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Overview mRNA synthesis learning center
5′-capping information
Home › Learning centers › mRNA and cDNA synthesis › mRNA synthesis › mRNA synthesis FAQs

mRNA and cDNA synthesis

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Overview mRNA synthesis learning center
5′-capping information

Takara IVTpro mRNA synthesis FAQs

Here is comprehensive information on a range of mRNA synthesis topics, from DNA template preparation to choosing the right mRNA synthesis kit for your successful in vitro transcription experiments.

If you're ready to get started, choose your Takara IVTpro kit now.

DNA template preparation

Is Cloning Kit for mRNA Template (included in Takara IVTpro mRNA Synthesis System) sold separately?

Yes, the Cloning Kit for mRNA Template is also available as a standalone kit.

What is required for generating a DNA template using the Cloning Kit for mRNA Template?

The only material you need to generate a DNA template for in vitro transcription is a target coding sequence (also called gene of interest or GOI). Note that the linearized template vector in Cloning Kit for mRNA Template carries the following sequences in this order:

  • T7 promoter sequence
  • Transcription start sequence (AGG) for CleanCap AG or other compatible cap analogs
  • 5′ UTR, including a Kozak sequence
  • 3′ UTR, Poly(A) sequence
  • Multiple restriction enzyme sites (e.g., HindIII or BspQ I)

An entire sequence data (.gb) of the linearized template vector is available under ‘Vector Documents’ on the Takara IVTpro mRNA synthesis system’s product page. We recommend including a stop codon in a target sequence to avoid stop codon readthrough.

How should I linearize my vector after generating the construct with a target coding sequence?

To linearize the vector with Cloning Kit for mRNA Template, we recommend using an appropriate restriction enzyme, either HindIII or BspQ I, which has a digestion site located right after the Poly(A) sequence. Note that if your GOI and/or junction sites between the GOI and vector sequence contain the restriction site(s), the site(s) need to be removed by altering the codon(s) without changing the amino acid sequence. Other restriction sites are also available but not recommended because extra sequences after poly(A) tail are known to affect mRNA translation.

Are there optimal DNA terminal structures for enabling efficient IVT reaction?

After restriction enzyme digestion, it is better for the linearized DNA to have 5′ overhangs or blunt ends. It is best to avoid 3' protruding ends, as these may produce undesirable RNA sequences.

What types of cap analogs can be used with the linearized template vector in Cloning Kit for mRNA Template?

CleanCap® Reagent AG (TriLink BioTechnologies, No. N-7113 or N-7413) is recommended because the linearized template vector in Cloning Kit for mRNA Template has a transcription start site AGG as a default sequence. ARCA and conventional m7G cap analogs can be also used. However, efficient IVT reaction with these cap analogs requires the transcription start site (+1 position) to start with a G nucleotide. Therefore, you must modify the transcription start sequence from AGG to GGG. Please refer to this technical note or the User Manual for detail.

What is the optimal size of a target coding sequence (GOI) for the IVT reaction?

We have confirmed that a GOI as large as ~12 kb could be successfully constructed using the linearized template vector in Cloning Kit for mRNA Template. Please note that the yield and quality of transcripts may be compromised for fragments larger than 4 kb. We confirmed that FLuc mRNA (approximately 1.9 kb) was generated with high quality and high yield using our kits.

In vitro transcription for RNA synthesis

What is the difference between the Takara IVTpro mRNA Synthesis System and the Takara IVTpro T7 mRNA Synthesis Kit?

Takara IVTpro mRNA Synthesis System includes a cloning kit for preparing the DNA template, which is also sold separately: Cloning Kit for mRNA Template. If you already have a DNA template for in vitro transcription, we recommend using the standalone kit, Takara IVTpro T7 mRNA Synthesis Kit.

What types of templates can be used for IVT reactions using the Takara IVTpro T7 mRNA Synthesis Kit?

You can use a linearized DNA vector included in Cloning Kit for mRNA Template or double-stranded DNA template that contains a T7 promoter sequence (i.e., a PCR amplicon or fully synthesized DNA fragment).

Does mRNA need to have both 5’ cap and 3’ poly(A) structures for translation experiments?

Yes. Both the 5’ and 3’ structures are critical for efficient target translation and mRNA stability in cells. Missing either of the structures will result in unsatisfactory translation and protein expression. For DNA template preparation, we recommend using Cloning Kit for mRNA Template, contained in the Takara IVTpro mRNA Synthesis System. This cloning kit is also sold separately. The T7 vector in this cloning kit contains a transcription start site that is compatible with CleanCap® AG, UTRs, and poly(A) sequence.

How much RNA can be synthesized per reaction using the Takara IVTpro mRNA Synthesis System or the Takara IVTpro T7 mRNA Synthesis Kit?

RNA yield of FLuc mRNA (approx. 1.9 kb size) is about 200 μg/reaction. If desired, the IVT reaction volume can be scaled up 10-fold (up to 200 μl reaction volume) without compromising the yield.

Which enzymes are included in the 10X Enzyme Mix?

10X Enzyme Mix contains T7 RNA Polymerase ver. 2 (Cat. #2541A) plus a proprietary mixture of supplemental enzymes. Therefore, the T7 promoter sequence in DNA templates is essential for in vitro transcription reaction.

What additional products are needed with the kits?

If resulting mRNA require cap structures, we recommend either separately purchasing your own cap analogs, such as CleanCap Reagent AG (TriLink BioTechnologies, No. N-7113 or N-7413), or using enzymatic post-transcriptional capping systems, including Vaccinia Capping Enzyme (Cat. #2460) or Faustovirus Capping Enzyme (Cat. #2480) along with mRNA Cap 2′-O-Methyltransferase (Cat. #2470). Please note that neither Takara IVTpro mRNA Synthesis System nor Takara IVTpro T7 mRNA Synthesis Kit contains capping systems.

Can I use modified NTPs along with the Takara IVTpro kits?

Yes. Modified NTPs, such as pseudo-UTP, etc., can be used instead of UTP to reduce the innate immune response. When using modified NTPs, replace the corresponding NTP with an equivalent amount. Please refer to the User Manual for details.

What do you recommend for cleaning up the RNA created with these kits?

Both the Takara IVTpro mRNA Synthesis System and the Takara IVTpro T7 mRNA Synthesis Kit contain LiCl for RNA purification. If your RNA size is less than 300 bp or if the RNA concentration is less than 0.1 μg/μl, we recommend purifying the RNA by spin column (NucleoSpin RNA Clean-up, Cat. #740948.10/.50/.250) or by traditional ethanol precipitation after phenol-chloroform extraction.

How can the 5’ cap structure be added?

The 5’ cap structure can be added co-transcriptionally using cap analogs (such as CleanCap, ARCA, or mCap) or post-transcriptionally using Vaccinia Capping Enzyme (Cat. #2460) or Faustovirus Capping Enzyme (Cat. #2480). Please refer to detailed information about 5′ capping of mRNA in our mRNA synthesis learning center.

A protocol for the co-transcriptional capping method can be found in the User Manual for the Takara IVTpro mRNA Synthesis System or the Takara IVTpro T7 mRNA Synthesis Kit. These are located in the Documents tab of the product page.

For a protocol of the post-transcriptional capping method, please refer to the User Manual for Vaccinia Capping Enzyme (Cat. #2460) or Faustovirus Capping Enzyme (Cat. #2480). Additionally, the cap-1 structure can be created using mRNA Cap 2′-O-Methyltransferase (Cat. #2470).

Post-transcriptional capping

Does Vaccinia Capping Enzyme (VCE) have thermostable capability?

No, our Vaccinia Capping Enzyme (Cat. #2460) does not have thermostable capability. Faustovirus Capping Enzyme (FCE, Cat. #2480) exhibits high enzyme activity over a broader temperature range, making it suitable for various 5′ sequences. 

What types of RNA can be used for capping reactions?

Capping Enzymes—Vaccinia Capping Enzyme (Cat. #2460) or Faustovirus Capping Enzyme (Cat. #2480)—can modify and convert an uncapped RNA (both 5′-triphosphate and 5′-diphosphate RNA) into m7G-capped RNA (cap-0 RNA structure).

How efficient is the 5'-capping procedure?

The capping efficiency by Capping Enzymes is expected to be close to 100% (data not shown). Although the procedure can be time-consuming, high capping efficiency is a major advantage over traditional co-transcriptional methods, including ARCA.

What types of RNA can be used for 2’-O-methylation on the first nucleotide?

The m7G-capped structure (cap 0) is required for 2′-O-methylation on the first nucleotide. In addition, 3'-O-methylated m7G-cap, such as ARCA, can also be used as a substrate for mRNA Cap 2′-O-Methyltransferase (Cat. #2470).

How should I prepare the cap-1 RNA from uncapped RNA?

Two options, either the 1-step or 2-step methods, are available for preparing cap-1 RNA from uncapped RNA. In the 1-step, direct modification method, Vaccinia Capping Enzyme (Cat. #2460) or Faustovirus Capping Enzyme (Cat. #2480) will generate a cap-0 structure while mRNA Cap 2′-O-Methyltransferase (Cat. #2470) simultaneously generates a cap-1 structure within the same tube. In the 2-step, indirect modification method, these two enzymatic reactions will occur sequentially as a separate step. The 2-step method needs at least one RNA purification step between the reactions. For more details, please see this technical note on post-transcriptional capping. 

Is it possible to convert to cap-2 RNA using mRNA Cap 2ʹ-O-Methyltransferase?

No. The mRNA Cap 2′-O-Methyltransferase (Cat. #2470) can convert a cap-0 into cap-1 RNA structure, but it is not possible to further convert to cap-2 RNA structure.

Are there any precautions I should take regarding the post-transcriptional capping reactions?

If the full RNA length is less than 200 bp, we recommend extending the incubation time with capping enzyme from 30 min to 1 hr for cap-0 RNA preparation. For cap-1 RNA preparation using both a capping enzyme and mRNA Cap 2′-O-Methyltransferase (Cat. #2470), extending the incubation time from 1 hr to 2 hr will enhance the capping and conversion efficiency.

General information regarding RNA synthesis

Is there a selection guide for Takara Bio’s in vitro transcription offerings?

Yes. Please refer to our selection guide to choose the right product(s) for your needs.


Takara IVTpro mRNA Synthesis System

The IVTpro system includes two kits, one for DNA template preparation and the other for the high-yield in vitro transcription reaction. Both kits are also sold separately. THe IVTpro system uses a highly efficient T7 RNA polymerase to generate up to 200 µg of mRNA with a cap structure and poly(A) sequence. A wide variety of capping systems can be used, including CleanCap or ARCA and/or modified nucleosides such as pseudouridine.

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