IHC buffers - Quenching - AP

IHC buffers - Quenching - AP


Chromogenic detection methods often use a conjugated enzyme to visualize epitope-antibody interactions. When using this method of detection, the endogenous activity of the same enzyme must be blocked. For example, protocols that include horseradish peroxidase (HRP) or alkaline phosphatase (AP) may require reagents to prevent non-specific signals. Tissues such as kidney, liver, or vascular areas with red blood cells, contain endogenous peroxidase activity. Peroxidase blocking reagents formulated with 3-10% H2O2 can be used to prevent endogenous peroxidase from cleaving the substrate. Endogenous AP found in intestine, kidney, lymphoid and other tissue can be blocked with 1 mM Levamisole. The intestinal form of AP is unaffected by Levamisole but can be blocked by using 1% acetic acid.

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Cat#
Description
Cond.
Price Bef. VAT
AOB9361-10
 10mg 
AOB9361-5
 5mg 
AOB9361-25
 25mg 
AOB9361-50
 50mg 
281321-5g
 5g 
AOB9361-100
 100mg 
015543-1g
 1g 
281321-25g
 25g 
281321-50g
 50g 
281321-100g
 100g 
281321-10g
 10g 
TRC-L331103-250MG
 250mg 
015544-1mg
 1mg 
TRC-A611775-5MG
 5mg 
TRC-A611775-50MG
 50mg 
TRC-A611775-10MG
 10mg 
TRC-H943725-2.5MG
 2.5mg 
TRC-H943725-25MG
 25mg