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Does anyone know what ratio of Ampure XP beads:sample I must use to remove material from my library that is 150bp and below? My library is in 30ul of 1x TE.
Also has anyone ever concentrated their final library in a DNA Speedvac/concentrator unit and sequenced it with reason being the library did not produce enough yield but the speedvac step allowed it to. I'm curious if the sequencing of this concentrated library worked out well?
Also has anyone ever concentrated their final library in a DNA Speedvac/concentrator unit and sequenced it with reason being the library did not produce enough yield but the speedvac step allowed it to. I'm curious if the sequencing of this concentrated library worked out well?
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