-1;Leukocyte surface antigen Leu-8;Leukocyte-endothelial cell adhesion molecule 1;LECAM1;Lymph node homing receptor;TQ1;gp90-MEL;CD62L;SELL;LNHR, LYAM1; |
| Assay Time | |
| Assay Type | |
| Detection Range | |
| Expression System | |
| Gene ID | |
| Immunogen | Expression system for standard: NS0; Immunogen sequence: W39-N332 |
| Product Type | |
| Reactivity | |
| Sample Type(s) | cell culture supernatants, serum and plasma (heparin, EDTA, citrate) |
| Sensitivity | |
| Storage | |
| Target | |
| UniProt # |
Background
Also known as: L-selectin, CD62 antigen-like family member L, Leukocyte adhesion molecule 1, LAM-1, Leukocyte surface antigen Leu-8, Leukocyte-endothelial cell adhesion molecule 1, LECAM1, Lymph node homing receptor.
Human sL-Selectin (SELL) 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. This analyte is often discussed in the context of cell-surface signaling and cell-state markers. Many receptors and surface markers act as gateways for signaling or as phenotypic indicators of specific cell populations and activation states.
Biological context
In experimental systems, protein abundance can reflect regulated expression, secretion, processing, or clearance. Interpreting changes benefits from considering compartment (cell-associated vs soluble), the time scale of regulation, and whether complexes or modified forms contribute to the measured signal.
Why it matters in research
- Systems-level readout: Quantification supports comparisons across conditions, time points, and treatment groups.
- Mechanistic interpretation: Pairing with upstream regulators and downstream markers helps contextualize changes.
- Biomarker-style profiling: Measuring panels of related analytes can improve interpretability in complex models.
Sample data
| Concentration (pg/ml) | 0 | 62.5 | 125 | 250 | 500 | 1000 | 2000 | 4000 |
| O.D. | 0.011 | 0.262 | 0.446 | 0.852 | 1.492 | 2.205 | 2.476 | 2.617 |
Intra/inter assay consistency
| Intra-Assay Precision | Inter-Assay Precision | |||||
|---|---|---|---|---|---|---|
| Sample | 1 | 2 | 3 | 1 | 2 | 3 |
| n | 16 | 16 | 16 | 24 | 24 | 24 |
| Mean (pg/ml) | 1187 | 543 | 1239 | 187 | 595 | 1352 |
| Standard deviation | 17.8%1 | 33.66 | 60.71 | 16.64 | 37.48 | 67.6 |
| CV (%) | 7.8% | 6.2% | 4.9% | 8.9% | 6.3% | 5% |
Kit components
Description|Quantity|Volume Anti-tag Pre-coated 96-well Strip Microplate|1|12 strips of 8 wells Standard||2 Antibody A|1|3ml Antibody B|1|3ml Sample Diluent|1|15ml TBS-T Wash Buffer (25x)|1|12ml Color Developing Reagent (TMB)|1|10ml Stop Solution|1|10ml Adhesive Plate Sealers|2|PieceMaterials required but not provided
- Microplate Reader capable of reading absorbance at 450nm.
- 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.
- Horizontal orbital microplate shaker capable of maintaining a speed of 500 rpm, amplitude 3mm.
►How does PicoKine® Quick ELISA differ from standard PicoKine®?
►How many samples can I run per plate?
►Can I extend the 90-minute incubation to improve sensitivity?
►Why is my Quick ELISA signal weak?
►Are the kit components sterile?
►How do I interpret and analyse the standard curve?
►What sample preparation is recommended for Quick ELISA?
►Can Quick ELISA kits be used interchangeably with standard PicoKine® kits for the same target?
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