We have synthesized random DNA library (containing N40 random region) for aptamer selection using solid phase DNA synthesis. But after deprotection and gel purification followed by desalting, we are getting only 10% compared to total amount before purification (Loss is approx. 90%). Can anyone suggest how to tackle this problem, what could be the possible solution for this?
Nguyễn An Thuận
Hi Leena,
Which chemistry did you use for synthesis? and how do you do deprotection?
Thuan
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Leena Laxmikant Badgujar
Nguyễn An Thuận we use phosphoramidite chemistry for DNA synthesis and deprotect the synthesized DNA using AMA solution or ammonia depending on the CPG used.
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