SKU: 73438262103

UniOne® TR-FRET Human cGMP Detection Kit

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Description

UniOne® TR-FRET Human cGMP Detection KitProduct Specification Host Human Stability & Storage 80 Background The kit employs homogeneous time resolved fluorescence technology (TR FRET), enabling precise measurement of cellular cGMP production. This method provides a high throughput format for simple and rapid screening of molecules that modulate phosphodiesterase activity. As illustrated, biotin labeled cGMP can bind to streptavidin (SA), while the Eu labeled anti cGMP antibody (TR FRET

Product Specification


Host Human
Stability & Storage

-80℃

Background

The kit employs homogeneous time-resolved fluorescence technology (TR-FRET), enabling precise measurement of cellular cGMP production. This method provides a high-throughput format for simple and rapid screening of molecules that modulate phosphodiesterase activity.

As illustrated, biotin-labeled cGMP can bind to streptavidin (SA), while the Eu-labeled anti-cGMP antibody (TR-FRET donor) and the Ac-labeled anti-Tag2 antibody (TR-FRET acceptor) bind to cGMP and biotin, respectively. The proximity of the donor and acceptor antibodies allows the excitation of the donor antibody to trigger fluorescence resonance energy transfer (FRET) to the acceptor antibody, resulting in a specific 665 nm emission signal. When cGMP is present in cell samples or standard curves, it competes with biotin-labeled cGMP for binding to the Eu-labeled anti-cGMP antibody, thereby reducing the FRET signal. This specific signal is proportional to the degree of interaction between the Eu-labeled anti-cGMP antibody, biotin-labeled cGMP, and SA. This homogeneous assay is simple to perform and requires no washing steps.

Components

Component

Concentration

100T

500T

2500T

10000T

Storage Temperature

Biotin-cGMP protein

100×

5μL

12.5μL

62.5μL

250μL

-80℃

cGMP calibrator

500μM

5μL

5μL

25μL

100μL

-80℃

Anti-cGMP Eu antibody

100×

L

25μL

125μL

500μL

-80℃

SA-Ac

12.5×

20μL

100μL

500μL

2mL

-80℃

Lysis & Detect Buffer

1×

2mL

10mL

50mL

200mL

-80℃

Stimulation Buffer (without IBMX)

1×

2mL

10mL

50mL

200mL

-80℃


Protocol

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1. Reagent Preparation

1.1 Thaw all reagents to room temperature before use. The reaction system for the 384-well plate is 20μL (reagent volumes are shown in the table below). Calculate the required volume before preparation. The following preparation is for reference only, using 500 reactions as an example.

Table 1. Reagent Preparation and Volumes

Reagent Name

Preparation

Volume per Well (μL)

Anti-cGMP Eu antibody

Take 25μL of Anti-cGMP Eu antibody stock solution and dilute to 2.5mL with Lysis & Detect Buffer, mix well.

5μL

cGMP Ac Mix

Take 12.5μL of Biotin-cGMP protein stock solution and dilute to 1.25mL with Lysis & Detect Buffer, mix well; take 100μL of SA-Ac stock solution and add to 1.25mL of Lysis & Detect Buffer, mix well. Mix the diluted Biotin-cGMP protein and SA-Ac in a 1:1 ratio to prepare the cGMP Ac Mix.

5μL


 

1.2 Gradient Dilution of Test Samples

Prepare according to experimental requirements. The following is for reference only.

Using cGMP calibrator as an example, the dilution buffer is Stimulation Buffer. Adjust the sample concentration as needed.

Table 2. cGMP Calibrator Preparation

 

Final Concentration (nM)

Preparation Concentration (nM)

Preparation Method

1

1,250.000

5,000.000

1μL of 500μM stock + 99μL Stimulation Buffer

2

416.667

1,666.667

20μL of ① + 40μL Stimulation Buffer

3

138.889

555.556

20μL of ② + 40μL Stimulation Buffer

4

46.296

185.185

20μL of ③ + 40μL Stimulation Buffer

5

15.432

61.728

20μL of ④ + 40μL Stimulation Buffer

6

5.144

20.576

20μL of ⑤ + 40μL Stimulation Buffer

7

1.715

6.859

20μL of ⑥ + 40μL Stimulation Buffer

8

0.572

2.286

20μL of ⑦ + 40μL Stimulation Buffer

9

0.191

0.762

20μL of ⑧ + 40μL Stimulation Buffer

10

0.064

0.254

20μL of ⑨ + 40μL Stimulation Buffer

11

0.021

0.085

20μL of ⑩ + 40μL Stimulation Buffer

Blank

0

0

40μL of 1× Stimulation Buffer


 

1.3 Pre-Treatment for Cell-Based Experiments

① Stimulation Buffer is used to dilute cells and stimulant drugs. The Stimulation Buffer provided in the kit does not contain IBMX. If the experiment aims to quantify the final concentration of cGMP in cells, it is necessary to add an appropriate concentration of IBMX to prevent cGMP degradation. If the experiment aims to evaluate the performance of PDE inhibitors, IBMX should not be added.

② Before conducting formal experiments, determine the number of cells per well and the incubation time with drugs based on cell and drug characteristics to ensure that the cGMP levels produced by cells fall within the linear range of the calibration curve.

2. Sample Addition and Controls

2.1 cGMP Standard Curve: 5μL of gradient-diluted cGMP reference, 5μL Stimulation Buffer, 5μL Anti-cGMP Eu antibody working solution, incubate for 10min, then add 5μL cGMP Ac Mix.

2.2 Test Samples: 5μL of gradient-diluted test sample, 5μL Stimulation Buffer, 5μL Anti-cGMP Eu antibody working solution, incubate for 10min, then add 5μL cGMP Ac Mix.

2.3 Cell-Based Experiments: Based on pre-experiment results, add 5μL of cells, 5μL of gradient-diluted drug, and incubate for the determined time. After incubation, add 5μL Anti-cGMP Eu antibody working solution, incubate at room temperature for 10min, then add 5μL cGMP Ac Mix.

2.4 Negative Control (NC): 5μL Stimulation Buffer instead of test sample or 5μL of untreated cells.

 

cGMP Standard Curve

Test Samples

Cell Experiments

Negative Control (NC)

Step 1

 

5μL cGMP calibrator

5μL test sample

5μL cells

5μL Stimulation Buffer or 5μL cells

5μL Stimulation Buffer

5μL Stimulation Buffer

5μL drug※

5μL Stimulation Buffer

5μL Anti-cGMP Eu antibody working solution

Incubate at room temperature for 10min

Step 2

5μL cGMP Ac Mix

Seal the plate, centrifuge at 1000rpm for 1min to mix, incubate at room temperature for 120min, then read the plate.


 

The incubation time of cells with drugs needs to be determined experimentally. Add subsequent reagents after drug stimulation of cells.

3.Detection

Measure using a TR-FRET-compatible microplate reader. Excitation wavelength: 320/340nm, emission wavelengths: 620nm and 665nm.

【Result Calculation】

1) Calculate the signal value (Ratio): Multiply the 665nm fluorescence signal by the 620nm fluorescence signal and then by 10,000.

Ratio = (665/620) × 10,000

2) Calculate CV (%):

CV (%) = Standard Deviation / Mean Ratio × 100%

【Data Example】

The following data is for reference only and may vary depending on the plate reader used.

 

3 /3Note: *Data is for reference only. Recommended microplate: 384-well plate, white, shallow well.

 

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