Hi Scientists,
I am looking to purify HIV neutralizing antibodies from human plasma using a protein A spin column kit (cosmo bio). The kit can only purify up to 0.4 mg of IgG. Other relevant information such as the binding and elution pH is not provided by the manufacturer.
To avoid overloading my column, I use 100 uL of plasma for IgG purification. However, the neutralizing ability of the subsequent IgG is very low relative to that of unfractionated plasma. I have checked the plasma flowthrough for any neutralization activity but there's none. I have also tried dialysis against PBS to no avail. So far I have been stuck at this stage for almost 4 weeks now.
I was wondering if the problem could be the binding capacity of the kit. Do you think a binding capacity of 0.4 mg is too low to elute a meaningful titer of my antibody of interest?
Have you experienced a similar problem with the kit (or another manufacturer's kit)? How did you go about?
Best Regards.
Hi Isaac Akuma
Check this recent study. Hope its interesting.
Article Low pH Exposure During Immunoglobulin G Purification Methods...
Human plasma contains tons of antibodies against many antigens, just imagine all those infectious diseases and vaccinations for example. Using a non-specific method like protein A you will catch all of them and a low-abundance antibody won't have a chance to bind in relevant quantities.
Maybe you find a possibility to immobilize the HIV and precipitate the neutralizing antibodies that way?
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