I was hoping to get some input regarding the process I use to extract P. falciparum mRNA from dried blood spots for use in qPCR.

I am trying to amplify Pfs25 mRNA, and I've been running into two major problems:

1. Issues with RNA purity

-overall concentrations are low, about 20-80 ng/uL according to NanoDrop

-260/280 values average around 1.5

-260/230 values average around 0.5

2. gDNA contamination of RNA samples

-no reverse transcriptase control in qPCR consistently shows amplification with Ct values close to the experimental wells

I use Qiagen buffer AL, buffer ATL, and proteinase K (DNA mini kit) to create the lysate from the dried blood spot, and then I use the Qiagen RNeasy mini kit to extract from that prepared lysate. I synthesize cDNA using the Qiagen Quantitect Reverse Transcription kit, and I do include the wipeout buffer step.

Has anyone else run into these problems while extracting RNA from dried blood spots? I've tried quite a bit of generic qPCR troubleshooting, and none of it has seemed to make any significant difference.

Thank you in advance for any advice you might be able to give me!

More Danielle Snider's questions See All
Similar questions and discussions