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Merck
CN

CS0370

Sigma-Aldrich

Cathepsin Detection Assay

Cathepsin B Detection Assay, sufficient for 100 assays

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UNSPSC代码:
12352200
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用途

sufficient for 100 assays

储存温度

2-8°C

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应用

Hoechst stain can be used to label the cell nuclei after labeling with the MR-Cathepsin B substrate. It is visualized under a microscope using a UV-filter with excitation at 365 nm and emission at 480 nm. Acridine orange (AO) helps identify lysosomes and other intracellular organelles. In the acidic pH of the lysosome AO, molecules aggregate. Aggregated AO fluoreses orange rather than green thus clearly differentiating the lysosomes from the other organelles.

生化/生理作用

Cathepsin B kit detects protease activity within whole living cells as a marker of intracellular cathepsin B activity. In the assay (z-Arginine-Arginine)2 (z-RR)2 derivative of the cresyl violet fluorophore easily penetrates the cell membrane and the membranes of the internal cellular organelles enabling to detect cathepsin B activity within whole living cells.
Cathepsin B, K, and L protease activities can be detected within whole living cells using substrate-based fluorescent assays, which utilize cathepsin target sequence peptides, derivatives of the cresyl violet fluorophore, conjugated to Magic Red™ (MR) fluorogenic substrate (cresyl violet). Following enzymatic cleavage inside the living cells at one or both arginine (R) amide linkage sites, the mono and non-substituted cresyl violet fluorophores generate red fluorescence when excited at 550-590 nm.
Cathepsins are apoptosis markers associated with Alzheimer′s disease, numerous types of cancer, autoimmune arthritis, and the breakdown of bone structure seen with osteoporosis.

法律信息

Magic Red™ trademark is owned by MP Biomedicals (Formerly ESP).

仅试剂盒组分

产品编号
说明

  • MR-(RR)2 substrate 1 vial

  • Hoechst 33342 stain 1 mL

  • Acridine orange stain .5 mL

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Zoltán Kukor et al.
The Journal of biological chemistry, 277(24), 21389-21396 (2002-04-05)
The lysosomal cysteine protease cathepsin B is thought to play a central role in intrapancreatic trypsinogen activation and the onset of experimental pancreatitis. Recent in vitro studies have suggested that this mechanism might be of pathophysiological relevance in hereditary pancreatitis

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