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mRNA Co-transcription Capping

mRNA Co-transcription Capping

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mRNA Co-transcriptional Capping

Compared with the two-step enzymatic capping, the one-step co-transcriptional capping method can significantly reduce the process flow. The method is result-oriented and involves the addition of cap analogs to the in vitro transcription (IVT) reaction. Cap analogs can be introduced at the start of transcription, and mRNA with cap structure can be obtained upon completion of transcription. Current third-generation cap analogs can avoid reverse capping and directly add Cap 1 structure to the transcription product.

For considerations of mRNA in vivo immunogenicity and translation efficiency, the IVT process often adopts certain kinds of modified NTPs, and common modified nucleotides are pseudouridine (Ψ), N1-methyl-pseudouri-dine (N1Ψ), and 5-methylcytosine (5mC).

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Figure: Diagram of mRNA Co-transcriptional and Capping Reaction

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Co-transcriptional capping

In vitro transcriptional response (Clean Cap analog)1-2
Nucleotide modifications (Ψ/N1Ψ/5mC)
DNA template removal (DNase I)

IVT condition optimization - optional

Reaction component design and optimization3-7
Our Features
  • Diversified Nucleotide Modification Strategies

Multiple optional nucleotide modification strategies can improve protein expression.

  • Optimized Reaction System

Achieve a high transcription ratio and high capping efficiency.

  • Stable Capping Process

Achieve a capping rate of more than 95%.

  • Stringent Control of RNase

Prevent mRNA degradation effectively by stringently controlling of RNase in the experimental environment and consumables.

Case study

Yaohai Bio-Pharma has built a mature co-transcriptional capping process platform, using clean cap analogs to directly add Cap1 structure while avoiding reverse capping. After standardized sample pre-treatment and capillary electrophoresis (CE) detection, the capping rate of enhanced green fluorescent protein (eGFP) mRNA can reach more than 95%.

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eGFP mRNA capping efficiency of  more than 95%

The eGFP mRNA and mCherry mRNA prepared by co-transcriptional capping are transfected into 293T cells, respectively, and a strong fluorescent signal is observed after 48h, suggesting that the mRNA is efficiently expressed in 293T cells.

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Expression of eGFP mRNA and mCherry mRNA in 293T Cell

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