21_NG_ProductOverview_HeaderIcons_SynBio-GeneFragments

Gene Synthesis NEW

Introducing our newly enhanced Gene Synthesis

This easy-to-use solution is for researchers who want to skip in-house cloning steps and move quickly into functional studies with 100% sequence-verified clonal DNA .

Ordering

Complete synthetic genes with 100% sequence verification are delivered in a cloning or expression vector and are ready to use for a variety of applications.

  • No reoccurring or hidden fees for custom vectors
  • Easy online ordering and transparent pricing
  • Guaranteed delivery dates

Genes in tubes

  • No order minimum for tubes
  • Delivered dry, normalized to 4 µg with scale up options available*
  • Glycerol stocks available 

Genes in plates

  • Available in PCR and Echo™ plates
  • 3 µg delivered dry or wet normalized to 20 ng/µl*
  • Orders require a minimum of 24 genes per plate§

* Gene sequences with added complexity can interfere with assembly and/or sequencing performance. Such sequences may result in less synthesis yield and/or additional services charges.

† The time required to manufacture a gene is dependent on length, complexity, and vector choice. >85% orders are ready to ship within the number of business days indicated. Sequences that are unstable and/or toxic to E. coli can substantially affect delivery times.

‡ Echo is a trademark of Labcyte Inc. A Beckman Coulter company

§ Plates with less than 24 fragments will incur an additional fee applied at checkout

 Need your Genes faster? Check out our new Rapid Genes!

Table 1. Additional Options for Genes.

FeatureAdditional TATFormatYield
Gene Glycerol StockN/ATubeN/A
Transfection Grade Midscale Prep (<10EU/µg)3 business daysTube or 96-Well Deepwell Plate**100 µg*
Endotoxin Free Midscale Prep(<0.1EU/µg) (includes endotoxin test and report)4 business daysTube or 96-Well Deepwell Plate100 µg*

*Vectors identified as low copy vectors will have a reduced yield of 50 ug. This will be determined during the custom vector onboarding process. 

IDT vectors

IDT has several catalog vectors available for use in your experiments, but if you don’t see one here that fits your needs see Custom Vector Onboarding below. We have several options for cloning vectors and vectors ready for protein expression experiments, in both bacteria and mammalian cells. When selecting our standard cloning vector option, if your insert is less than 250 bases we will use the pIDTSmart vector. All other lengths will be cloned into our pUCIDT with the antibiotic selection marker of your choice. We also offer vectors that have been optimized for use with Golden Gate Assembly; they will not have the most frequently used Type IIS restriction sites. Upon receiving your gene, you can then subclone it into the vector of your choice using a variety of methods. The identity of the cloning vector used, its sequence, and insertion site will be confirmed in the documentation that accompanies your product.

Table 2. Best-fit vectors for Genes ≤5000 bp.

Vector nameSelection markerApplicationSequence
pUCIDT (Amp)AmpicillinCloningTXT, GB, PDF
pUCIDT (Amp) Golden GateAmpicillinCloningTXT, GB, PDF
pUCIDT (Kan)KanamycinCloningTXT, GB, PDF
pUCIDT (Kan) Golden GateKanamycinCloningTXT, GB, PDF
pIDTSmart (Amp)AmpicillinCloningTXT, GB, PDF
pIDTSmart (Kan)KanamycinCloningTXT, GB, PDF
pEXP-IDTAmpicillinMammalian ExpressionTXT, GB, PDF
pET-IDTKanamycinBacterial ExpressionTXT, GB, PDF
pET-IDT C HisKanamycinBacterial ExpressionTXT, GB, PDF
pET-IDT Dual His + ThrombinKanamycinBacterial ExpressionTXT, GB, PDF
pET-IDT N His + ThrombinKanamycinBacterial ExpressionTXT, GB, PDF

For genes >5000 bp, please contact us.

Custom Vector Onboarding NEW

If your experiment requires a vector that isn’t available in our standard genes tool, no problem. You can easily onboard your own custom vector through our website without requesting a quote.

 

Advantages to onboarding your vector with IDT:

  • Saves you time and we do the cloning for you. Once onboarded you can order cloned genes in your vector anytime
  • Onboarding has a one-time cost, no recurring fees for additional inserts
  • Fast turnaround times
  • Confidentiality is a high priority to ensure your IP is protected

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Custom Vector Onboarding
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Request a consultation

Have questions for our experts? Want to onboard your own vector? Your time is valuable and we’ll prioritize your inquiry. Click on “Request a consultation” to provide brief information about your project, and we’ll be in touch to discuss it ASAP.

Request a consultation

$500 off

when you onboard your own vector 

Applies to first gene synthesis order after onboarding. Promo credit will be issued upon completion of IDT vector onboarding.

Expires: December 31, 2024

Product details

Genes and MiniGenes™ are NGS-verified, circular double-stranded DNA in a plasmid. DNA sequences 25 bp to 5 kb are provided with IDT’s in-house vectors, expression vectors, or a custom vector of your choice without additional cloning fees (see Table 1) . Sequences greater than 5 kb can be reviewed for acceptance as a custom project. Plasmids are delivered ready-to use in your preferred configuration with an accompanying QC report.

Storage conditions

Short term (<2 weeks)4°C
Long term (up to 2 years)–20°C

Product data

Sequence verification

All inserts for Genes and MiniGene products are sequence-verified by NGS. Upon delivery of the plasmids, an NGS‑sequencing report, plasmid map, and FASTA file are all available to you in your online IDT account.

NGS QC example, depth of coverage-percent wild type

Sample NGS report

Frequently asked questions

We store onboarded custom vectors for two years after the most recent order in that vector, at no additional fee.

View FAQ

We are open to reviewing your vector if it does not meet the above criteria. Please contact your regional scientific applications support team with details of your vector, providing the sequence in FASTA format, if possible.

View FAQ

IDT Genes and Mini Gene™ sequences are delivered as double-stranded DNA, cloned into your provided custom vector.

View FAQ

Please provide the 50 bases of sequence flanking the insertion site you wish us to use. IDTs proprietary assembly method requires no restriction sites and can remove existing sequences from a vector.

View FAQ

Simple plasmid preps using a spin column or alkaline lysis method of purification are acceptable. Vectors greater than 8 kilobase pairs in size, those which require specialized cell lines or growth conditions for propagation, or those with exceptionally low yields may incur additional costs and/or turnaround time for gene production after validation.

View FAQ

  • An E. coli origin of replication
  • Kanamycin, Ampicillin, or Chloramphenicol resistance marker
  • 1 µg of circular plasmid

A minimum of 50 bases of sequence flanking the insertion site you would like us to use for the assembly of your gene inserts into the vector. Therefore, you do not need to specify restriction sites for assembly.

View FAQ

Synthesis time depends on the length of the custom gene.

Length of custom gene Time to ship after order confirmation (business days)
Up to 500 bp 8
501–5000 bp 12
 More than 5000 bp Inquire*

* Longer sequences may take additional time depending on their length and complexity. Contact us to submit sequences longer than 5000 bp for an official review and quote, including an estimated turnaround time.

View FAQ

We can synthesize custom genes from 25 bp to more than 5 kb in length.

If you would like to submit a sequence for review or obtain an official quote, contact us.

View FAQ

We have removed the multiple cloning site and most common restriction sites from our standard vectors.

Because of this, you should be able to add any convenient restriction sites to your sequences to facilitate subcloning. If you would like more information about our standard vectors, contact us.

View FAQ

By not having a set multiple cloning site in our vectors, customers are able to choose the optimal restriction site set required to subclone into their choice of destination vector. You should add the restriction sites to your sequences when placing your order.

View FAQ

IDT can synthesize genes in customer supplied vectors. Before we can accept orders in the custom vector, we will need to complete a validation process to confirm it is compatible with our synthesis process.

If you have questions about vector validation or would like an official quote, contact us for more details. The custom vector onboarding has a minimal fee associated, however, if the vector is accepted and successfully onboarded there are no additional fees for using a custom vector.

View FAQ

IDT ships custom gene dry unless otherwise requested. While dry they should be stable up to 2 years. After resuspending in a high-quality, molecular-grade water or buffer, pH 7.5–8.0, you should store the DNA at –20°C, and if necessary, aliquot to avoid more than 2 or 3 freeze-thaw cycles.

View FAQ

Plasmid DNA is fragmented prior to sequencing. Next, the fragmented DNA must be converted to a library that is compatible with the NGS sequencing platform, which is done using transposases to randomly add sequencing adapters to the fragments.

While this process is somewhat random, it is influenced by the structure and composition of the sequence.

Similarly, the success of individual reads within the run is also influenced by structure and sequence. Highly structured areas, areas with extremes in GC, and other complexities tend to affect read depths in areas where they occur.


View FAQ

Even with clonally pure samples, NGS traces rarely show 100% sequence identity. This is because errors do occur during sequencing reactions and the subsequent data analysis.

These error rates are typically between 0.1% and 0.01%, but they can be locally elevated in regions of extreme GC content or secondary structure. Misalignment of the traces can also occur, particularly in highly repetitive sequences.

Finally, small subpopulations of sequence variants can arise during propagation of E. coli.

View FAQ

To optimize manufacturing and delivery time, synthetic genes ≤5 kb in length will be provided in a “best-fit” IDT cloning vector (unless the Golden Gate vectors are selected). A choice of either ampicillin or kanamycin selection markers is available. Your high-quality, synthetic gene can then be subcloned into the vector of your choice using a variety of methods.

View a list of the IDT cloning vectors and sequence information. The identity of the cloning vector used, its sequence, and insertion site will be confirmed in the documentation accompanying the product.

View FAQ

To optimize manufacturing and delivery time, synthetic genes ≤5 kb in length will be provided in a "best-fit" IDT cloning vector. A choice of either ampicillin or kanamycin selection markers is available. Your high-quality, synthetic gene can then be subcloned into the vector.

For more information, and a list of the IDT cloning vectors. The identity of the cloning vector used, its sequence, and insertion site will be confirmed in the documentation accompanying the product.

View FAQ

IDT has a free, online codon optimization tool available through our SciTools™ Web Tools suite that you can use to perform codon optimization before ordering your oligonucleotide.

To optimize, simply paste in an amino acid or nucleotide sequence and select your desired expression host. If you need additional assistance, contact us.

View FAQ

We do not have a tool on our website that will analyze the restriction enzyme sites in your sequence.

However, NEB has a tool will identify the restriction sites within your sequence at https://nc2.neb.com/NEBcutter2/.

View FAQ

No, IDT Genes and Mini Gene™ sequences cannot have mixed or degenerate bases. Gene and Mini Gene sequences may only be composed of A/C/G/T bases.

Gene sequences desired with multiple bases at the same position must be ordered as a wild type gene and the corresponding number of separate mutant genes.

View FAQ

IDT Genes and Mini Gene™ sequences are delivered as double-stranded DNA, cloned into an IDT vector.

View FAQ

View all custom gene synthesis FAQs

Biosecurity

Sequence Information is secure and confidential at IDT. Please see our Confidentiality Statement for more information. All online ordering steps, including sequence entry and your choice of parameters, are also secure and protected.

We screen the sequence of every gene, gene fragment, and Megamer™ ssDNA fragment order we receive to (1) identify any regulated and other potentially dangerous pathogen sequences, and (2) verify that IDT’s gene customers are legitimate scientists engaged in beneficial research.

IDT is among the five founding members of the International Gene Synthesis Consortium (IGSC) and helped to create the IGSC’s Harmonized Screening Protocol. The Harmonized Screening Protocol describes the gene sequence and customer screening practices that IGSC member companies employ to prevent the misuse of synthetic genes. IDT takes the steps set out in the Harmonized Screening Protocol to screen the sequences of ordered genes and the prospective customers who submit those orders.

For more information about the IGSC and the Harmonized Screening Protocol, please visit the website at www.genesynthesisconsortium.org.

logo_igsc

In October 2010, the United States government issued final Screening Framework Guidance for Providers of Synthetic Double-Stranded DNA, describing how commercial providers of synthetic genes should perform gene sequence and customer screening. IDT and the other IGSC member companies supported the adoption of the Screening Framework Guidance, and IDT follows that Guidance in its application of the Harmonized Screening Protocol. For more information, please see 75 FR 62820 (Oct. 13, 2010), or https://federalregister.gov/a/2010-25728.

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