Antitrypsin Activity Measurement

  • Product Code: 125877
This antitrypsin activity assay is important because it measures the ability of a sample (e.g., plant extract) to inhibit the proteolytic enzyme trypsin, which is crucial in many biological and industrial contexts (e.g., therapeutic enzyme modulation, functional food ingredient evaluation). The method uses BApNA, a chromogenic substrate that releases a yellow-colored product (p-nitroaniline) upon hydrolysis by trypsin. By comparing absorbances of control vs. sample, one can calculate the percentage inhibition of trypsin activity. Tris-HCl buffer is used instead of phosphate buffer to avoid unwanted buffer-catalyzed BApNA hydrolysis, ensuring reliable and accurate measurement.
฿2,990.00

label ชื่อตัวอย่าง

info Please add exactly one sample

assignment คำแนะนำ

info โปรดระบุข้อกำหนดหรือเงื่อนไขเฉพาะสำหรับการทดสอบ

insert_drive_file Report of Previously Tested Sample

Select a tab and click View to open the report.

timeline ขั้นตอนการให้บริการ

ขั้นตอน ขั้นตอน ผลลัพธ์ที่คาดหวัง
1

Prepare the...

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A 1 mg/mL plant extract solution ready for testing.

2

Add 40...

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Each well contains 40 µL of trypsin.
3

Add 40...

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Each well now contains 80 µL total volume: 40 µL trypsin + 40 µL sample/control.

4

Incubate the...

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Pre-incubation for trypsin inhibition reaction to occur.

5

Add 100...

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Substrate is introduced, final well volume is 180 µL.

6

Incubate the...

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Enzymatic hydrolysis of BApNA occurs (or is inhibited), generating color.

7

Add 30%...

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Reaction is halted by acidification; color development is stabilized.

8

Measure and...

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Absorbance values (OD) for control and sample wells are obtained.

9

Calculate percentage...

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Percentage inhibition result for each sample.

คุณจะได้รับรายงานสำหรับ % Inhibition of Trypsin ฟิลด์เมื่อเราให้บริการนี้

Antitrypsin Activity Measurement
This antitrypsin activity assay is important because it measures the ability of a sample (e.g., plant extract) to inhibit the proteolytic enzyme trypsin, which is crucial in many biological and industrial contexts (e.g., therapeutic enzyme modulation, functional food ingredient evaluation). The method uses BApNA, a chromogenic substrate that releases a yellow-colored product (p-nitroaniline) upon hydrolysis by trypsin. By comparing absorbances of control vs. sample, one can calculate the percentage inhibition of trypsin activity. Tris-HCl buffer is used instead of phosphate buffer to avoid unwanted buffer-catalyzed BApNA hydrolysis, ensuring reliable and accurate measurement. Sample Count: Accepts exactly 1 sample.
This antitrypsin activity assay is important because it measures the ability of a sample (e.g., plant extract) to inhibit the proteolytic enzyme trypsin, which is crucial in many biological and industrial contexts (e.g., therapeutic enzyme modulation, functional food ingredient evaluation). The method uses BApNA, a chromogenic substrate that releases a yellow-colored product (p-nitroaniline) upon hydrolysis by trypsin. By comparing absorbances of control vs. sample, one can calculate the percentage inhibition of trypsin activity. Tris-HCl buffer is used instead of phosphate buffer to avoid unwanted buffer-catalyzed BApNA hydrolysis, ensuring reliable and accurate measurement. Sample Count: Accepts exactly 1 sample.
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Service Steps
Step Procedure Expected Result
1

Prepare the...

A 1 mg/mL plant extract solution ready for testing.

2

Add 40...

Each well contains 40 µL of trypsin.
3

Add 40...

Each well now contains 80 µL total volume: 40 µL trypsin + 40 µL sample/control.

4

Incubate the...

Pre-incubation for trypsin inhibition reaction to occur.

5

Add 100...

Substrate is introduced, final well volume is 180 µL.

6

Incubate the...

Enzymatic hydrolysis of BApNA occurs (or is inhibited), generating color.

7

Add 30%...

Reaction is halted by acidification; color development is stabilized.

8

Measure and...

Absorbance values (OD) for control and sample wells are obtained.

9

Calculate percentage...

Percentage inhibition result for each sample.