An optimized 80mer Synthego Scaffold is added on the 3′ end of your target sequence. For example, you will receive a sgRNA with the following format:

5′-AAUUUCACAGCUGCACAUA+Synthego Scaffold-3′

Synthego 100-mer sgRNA (MS Trace). Large single peak represents full-length product.

IVT-derived 105-mer guide RNA (MS Trace). Large n-1, n+1 and n+2 species are present.

CRISPRevolution sgRNA Efficiency & Consistency

Hi Quality In = High Quality Out

The chart below compares the editing efficiency (solid bars) and consistency (black lines) of sgRNAs against in vitro transcribed guide RNAs in HEK293T cells. The experiment was conducted by a third-party using three different gene targets and was replicated three times.

Working with stem cells or other difficult targets?
Try Chemically Modified Synthetic RNA.

Chemically modified sequences can provide additional RNA stability with improvements in editing efficiency for particular cell types (e.g. stem cells, K562, prokaryotic) and genomic targets that prove otherwise challenging to edit. For a chemically modified version of our synthetic RNA, we offer 2’-O-methyl analogs and 3’ phosphorothioate internucleotide linkages at the first three 5’ and 3’ terminal RNA residues.

• Editing Efficiency ++++
• Excellent Reproducibility
• General Cell Types and Basic Applications
• Full Length 100-mer Single Guide
• Your 17-20nt Target Sequence
• No Annealing
• Material for 10-20 Transfections
• Quantity: 3 nmol by OD260
• TE Buffer
• Nuclease-free Water
• Ships in 5-7 Business Days

*chemically modified

• Editing Efficiency +++++
• Excellent Reproducibility
• Primary and Stem Cells; Therapeutic Applications
• Full Length 100-mer Single Guide
• Your 17-20nt Target Sequence
• No Annealing
• Material for 10-20 Transfections
• Quantity: 3 nmol by OD260
• TE Buffer
• Nuclease-free Water
• Ships in 7-10 Business Days