I want to first amplify the HIV-1 env gene from a patient's plasma samples and then I want to clone it into a plasmid vector. I am using the QIAamp viral RNA mini kit for the extraction of HIV-1 RNA from the plasma. I have extracted RNA from a 560 µL plasma specimen. The problem is I have failed to generate cDNA and subsequently failed to amplify the env gene. Viral load in the serum ranges from 4000 to 550000 copies /mL. For cDNA synthesis I have used ReverTra A reverse transcriptase.
I would appreciate it if fellow researchers would share their experiences with plasma samples from HIV-1 positive patients.