그림1. The Guide-it Indel Identification Kit provides a complete workflow foridentifying the variety of insertions and deletions (indels) introduced bynuclease-based genome editing. The protocol uses direct PCR to amplify a genomic DNA fragment (~500 to 700 bp) containing thetarget site directly from crude cell lysates (step 1). The resulting amplifiedfragments contain a pool of edited target sites from individual cells. ThesePCR products are cloned directly into a pre-linearized pUC19 vector using theIn-Fusion cloning system (step 2).After transformation of an optimized E.coli strain, colony PCR is used to amplify the target site from the plasmid(step 3). DNA sequencing is then used to identify the different indelsgenerated at the targeted genomic site (step 4).

그림2. Identification of insertions and deletions (indels) in the CD81 gene afterCRISPR/Cas9 targeting. HeLa cells were transfectedwith plasmids encoding Cas9 and an sgRNA targeting the CD81 gene. The Guide-itIndel Identification Kit was used to prepare CD81 target sites for DNA sequenceanalysis. The sequencing data from six clones was aligned with the wild-typesequence, revealing a broad range of indels in the CD81 gene.

● Detecting insertions and deletions introduced in mammalian genomic DNA

● Characterizing the variety of indels that are present in a cell population after nuclease-based gene editing

● Guide-it Indel Identification Components

● 110μl Terra PCR Direct Polymerase Mix

● 3x 1 ml 2X Terra PCR Direct Buffer (with Mg²⁺, dNTP)

● 400μl Extraction Buffer 1

● 40 μl ExtractionBuffer 2

● 10 μl pUC19Cloning Vector, linearized (50 ng/μl)

● 200 μl ColonyPCR Forward Primer (15 μM)

● 200 μl ColonyPCR Reverse Primer (15 μM)

● 6x 1 ml PCR-Grade Water

● In-Fusion HD Cloning Kit

● NucleoSpin Gel and PCR Clean-Up Kit

● Stellar Competent Cells