Hi guys, I am currently working on qRT-PCR. However, the amount cDNA I got from RT reaction is too little to assess all the targets.
I saw some papers and websites mentioning amplifying cDNA with PCR, I wonder if it is a good thing to do, or if it is better to redo all from the very beginning (extract RNA from tissue).
Many Thanks!
If you don't have enough cDNA, then you have to start with more RNA. There is no way to ensure that you can increase all of the cDNA molecule types and keep the proportions the same.
Typically, unless your target genes are all really low copy number, you can dilute out your cDNA before using it for qPCR.
Good luck!
Have you looked at preamplification method/assays i.e.
Article Pre-amplification as a method for improvement of quantitativ...
https://www.qiagen.com/us/product-categories/discovery-and-translational-research/pcr-qpcr-dpcr/preamplification
https://www.bio-rad.com/en-tr/product/preamplification-supermix?ID=NVENAUMNI
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