Does anyone know if there is an upper size limitation to the DNA that will precipitate and be bound by Ampure XP beads? I'm specifically thinking of cleaning up Phi29 WGA reactions and long cDNAs.
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"The size of fragments eluted from the beads (or that bind in the first place) is determined by the concentration of PEG, and this in turn is determined by the mix of DNA and beads. A 50ul DNA sample plus 50ul of beads will give a SPRI
NA ratio of 1, as will 5ul pipetting (but much harder to get right). As this ratio is changed the length of fragments binding and/or left in solution also changes, the lower the ratio of SPRI
NA the higher larger the final fragments will be at elution"
Maybe this link can be of help
Someone recently asked me, “how do SPRI beads work” and I realized I was not completely sure so I went to find out. My lab uses kits. Lots...
BW
Roberta
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Thanks for the reply, but that's not exactly what I'm asking. Since the beads are typically used for PCR cleanup and size-selection of small fragments, I wondered if larger molecules of DNA, like 15-100kb, are efficiently bound to the beads and are efficiently eluted.
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I'll echo ECO and melop in saying that I've tried SPRI beads (Ampure and Seramag speedbeads) to clean up WGA products as well as genomic DNA from home-brew library prep and genomic DNA extraction protocols. As ECO mentioned, they do tend to clump and stick together with higher molecular weight fragments. It might help slightly if you avoid drying the bead pellet till it cracks. Longer elution times (I often incubate overnight at 4 Celsius for genomics extracts) and a small amount of Tween-20 seems to help elute more of the bound DNA.
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Yes - I agree. Didn't add tween 20 so recovery is probably lower than optimal, but it's more than enough for what I need so can't complain. Attached is a gel picture of genomic DNA extracted directly after SDS + proteinase K digestion without phenol-chloroform wash from a small piece of fish finclip (1mm x 4 mm). RNA is co-purified because I didn't treat with RNase. Qubit shows a yield of 1.5-2.5 ug per extract.Originally posted by ATϟGC View PostI'll echo ECO and melop in saying that I've tried SPRI beads (Ampure and Seramag speedbeads) to clean up WGA products as well as genomic DNA from home-brew library prep and genomic DNA extraction protocols. As ECO mentioned, they do tend to clump and stick together with higher molecular weight fragments. It might help slightly if you avoid drying the bead pellet till it cracks. Longer elution times (I often incubate overnight at 4 Celsius for genomics extracts) and a small amount of Tween-20 seems to help elute more of the bound DNA.Attached Files
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genomic with spri beads
I know this thread is old but I'm hoping Melop could tell me the ratio of sample to beads used for genomic DNA purification. I looked around online and since the protocols aren't designed for DNA this size I haven't found any suggestions.
Thanks.
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You can do as low as 0.6X beads. I usually use 1X. It usually doesn't matter too much for genomic extracts. I also keep the beads in, they don't affect with PCR or library prep.Originally posted by urchin View PostI know this thread is old but I'm hoping Melop could tell me the ratio of sample to beads used for genomic DNA purification. I looked around online and since the protocols aren't designed for DNA this size I haven't found any suggestions.
Thanks.
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I elute in 30ul of Tris pH=8.0. I pipette it until the beads get re-suspended, and directly used that mixture for down-stream workflows without removing the beads.Originally posted by pmiguel View PostHi melop,
What are your elution conditions?
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Phillip
If you want to remove the beads, incubate at 37C overnight.
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by GATTACATLove this - good data definitely starts from good input, and poor input can only give relatively poor data. I particularly like the mention of Nanodrop/absorbance based methods for quantification. It's such a toss up if you'll get an accurate reading or what amounts to a randomly generated number, and a lot of library/sequencing related issues can be traced back to poor quant.
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by SEQadmin2
I’m not a sequencing expert. I’m a purification scientist who uses NGS to evaluate workflows my group develops. With this perspective, we think about the sample first and the NGS workflow second. The sequencer is an exceptionally honest reporter, but it can only report on what you give it, so whether you get clean, interpretable data from an NGS workflow is largely determined before you begin.
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