SKU: 46289626160

UniOne® TR-FRET Human IL33/ST2 Binding Kit

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Description

UniOne® TR-FRET Human IL33/ST2 Binding KitProduct Specification Host Human Stability & Storage 80 Background The reagent kit employs homogeneous time resolved fluorescence technology (TR FRET) for measuring the interaction between Human IL33 (Interleukin 33) and Human ST2 (also known as IL1RL1, Interleukin 1 Receptor Like 1). This method enables simple and rapid high throughput screening of inhibitors and antibody blockers. As illustrated, the interaction between IL33 and ST2 is detected

Product Specification


Host Human
Stability & Storage

-80℃

Background

The reagent kit employs homogeneous time-resolved fluorescence technology (TR-FRET) for measuring the interaction between Human IL33 (Interleukin-33) and Human ST2 (also known as IL1RL1, Interleukin 1 Receptor Like 1). This method enables simple and rapid high-throughput screening of inhibitors and antibody blockers.

As illustrated, the interaction between IL33 and ST2 is detected using Eu-labeled anti-Tag1 antibody (TR-FRET donor) and Accepter-labeled Tag2 antibody (TR-FRET acceptor). The binding of IL33 and ST2 brings the donor and acceptor antibodies into proximity, allowing the excitation of the donor antibody to trigger fluorescence resonance energy transfer (FRET) to the acceptor antibody, resulting in a specific emission signal at 665 nm. The positive control drug Itepekimab blocks the binding of IL33 and ST2, preventing FRET signal generation. The stronger the blocking effect of the screened drug on the IL33-ST2 interaction, the lower the signal. The signal is proportional to the degree of IL33-ST2 interaction. No washing steps are required.

Components

组分

浓度

100T

500T

2500T

10000T

储存温度

Tag1-ST2 protein

100 ×

5μL

20μL

100μL

400μL

-80℃

Tag2- IL33 protein

100 ×

5μL

20μL

100μL

400μL

-80℃

Eu-anti-Tag1

50 ×

10μL

50μL

250μL

1000μL

-80℃

Ac-anti-Tag2

12.5 ×

40μL

200μL

1mL

4mL

-80℃

Detection buffer

10 ×

400μL

2mL

10mL

40mL

-80℃


Protocol

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1. Reagent Preparation

1.1 Thaw all reagents at room temperature before use (equilibrate for at least 30 min). The reaction system for 384-well shallow plates is 20μL (reagent volumes are shown in the table below). Calculate the required volume before preparation and prepare accordingly. The following preparation is for reference only, using 500 reactions as an example.

Table 1. Reagent Preparation

Reagent Name

Preparation

Volume per Well (μL)

Detection buffer

Take 2 mL of 10× Detection buffer and add 18 mL deionized water to dilute to 1×. Mix well.

-

Tag1-ST2 protein

Take 20 μL of 100× Tag1-ST2 protein stock and add to 1.98 mL 1× Detection buffer to dilute to 1×. Mix well.

4μL

Tag2-IL33 protein

Take 20 μL of 100× Tag2-IL33 protein stock and add to 1.98 mL 1× Detection buffer to dilute to 1×. Mix well.

4μL

Detection Mix

Take 50 μL of 50× Eu-anti-Tag1 stock and add 2.45 mL 1× Detection buffer to dilute to 2.5 mL. Mix well;

Take 200 μL of 12.5× Ac-anti-Tag2 stock and add 2.30 mL 1× Detection buffer to dilute to 2.5 mL. Mix well;

Mix the two solutions 1:1 to prepare the Detection Mix.

10μL


1.2 Sample Serial Dilution

Using Itepekimab as an example, dilute with 1× Detection buffer. To minimize matrix interference, it is recommended to use a solution with the same matrix as the sample. Adjust dilution based on actual sample concentration.

Table 2. Serial Dilution of Positive Control (Itepekimab) (Adjust as needed)

Final Conc. (nM)

Prep. Conc. (nM)

Preparation Method

100.000

1000.000

2 μL of 10 μM stock + 18 μL 1× Detection buffer

25.000

250.000

5 μL of ① + 15 μL 1× Detection buffer

6.250

62.500

5 μL of ② + 15 μL 1× Detection buffer

1.563

15.625

5 μL of ③ + 15 μL 1× Detection buffer

0.391

3.906

5 μL of ④ + 15 μL 1× Detection buffer

0.098

0.977

5 μL of ⑤ + 15 μL 1× Detection buffer

0.024

0.244

5 μL of ⑥ + 15 μL 1× Detection buffer

0.006

0.061

5 μL of ⑦ + 15 μL 1× Detection buffer

Blank

0

0

20 μL 1× Detection buffer


2. Sample Loading and Controls

2.1 Sample wells: Add sequentially to 384-well shallow plates—2 μL diluted sample, 4 μL Tag2-IL33 protein working solution, 4 μL Tag1-ST2 protein working solution, and 10 μL Detection Mix.

2.2 Maximum signal control: Add sequentially—2 μL 1× Detection buffer, 4 μL Tag2-IL33 protein working solution, 4 μL Tag1-ST2 protein working solution, and 10 μL Detection Mix.

2.3 Negative control (NC): Add sequentially—10 μL 1× Detection buffer and 10 μL Detection Mix.

After loading, centrifuge and seal with plate film. Incubate at room temperature for 2 hours.

Sample

Max Signal Control

Negative Control (NC)

Step 1

2 μL sample

2 μL 1× Detection buffer

10 μL 1× Detection buffer

4 μL Tag2-IL33 protein working solution

Incubate at RT for 10 min

Step 2

4 μL Tag1-ST2 protein working solution

10 μL Detection Mix

Seal and incubate at RT for 2 h


3.Detection

Read on a TR-FRET-compatible microplate reader. Excitation wavelength: 320/340 nm; emission wavelengths: 620 nm and 665 nm.

[Data Analysis]

1) Calculate signal ratio (Ratio): Divide 665 nm fluorescence by 620 nm fluorescence, then multiply by 10,000.

Ratio = (665/620) × 10000

2) Calculate Net signal:

Net signal = (Std - NC)/NC × 100

3) Calculate CV (%):

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

[Example Data]

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

Note: Recommended microplate (384-well, white, shallow)

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Lowell, US
★★★★★ 5
One wild night you can't remember brings bad choices to the surface- only in Vegas it's a future.
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I recieved an ARC copy of this book and was delighted with all the feels. A crazy meet in Vegas and one wild night changes so many lives. Drew carries the weight of so much and trusts no one. Relationships are not her strong trait. A Wyoming ranch girl at a rodeo trying to win a contest to save the ranch. She meets Maisie who is a straight girl that catches her hatwhen it flies off Drew's head. Sparks fly and a connection is felt. They bump into each other couple more times and end time in Vegas with one forgotten wild night. I rode a wonderful bunch of feels with this book. I yelled more than once at these characters who clearly cared for each other but could not get out of their own way. So stubborn and full of false bravado I just want them to share thoughts. It was a delicate balance to navigate the mine field which was their past and the surprise that is their future. The best part of the story was watching how love was changing everyone on the ranch. They give new meaning to running away from your feelings. It was a sweet, often funny and challenging romance. I was curious how or if they would find ways to share feelings. It kept me turning pages just to see what was next. I really enjoyed the characters and the ranch life. A good stranger to lover and then get to know you story.
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Reviewed in the United States on March 26, 2022
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Raven reads
Birmingham, US
★★★★★ 4
Cute
Format: Kindle
I enjoyed this story much more than I expected to. Maisie and Drew couldn’t be more different in many ways but they make a good pair. Both women are stubborn and determined and they butt heads more than once but that is ultimately what makes them work. This is a good sapphic story and is worth a read.
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Carina
Pawtucket, US
★★★★★ 5
Great story
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Well developed characters and great story. What happens in Vegas does not stay in Vegas. I will highly recommend this book.
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Emily G
West Palm Beach, US
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Everything
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TB Markinson + Miranda MacLeod = winning combination. This book was everything I needed. To be fair, having read their previous collaborations, as soon as I saw this book I hit "buy" without even paying much attention to the blurb. I was not disappointed. When I eventually got around to reading the blurb (post-purchase) I was even more excited to read it. The storyline was great, the story well-written, the characters quite likeable and relatable and all in all a great book. I went through all the feels with this: there were parts that made me laugh, parts where I had to put it down because I really wanted to shake the characters, parts where I went "awww" and couldn't hold back a tear. So, long story short, read this book, you won't regret it
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Sabra
Cuba, US
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Loved this story.
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First things first. Will there be a sequel, ladies? Perhaps children for Maisie and Drew? Hannah finding a woman to love? I really loved this story. Horses, critters, angst and some good lovin’. What more could a woman ask for? Well done you two. You made this old broad pine for a ranch and a lovely cowgirl.
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Reviewed in the United States on December 29, 2024

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