The kit provides all the necessary components for cDNA synthesis from total RNA or mRNA. It is provided at 5× concentration and used at 1× concentration by adding gDNA remover, RNA and H2O. Simultaneous genomic DNA removal and cDNA synthesis are performed. After cDNA synthesis, gDNA remover and reverse transcriptase are inactivated by heating at 85℃ for 5 seconds. The resulting cDNA is suitable for qPCR, not for regular PCR.
• Simultaneous genomic DNA removal and cDNA synthesis.
• The optimal ratio of Oligo(dT)20 Primer to random primer(N9) for qPCR ready cDNA.
• qPCR ready cDNA in 15 minutes.
• cDNA up to 250 bp.
Applications
• Multiple copy and low copy gene detection
• GC-rich or complex secondary structure RNA template
Storage
at -20 ℃ for two years
Shipping
Dry ice (-70 ℃)
Product Contents
Component |
AH341-01 (50 rxns ) |
5×TransScript® II All-in-One SuperMix for qPCR |
200 μl |
5×TransScript® II All-in-One No-RT Control SuperMix for qPCR |
20 μl |
gDNA Remover |
50 μl |
RNase-free Water |
1 ml |
Citations
Cui X . Exploring the formation and recognition of an important G-quadruplex in a HIF1α promoter and its transcriptional inhibition by a benzo[c]phenanthridine derivative.[J]. Journal of the American Chemical Society, 2014, 136(6):2583.
Gu Q , Chen Z , Yu X , et al. Melatonin confers plant tolerance against cadmium stress via the decrease of cadmium accumulation and reestablishment of microRNA-mediated redox homeostasis[J]. Plant Science, 2017, 261:28-37.
Huang X , Huang B , Chen J , et al. Cellular responses of the dinoflagellate\r, Prorocentrum donghaiense\r, Lu to phosphate limitation and chronological ageing[J]. Journal of Plankton Research, 2016, 38(1):83-93.
Guo J , Zu G , Zhou T , et al. Clinicopathological significance of orphan nuclear receptor Nurr1 expression in gastric cancer[J]. Clinical and Translational Oncology, 2015, 17(10):788-794.