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Comparison of the Guide-it Mutation Detection Kit with a CEL nuclease-based assay

Simple method to identify insertions or deletions in mammalian cells:
Amplify genomic regions directly from cells without the need for DNA purification, and detect mutations with the highly efficient Guide-it Resolvase enzyme

Faster and more efficient than CEL nuclease-based assays:
The Guide-it mutation detection protocol is several hours shorter, more sensitive, and less prone to non-specific cleavage

Introduction Results Conclusions

Introduction  

Recently-developed genome editing tools such as zinc finger nucleases, transcription activator-like effector nucleases (TALENs), and the clustered regularly interspaced short palindromic repeats (CRISPR)/Cas9 system allow precise manipulation of virtually any gene. All of these editing techniques can be used to introduce double strand breaks at a target DNA sequence that are repaired by the error-prone non-homologous end joining (NHEJ) DNA repair pathway, resulting in introduction of insertion or deletion mutations (INDELs). Detecting these types of induced INDELs at target loci requires a simple and robust method.

Results  

A PCR-based method to confirm the presence of mutations

Mutation detection is often based on PCR amplification of the region of interest and detection of mismatches in heteroduplexed DNA. With the Guide-it Mutation Detection Kit, the target sequence is amplified directly from cells, without genomic DNA extraction/purification (Figure 1, step 1). Then, the PCR products are melted and rehybridized, forming mismatched targets that can be cleaved by the Guide-it Resolvase (Figure 1, steps 2 and 3).


Figure 1. Overview of the Guide-it Mutation Detection Kit method to confirm the presence of mutations in genomic DNA.

Figure 1. Overview of the Guide-it Mutation Detection Kit method to confirm the presence of mutations in genomic DNA.

Comparison of the Guide-it Mutation Detection Kit with a CEL nuclease-based assay

The key component of the Guide-it Mutation Detection Kit is the Guide-it Resolvase, a mismatch-specific nuclease that recognizes heteroduplexed DNA. This enzyme is more efficient and more robust than other similar nucleases, such as Cel1.To compare the Guide-it system and an assay based on CEL nuclease for detecting CRISPR/Cas9-introduced mutations in mammalian cells, 293T cells were transfected with plasmids encoding Cas9 and an sgRNA specific for the AAVS1 locus. Transfected cells harvested 48 hours post-transfection were mixed with untransfected cells at varying ratios (Figure 2, top). A DNA fragment containing the AAVS1 locus was generated by PCR using Terra Direct Polymerase, and the products were purified and cleaved with either Guide-it Resolvase (Guide-it Mutation Detection Kit) or the Cel1 enzyme (Company T). Mutations were easily discernible when using the Guide-it kit (Figure 2, bottom). In contrast, the CEL assay showed considerable smearing, making it difficult to determine cleavage efficiency and reducing the ability to detect lower levels of mutation (Figure 2, bottom).

Figure 2. Comparison of the Guide-it Mutation Detection kit and a CEL nuclease assay for detecting CRISPR/Cas9-introduced mutations in mammalian cells. Mutations were easily discernible when using the Guide-it kit (estimation of cleavage, 1: 59%, 2: 46%, 3: 28%, 4: 15%, 5: <10%, 6: 0%). In contrast, the CEL nuclease assay showed considerable smearing, making it difficult to determine cleavage efficiency and reducing the ability to detect low levels of mutation.

Figure 2. Comparison of the Guide-it Mutation Detection kit and a CEL nuclease assay for detecting CRISPR/Cas9-introduced mutations in mammalian cells. Mutations were easily discernible when using the Guide-it kit (estimation of cleavage, 1: 59%, 2: 46%, 3: 28%, 4: 15%, 5: <10%, 6: 0%). In contrast, the CEL nuclease assay showed considerable smearing, making it difficult to determine cleavage efficiency and reducing the ability to detect low levels of mutation.

Figure 2. Comparison of the Guide-it Mutation Detection kit and a CEL nuclease assay for detecting CRISPR/Cas9-introduced mutations in mammalian cells. Mutations were easily discernible when using the Guide-it kit (estimation of cleavage, 1: 59%, 2: 46%, 3: 28%, 4: 15%, 5: <10%, 6: 0%). In contrast, the CEL nuclease assay showed considerable smearing, making it difficult to determine cleavage efficiency and reducing the ability to detect low levels of mutation.

Conclusions  

The Guide-it protocol, which amplifies genomic regions directly from cells without the need for DNA purification, reduced assay time from the 6 hours required by existing mismatch detection protocols to just 3.5 hours. In addition, this protocol provided increased mutation detection efficiency and demonstrated less sensitivity to buffers used in the PCR reaction than existing protocols.

In summary, compared to a CEL nuclease assay, the Guide-it mutation detection protocol is several hours shorter, more sensitive, and less prone to non-specific cleavage.

Learn more about the Guide-it Mutation Detection Kit »

Related Products

Cat. # Product Size Price License Quantity Details
631443 Guide-it™ Mutation Detection Kit 100 Rxns USD $552.00

The Guide-it Mutation Detection Kit contains all the reagents needed for PCR-based identification of insertions or deletions generated during cellular non-homologous end joining (NHEJ) repair. The first step is the amplification of the putative target sequence directly from cells. This kit uses Terra PCR Direct Polymerase Mix and Buffer, so there is no need to extract genomic DNA from your cell population prior to amplification of your target sequence. The amplicon is then melted and hybridized to form the mismatched targets for cleavage by the Guide-it Resolvase. Sufficient material is provided for 100 amplification and cleavage reactions.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

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The Guide-it Mutation Detection Kit is used to confirm the presence of mutations in genomic DNA

The Guide-it Mutation Detection Kit is used to confirm the presence of mutations in genomic DNA
The Guide-it Mutation Detection Kit is used to confirm the presence of mutations in genomic DNA. In the first step your target sequence is amplified directly from your target cells using the Terra PCR Direct Polymerase included in the kit, so there is no need to extract and purify genomic DNA from your cell population prior to amplification of your target sequence. The amplicon is then melted and hybridized to form the mismatched targets that can be cleaved by the Guide-it Resolvase.

Back

Comparison of the Guide-it and Surveyor assays for detecting mutations in mammalian cells

Comparison of the Guide-it and Surveyor assays for detecting mutations in mammalian cells

Comparison of the Guide-it and Surveyor assays for detecting mutations in mammalian cells. 293T cells were transfected with plasmids encoding Cas9 and a sgRNA specific for the AAVS1 locus. Transfected cells were harvested 48 hr post-transfection and mixed with untransfected cells at varying ratios. An amplicon containing the targeted AAVS1 locus was generated using Terra Direct Polymerase Mix, and the PCR products were purified and cleaved using either Guide-it Resolvase or the Cel1 enzyme (Surveyor assay). Mutations were easily discernable when using the Guide-it kit. In contrast, the Surveyor Assay showed considerable smearing, making it difficult to determine cleavage efficiency and reducing the ability to detect low levels of mutation.

Back

Successful knockout of AcGFP1 in HT1080 cells using the CRISPR/Cas9 system

Successful knockout of AcGFP1 in HT1080 cells using the CRISPR/Cas9 system

Successful knockout of AcGFP1 in HT1080 cells using the CRISPR/Cas9 system. Panel A. Schematic of the AcGFP DNA sequence and the location of sgRNAs tested and primer placement for the mutation detection assay. HT1080 cells containing a single copy of AcGFP1 were transfected with 1.5 μg of plasmid DNA for Cas9 expression and 1.5 μg of a plasmid harboring one of two sgRNAs (T1 or T2) using Xfect Transfection Reagent. The cell population was assayed 6 days post-transfection for cleavage efficiency and loss of fluorescence. Panel B. Using the Guide-it Mutation Detection Kit, cleavage products were detected for both sgRNAs, indicating that both CRISPRs successfully disrupted the AcGFP1 locus. Panel C. The AcGFP1 disruptions were functionally relevant, as a subpopulation of non-fluorescent cells could be detected by FACS.

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631443: Guide-it Mutation Detection Kit

631443: Guide-it Mutation Detection Kit

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The CRISPR/Cas9 system, a simple, RNA-programmable method to mediate genome editing in mammalian cells

The CRISPR/Cas9 system, a simple, RNA-programmable method to mediate genome editing in mammalian cells

The CRISPR/Cas9 system, a simple, RNA-programmable method to mediate genome editing in mammalian cells. The CRISPR/Cas9 system relies on a single guide RNA (sgRNA) directing the Cas9 endonuclease to induce a double strand break at a specific target sequence three base-pairs upstream of a PAM sequence in genomic DNA. This DNA cleavage can be repaired in one of two ways: 1) nonhomologous end joining, (NHEJ) resulting in gene knockout due to error-prone repair (orange), or 2) homology-directed repair (HDR), resulting in gene knockin due to the presence of a homologous repair template (purple).

631448 Guide-it™ Mutation Detection Kit 25 Rxns USD $260.00

The Guide-it Mutation Detection Kit contains all the reagents needed for PCR-based identification of insertions or deletions generated during cellular non-homologous end joining (NHEJ) repair. The first step is the amplification of the putative target sequence directly from cells. This kit uses Terra PCR Direct Polymerase Mix and Buffer, so there is no need to extract genomic DNA from your cell population prior to amplification of your target sequence. The amplicon is then melted and hybridized to form the mismatched targets for cleavage by the Guide-it Resolvase. Sufficient material is provided for 100 amplification and cleavage reactions.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

Documents Components You May Also Like Image Data

Back

The Guide-it Mutation Detection Kit is used to confirm the presence of mutations in genomic DNA

The Guide-it Mutation Detection Kit is used to confirm the presence of mutations in genomic DNA
The Guide-it Mutation Detection Kit is used to confirm the presence of mutations in genomic DNA. In the first step your target sequence is amplified directly from your target cells using the Terra PCR Direct Polymerase included in the kit, so there is no need to extract and purify genomic DNA from your cell population prior to amplification of your target sequence. The amplicon is then melted and hybridized to form the mismatched targets that can be cleaved by the Guide-it Resolvase.

Back

Comparison of the Guide-it and Surveyor assays for detecting mutations in mammalian cells

Comparison of the Guide-it and Surveyor assays for detecting mutations in mammalian cells

Comparison of the Guide-it and Surveyor assays for detecting mutations in mammalian cells. 293T cells were transfected with plasmids encoding Cas9 and a sgRNA specific for the AAVS1 locus. Transfected cells were harvested 48 hr post-transfection and mixed with untransfected cells at varying ratios. An amplicon containing the targeted AAVS1 locus was generated using Terra Direct Polymerase Mix, and the PCR products were purified and cleaved using either Guide-it Resolvase or the Cel1 enzyme (Surveyor assay). Mutations were easily discernable when using the Guide-it kit. In contrast, the Surveyor Assay showed considerable smearing, making it difficult to determine cleavage efficiency and reducing the ability to detect low levels of mutation.

Back

Successful knockout of AcGFP1 in HT1080 cells using the CRISPR/Cas9 system

Successful knockout of AcGFP1 in HT1080 cells using the CRISPR/Cas9 system

Successful knockout of AcGFP1 in HT1080 cells using the CRISPR/Cas9 system. Panel A. Schematic of the AcGFP DNA sequence and the location of sgRNAs tested and primer placement for the mutation detection assay. HT1080 cells containing a single copy of AcGFP1 were transfected with 1.5 μg of plasmid DNA for Cas9 expression and 1.5 μg of a plasmid harboring one of two sgRNAs (T1 or T2) using Xfect Transfection Reagent. The cell population was assayed 6 days post-transfection for cleavage efficiency and loss of fluorescence. Panel B. Using the Guide-it Mutation Detection Kit, cleavage products were detected for both sgRNAs, indicating that both CRISPRs successfully disrupted the AcGFP1 locus. Panel C. The AcGFP1 disruptions were functionally relevant, as a subpopulation of non-fluorescent cells could be detected by FACS.

Back

631448: Guide-it Mutation Detection Kit

631448: Guide-it Mutation Detection Kit

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