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broken emulsions from emPCR affected by DNA concentration?
Hi Everyone,
I've been having problems with my emPCR emulsions (for GS Junior)- at times 1/3-1/2 broken emulsions out of 64 wells. For the past several tries, I've wondered if it was the way I've been dispensing the oil emulsions, so I've tried dispensing with automatic pipet, combitip, and manual pipet - and I still got broken emulsions. Finally, I decreased my copies per bead from 1.5 to 0.5 and got only 6 broken emulsions out of 68 wells, but after the oil-breaking step, I still got DNA enriched beads slightly about the top edge of the bead count window. I then re-measured my pooled amplicon DNA library and found that I could have been under-estimating my DNA concentration previously (so I was actually loading a higher concentration of DNA). I then re-calculated the DNA concentration and this time loaded 0.5 copies per bead and ran the emPCR again. This time most of the wells have broken emulsions! So I was wondering if anyone has noticed that either under- or over-estimating DNA concentration would lead to broken oil emulsions? And that I should've still started at 1.5 cpb instead of 0.5 cpb? I also noticed with these past tries, I would get an air bubble at the top of the oil as I was dispensing the oil emulsions into each well (I let the oil drop from the side of the well, not straight into the well). Has anyone seen that lately? I've never seen it before.
Thanks for your help!
I've been having problems with my emPCR emulsions (for GS Junior)- at times 1/3-1/2 broken emulsions out of 64 wells. For the past several tries, I've wondered if it was the way I've been dispensing the oil emulsions, so I've tried dispensing with automatic pipet, combitip, and manual pipet - and I still got broken emulsions. Finally, I decreased my copies per bead from 1.5 to 0.5 and got only 6 broken emulsions out of 68 wells, but after the oil-breaking step, I still got DNA enriched beads slightly about the top edge of the bead count window. I then re-measured my pooled amplicon DNA library and found that I could have been under-estimating my DNA concentration previously (so I was actually loading a higher concentration of DNA). I then re-calculated the DNA concentration and this time loaded 0.5 copies per bead and ran the emPCR again. This time most of the wells have broken emulsions! So I was wondering if anyone has noticed that either under- or over-estimating DNA concentration would lead to broken oil emulsions? And that I should've still started at 1.5 cpb instead of 0.5 cpb? I also noticed with these past tries, I would get an air bubble at the top of the oil as I was dispensing the oil emulsions into each well (I let the oil drop from the side of the well, not straight into the well). Has anyone seen that lately? I've never seen it before.
Thanks for your help!
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