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Restriction Enzyme Reference

Searchable guide for 60+ common restriction enzymes — recognition sequences, cut sites, overhang types, heat inactivation, and buffer recommendations. Click any enzyme for full details.

✂️ Restriction Enzyme Reference FREE TOOL
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Overhang: 5′ Sticky 3′ Sticky Blunt
Showing 60 enzymes — click any row for full details
Enzyme Recognition Sequence (5′→3′) Cut Site Overhang Overhang Seq Heat Inact. Buffer

How to Use the Restriction Enzyme Reference

Search: Type an enzyme name (e.g. EcoRI), recognition sequence (e.g. GAATTC), or overhang type (e.g. 5-prime) to filter instantly.

Filter buttons: Filter by overhang type — 5′ sticky ends, 3′ sticky ends, or blunt ends.

Click any row to see the full detail panel with recognition sequence diagram, compatible ends, methylation sensitivity, and protocol notes.

About Restriction Enzymes

Restriction endonucleases are bacterial enzymes that cut double-stranded DNA at or near specific recognition sequences. They are essential tools in molecular cloning, DNA mapping, and recombinant DNA technology.

// Types of restriction enzyme cut ends:
5′ overhang (sticky): 5′—AATTC—3′ ← most common, e.g. EcoRI
3′—C —5′

3′ overhang (sticky): 5′—C —3′ ← e.g. KpnI, SacI
3′—CATGG—5′

Blunt ends: 5′—GG|CC—3′ ← e.g. SmaI, EcoRV
3′—CC|GG—5′

// ↑ = cut position on top strand
// Compatible (cohesive) ends ligate efficiently

Choosing the Right Enzyme

When planning a cloning experiment, choose enzymes that produce compatible ends for ligation. Check that the enzyme does not cut within your insert or vector sequence. Also verify that the enzyme is not blocked by Dam, Dcm, or CpG methylation if your DNA is from a methylation-positive strain.

Heat Inactivation

Many restriction enzymes can be inactivated by heating to 65°C or 80°C for 20 minutes, eliminating the need for column purification before ligation. Enzymes marked "No" or "65°C" in this table require gel or column cleanup before ligation.

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