Home Protocols Nicking a single ribonucleotide site within a dsDNA substrate or an Okazaki fragment with RNase HII (NEB #M0288)

Nicking a single ribonucleotide site within a dsDNA substrate or an Okazaki fragment with RNase HII (NEB #M0288)

Overview

The following is a typical reaction protocol for nicking at the site of a single ribonucleotide within a dsDNA substrate or for nicking an Okazaki fragment 5´ to the ribonucleotide adjacent to the DNA

Protocol

Reaction mix:

Resuspend 100 pmol of double-stranded substrate into 50 μl of 1X ThermoPol Buffer.
Add 1 μl of RNase II and mix thoroughly.
Incubate at 37°C for 30 minutes.

Note: To achieve the best results for a given substrate, it is often helpful to test more than one concentration of ribonuclease.

Nicking a single ribonucleotide site within a dsDNA substrate or an Okazaki fragment with RNase HII (NEB #M0288)

Overview

Protocol

Choose your country

North America

Europe

Asia-Pacific

Find a Golden Butterfly for a Chance to Win!