Hello everyone,
We have observed a discrepancy of approx. factor 2 of our measured copies/ well and the theoretical copies/ well. The measured copies are around 50 % of where they should be.
I've looked through all previous questions on ddPCR here, and this didn't come up. Hope someone can help.
Also if anyone has ideas on how to reduce the %RE for replicates, ideas are welcome.
Thanks in advance.
Hi Christine,
It all depends on how you determined the "theoretical copies/well". What reference are you using? Is it a spiked control with known concentration (how did you determine the concentration)? Or did you measure the Qubit concentration of the input sample and assumed a certain number of copies per ng of input material?
What input material are you using? Is it intact or fragmented DNA/RNA?
Without further details on your experimental setup we can only speculate about the discrepancy.
Hope this helps! :)
Good luck, Daan
Hi Christine,
Did you find any solution for your problem? I am have quite similar kind issue.
Thank you!
Regards,
Charan
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