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Protease inhibitor and phosphorylase inhibitor

Manufactured by Boster Bio

Protease inhibitor and phosphorylase inhibitor are laboratory reagents used in biochemical and molecular biology research. The protease inhibitor is designed to inhibit the activity of proteolytic enzymes, while the phosphorylase inhibitor is used to inhibit the activity of phosphorylases. These reagents are commonly used in experimental procedures to control enzymatic processes and maintain the integrity of target molecules or samples.

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2 protocols using protease inhibitor and phosphorylase inhibitor

1

Western Blot Protein Analysis

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Total cellular protein was extracted with RIPA lysate buffer (Boster Biological Technology) containing protease inhibitor and phosphorylase inhibitor (Boster Biological Technology), and determined protein concentration with BCA protein detection kit (Boster Biological Technology), then separated by SDS-PAGE electrophoresis kit (cwbiotech). The amount of each group proteins was 20μg. After separation, the proteins were transferred to PVDF membrane (0.22um). When sealed by 0.5% non-fat milk powder still 1 h, the PVDF membrane was incubated with polyclonal primary antibody and secondary antibody combined with HRP. The membrane was colored by ECL enhanced chemiluminescence kit (Boster Biological Technology) and formed by Biological Spectrum Image System Scanning.
Primary antibodies used in this study include anti-β-actin(1:5000, AP0060, Bioworld Technology, Inc), anti-bcl-2(1:1000, AF6139, Affinity), anti-Bax(1:1000, AF0120, Affinity), anti-p-VEGFR-2(1:500, AF3279, Affinity), anti-MMP-2(1:500, AF5330, Affinity). The secondary antibodies include HRP-conjugated affinipure goat anti-Rabbit IgG(1:5000, Boster Biological Technology, BA1054).
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2

Western Blot Protein Analysis

Check if the same lab product or an alternative is used in the 5 most similar protocols
Total cellular protein was extracted with RIPA lysate buffer(Boster Biological Technology) containing protease inhibitor and phosphorylase inhibitor(Boster Biological Technology), and determined protein concentration with BCA protein detection kit(Boster Biological Technology), then separated by SDS-PAGE electrophoresis kit(cwbiotech). The amount of each group proteins was 20ug. After separation, the proteins were transferred to PVDF membrane (0.22um). When sealed by 0.5% non-fat milk powder still 1 h, the PVDF membrane was incubated with polyclonal primary antibody and secondary antibody combined with HRP. The membrane was colored by ECL enhanced chemiluminescence kit(Boster Biological Technology) and formed by Biological Spectrum Image System Scanning.
Primary antibodies used in this study include anti-β-actin(1:5000, AP0060, Bioworld Technology, Inc), antibcl-2(1:1000, AF6139, A nity), anti-Bax(1:1000, AF0120, A nity), anti-p-VEGFR-2(1:500, AF3279, A nity), anti-MMP-2(1:500, AF5330, A nity). The secondary antibodies include HRP-conjugated a nipure goat anti-Rabbit IgG(1:5000, Boster Biological Technology, BA1054).
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