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Dino-DNA extraction buffer stock solution:
20L nuclease free !! water
60L Ethanol
pH to 5.5 with HCl
*some* EDTA
other additives that block DNAses.
You wouldn't do this in one step, or did I get it wrong?
First, extract the limestone over a few weeks. The ethanol keeps the DNA solid/precipitated to the left over matrix (will there be a solid matrix left over?) or the DNA will sink to the ground
Then discard the supernatant, add water to dissolve th DNA.
But in the rock the DNA is captured in a dry state, protected from UV radiation.
So isn't it believable that the DNA survived to some degree?
It's protected from UV, but not gamma, which permeates rock plenty over 65my, and causes DSBs. Big problem. I think the focus on DNA is not only unwarranted, but will cause some frustration as to feasibility. Like I said, you need long DNA stretches to get some actual info. But you can infer some structure and function with short polypeptides. We should try to work out how they worked at the cellular level before we can grow whole beasties. They skip that step in JP, I know. Movie science!
But I'm liking this protocol talk for demineralization. What I've read, they simply add 1 M EDTA in tris, pH 8, let it sit, spin down and repeat til there are no visible changes. But that was just for peptides. Is there a reason that wouldn't work for DNA? I'm no biochemist.
~A.J.
<typed with thumbs>
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On Jul 18, 2013 12:01 AM, "Andreas Sturm" <masters...@gmail.com> wrote:
>
> >He described the methods they attempted to recover DNA from
> bone, chiefly involving dissolution of the bone matrix..using HCl. A
> fantastic way to rapidly degrade your paleo-DNA.
>
> Ok, but how would it be possible to dissolve it? unsing just deionized water+ethanol which takes up the limestone? The ethanol for not dissolving DNA
>
>
>
> >DNA just isn't that stable on geologic time scales. It's half life, even in the best of frozen permafrosty circumstances, is around 500 years.
>
> Wasn't the same thought for peptides? :D
>
>
>
>
> >It's so hard to do that I think it a poor use of resources.
>
> Yes, but you'll learn a lot of things that aply for other uses...
>
> > It's going to be the artist's/engineer's conception of what a "dinosaur" looks like, and thus will look cool and dinosaury but be inauthentic.
>
> Did they have feathers? Very likely yes, but we'll know it for sure if we clone one :D
>
>
> Is there a DNA Polymerase that doesn't need a primer? Or can one be engineereed?
Nature already did that. It's called tdt or terminal deeoxynucleotide transferase, or simply terminal transferase.
Sorry I meant it doesn't need a template! For something without a known primer, you simply ligate on a know sequence and use a primer for that
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