Recycle Those DNA Extraction Columns
You know those ridiculously priced and throw-away DNA mini, midi and maxi-prep columns? Well the good news is that you can actually re-use them if you are reasonably careful at regenerating them, with this simple and cheap method described in detail by Nagadenahalli B. Siddappa in Biotechniques in 2007.
Apparently these columns can be reused up to 20 times… perhaps more a guesstimate than a real number, but hey, who’s complaining?
Essentially the columns are treated with 1M HCl overnight, rinsed extensively with dH2O and then re-equilibrated with buffer from the kit you use (e.g. Qiagen QBT). If you are worried about finishing the buffers in the kits, look in the back of the manual, there are often simple recipes about how to remake them.
The authors allay concerns about plasmid carryover contamination by assaying for plasmid using RT-PCR and transfection assays which all showed zero carryover between recycled uses of the columns. In fact they showed that the plasmid DNA had been chemically sheared into low molecular weight fragments and could not be used as a template.
They also stated that prolonged exposure to 1M HCl (1 month) did nothing to the binding capacity of the columns, so even if you forget about it, there is no need to stress.
Our lab has modified the protocol to include passing warm water through the treated columns when regenerating to ensure that all DNA and any other contaminants are removed. Also pre-warming the elution buffer to 42oC or thereabouts seems to increase the elution of any plasmid DNA bound to the column, although what extra compounds it releases is unknown but probably negligible.
It may be our imagination, but we have often gotten higher yields of plasmid DNA from a treated reused column, than a new one.
Go ahead, stretch those budgets further.
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Thanks for the tip, I was using it for a while, but I am a little confused here. The article on BioTechnique was not clear to me, could you please make an order what have you done to regenerate those columns. (e.g 1-wash dH2O 5times, 2-Wash with washing buffer 2 times etc…)
And how about Invitrogen columns, has anybody tried them?
Thanks in advance!
-J
Hi Liam
LIC is certainly reliable enough for generating constructs for protein expression.
It’s a bit different from TA cloning – the principle is explained in this article: https://bitesizebio.com/2008/01/08/get-your-clone-90-of-the-time-with-ligation-independent-cloning/
Nice tip,I’ve tried this with atleast mini-prep columns – and the columns get damaged! probably because they’re cheap ones! a few of my friends say that this method works great with Maxi kit columns, would try that out and post the outcome.
For the cleaning of the columns, I recommend a vacuum manifold, e.g. like the one from Promega, it makes the cleaning of these columns very quick. We convinced them to give us one in exchange for using their maxiprep kits, which we now recycle.
Nick
I was wondering, not having read the ligation independent cloning technique in detail (it is in effect TA cloning of sorts is it not ?), as to whether it can be used, or whether it is reliable enough to generate DNA constructs for protein expression, where everything needs to be in frame ?
Liam