Sequential Double Digest

Abstract

This is the Sequential Double Digest Protocol with Standard Restriction Enzymes. If there is no buffer in which the two enzymes exhibit > 50% activity, this sequential digest can be performed.

Before start

NEB's online tools, Double Digest Finder and NEBcloner will help guide your reaction buffer selection when setting up double digests.

Steps

Set up the following reaction using the restriction endonuclease that has the lowest salt concentration in its recommended buffer (total reaction volume 50 µl ).

Note

A 50 µl reaction volume is recommended for digestion of 1 µg of substrate.

Note

The enzyme should be the last component added to reaction

Mix components by pipetting the reaction mixture up and down, or by "flicking" the reaction tube.

Quick ("touch") spin-down in a microcentrifuge. Do not vortex the reaction.

Incubate for 1 hour at the enzyme-specific appropriate temperature.

Adjust the salt concentration of the reaction (using a small volume of a concentrated salt solution) to approximate the reaction conditions of the second restriction endonuclease.

Note

Alternatively, a spin column can be used to isolate the DNA prior to the second reaction.

Add the second enzyme.

Mix components by pipetting the reaction mixture up and down, or by "flicking" the reaction tube.

Quick ("touch") spin-down in a microcentrifuge. Do not vortex the reaction.

Incubate for 1 hour at the enzyme-specific appropriate temperature.

Abstract

Before start

Steps

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