SKU: 46299405497

Anti-GST Tag Acceptor Beads

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Description

Anti-GST Tag Acceptor BeadsProduct Specification Stability & Storage Store at 28C away from light; product shelf life is 12 months. Background Homogeneous Immuno Chemiluminescence Assay (HICA) is a homogeneous immunoassay method based on energy transfer between donor beads and acceptor beads at close proximity to generate luminescence. Donor beads recognize protein 1 (Tag1 label), and acceptor beads recognize protein 2 (Tag2 label). When protein 1 binds to protein 2, the

Product Specification


Stability & Storage

Store at 2~8°C away from light; product shelf life is 12 months.

Background

Homogeneous Immuno Chemiluminescence Assay (HICA) is a homogeneous immunoassay method based on energy transfer between donor beads and acceptor beads at close proximity to generate luminescence.

Donor beads recognize protein 1 (Tag1 label), and acceptor beads recognize protein 2 (Tag2 label). When protein 1 binds to protein 2, the distance between the beads becomes less than 200nm. Upon excitation at 680nm, the donor beads generate singlet oxygen, which diffuses to the acceptor beads. The acceptor beads then undergo a redox reaction, emitting light at 615nm. The signal intensity is directly proportional to the strength of the protein interaction.

This product features a simple operation process, requires no washing, and offers fast results with high sensitivity. It is capable of detecting weak interactions.

Components

Specification

Fill Volume

250 μg

50 μL

5 mg

1 mL

25 mg

1 mL x 5


Protocol

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【Required Reagents】

Name

Catalog No.

Anti-GST Tag Acceptor Beads UA086102
Streptavidin Donor Beads UA086104
Universal Buffer 1 UA086113


 

【Detection Procedure (For Reference)】

Detection Steps

Procedure 1 (37°C Rapid Detection)

Procedure 2 (Room Temperature Detection)

Step 1:

4μL Tag1-M1 +4μL Tag2-M2+ 6μL Acceptor Beads,Light-protected/Green light

4μL Tag1-M1 +4μL Tag2-M2+ 6μL Acceptor Beads,Light-protected/Green light

Incubation

​37°C shaking incubation for 20 minutes,Light-protected/Green light

​Room temperature incubation for 60 minutes,Light-protected/Green light

Step 2:

Add 6μL Donor Beads,Light-protected/Green light

Add 6μL Donor Beads,Light-protected/Green light

Incubation

​37°C shaking incubation for 10 minutes,Light-protected/Green light

​Room temperature incubation for 30 minutes,Light-protected/Green light

Readout

Instrument readout

Instrument readout


 

【Performance Validation】

Sample Preparation:

Biotinylated GST (Bio-GST) was pre-diluted to 8.1μg/mL (300nM) using Universal Buffer 1 as the stock solution, followed by serial dilution as below:

ID

Final Concentration (nM)

Universal Buffer 1

Volume (μL)

High Concentration Addition

Volume (μL)

C12

1.0E+01

270

30μL stock

C11

3.0E+00

210

90μL C12

C10

1.0E+00

180

90μL C11

C9

3.0E-01

210

90μL C10

C8

1.0E-01

180

90μL C9

C7

3.0E-02

210

90μL C8

C6

1.0E-02

180

90μL C7

C5

3.0E-03

210极p>

90μL C6

C4

1.0E-03

180

90μL C5

C3

3.0E-04

210

90μL C4

C2

1.0E-04

180

90μL C3

C1

0

180

/


 

Detection Reagent Preparation:

Name

Preparation Concentration

Diluent

Anti-GST Tag Acceptor Beads

25 μg/mL

Universal Buffer 1

Streptavidin Donor Beads

25 μg/mL

Universal Buffer 1


 

 

37°C Incubation Mode Results:

 

Max signal: 1142982

Min signal: 644

EC50= 0.8679nM

Room Temperature Incubation Mode Results:

Max signal: 438266

Min signal: 295

EC50= 0.8027nM

```

Guidelines

1. This experiment is light-sensitive; ensure all operations are performed in the dark. It is recommended to carry out preparation, sample loading, and incubation steps under green light (illuminance below 100 LUX). 2. This product is compatible with multifunctional microplate readers equipped with an Alpha detection module. 3. Vortex thoroughly before use. Alternatively, briefly centrifuge (2000×g, 5–10 seconds) to ensure complete retrieval. 4. It is recommended to use the company's配套 diluent for reagent preparation and sample dilution. If additional components are required, they can be directly added to this diluent. 5. To ensure comparability of experimental data across different batches, strictly control incubation temperature and duration. 6. Avoid generating bubbles during sample loading.
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