UA-Blue SEAP Detection Kit

Secreted Alkaline Phosphatase (SEAP) is widely used in reporter gene analysis studies. Its advantage is that it only requires the analysis of cell culture supernatant, without the need to lyse cells. Moreover, SEAP is relatively heat-resistant and has a high tolerance for specific alkaline phosphatase inhibitors. Therefore, samples can be subjected to specific pre-treatment to inactivate endogenous alkaline phosphatase and eliminate interference.

The UA-Blue SEAP Detection Kit is a homogeneous ready-for-use reagent that completes the detection through the simple steps of “add-mix-detect.” This kit is used to detect alkaline phosphatase activity in the culture medium of cells transfected with the SEAP reporter gene. There is no need to lyse the cells, which can be further cultured or used for other multiplex analyses. Compared with other similar products, the detection sensitivity is at least one time higher, and the reaction time is shortened by at least one time. It is particularly suitable for the analysis of cells with low enzyme activity and the screening of inhibitory compounds.

1). Cell Seeding & Preparation

Plate cells expressing SEAP reporter gene in 96-well or 384-well plates.

If using FBS-containing medium: Heat-inactivate FBS at 56°C for 30 min to eliminate endogenous alkaline phosphatase (AP) activity.

2). Cell Treatment & Stimulation

Treat cells with test compounds and stimulate reporter gene expression as required.

3). Sample Collection & Pre-Treatment

Collect cell culture supernatant at the desired timepoint post-stimulation. For high endogenous AP background: Heat samples at 65°C for 5-10 min to inactivate interfering phosphatases (optional).

Note: The QT-Blue™ SEAP Assay Kit reagent suppresses low levels of endogenous AP without affecting SEAP activity.

4). Reagent Preparation

Equilibrate UA-Blue detection reagent to room temperature (RT) before use.

Buffer Handling (40×  Buffer)

May appear slightly turbid (no precipitate) - vortex well before dilution.

Storage: 4°C: Stable for 2 weeks; -20°C: Long-term storage

Substrate Handling (250× Substrate)

Appearance: Red-brown solution; precipitate may form during storage.

To resolubilize: Vortex vigorously for 1–2 min, OR Incubate at 37°C for 5–10 min.

Storage: 4°C: Stable for 4 weeks; -20°C: Long-term storage

5). 1× Working Solution Preparation

Example (40 mL 1× detection reagent):

- Dilute 1 mL 40× Buffer in 39 mL sterile water → 1× QB Buffer.

- Add 167 µL 250× Substrate → immediate flocculation occurs. Vortex immediately until fully dissolved (clear solution). Delay in mixing causes irreversible precipitation.

6). HTS Optimization (e.g., 1536-well plates):

Prepare 3× or 6× concentrated detection reagent to minimize pipetting steps. Example:

3× reagent (2 µL) + 4 µL sample → 1× final concentration.

Storage for 1x/3x/6x detection reagents: 4°C, stable for 1 week (may form slight precipitate; vortex before use).

7). Assay Setup (96-Well Plate Example)

- Add 20 µL sample/control per well.

- Add 180 µL 1× detection reagent.

- Mix on plate shaker (15 sec).

8). Incubation: 37°C for 30 min-6 hrs (protect from light).

9). Detection: Measure absorbance at 600-650 nm (OD) using a plate reader.

Signal Stability: Readings should be taken within 6 hr of reagent addition.

HTS Adaptation: For 384/1536-well plates, scale down volumes proportionally.

Interference Control: Heat pretreatment (65°C) is recommended for high-background samples.