RNase H MBG

For the removal of mRNA after first-strand cDNA synthesis

S_1283_1_LS_IR_Enzyme_Rnase_H_MBG_250U
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RNase H MBG (250 U)

Cat. No. / ID:   RT34-025

5 U/μL concentration. Storage temperature: -20°C
480,00 BRL
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Quantity
250 U
1250 U
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The RNase H MBG is intended for molecular biology applications. This product is neither intended for the diagnosis, prevention or treatment of a disease, nor has it been validated for such use either alone or in combination with other products.
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Features

  • Specifically hydrolyzes the phosphodiester bonds of RNA hybridized into DNA
  • Prevents degradation of single and double-stranded DNA or un-hybridized RNA
  • Improves sensitivity and prevents binding of amplification primers in a PCR reaction through binding of RNA to cDNA template

Product Details

RNase H is an 18.9 kDa recombinant endoribonuclease purified from an Escherichia coli strain, which over-expresses cloned RNase H gene (rnh).


It specifically hydrolyzes the phosphodiester bonds of RNA hybridized to DNA and produces 5´ phosphate-terminated oligoribonucleotides and single-stranded DNA. RNase H does not degrade single and double-stranded DNA or unhybridized RNA. It is a key enzyme in the removal of mRNA after first-strand cDNA synthesis.


It is supplied with 200 mM Tris-HCl (pH 8.4), 500 mM KCl, 50 mM MgCl2 and 200 mM DTT Reaction Buffer (10x).


One unit catalyzes the hydrolysis of 1 nmol of RNA in [3H]-labeled poly(A)×poly(dT) to acid-soluble ribonucleotides in a total reaction volume of 50 µL in 20 minutes at 37°C in 1x Reaction Buffer.

 

Performance

Assay Specification
Protein Purity >90%
RNase contamination None detected
DNase contamination None detected
Proteases contamination None detected

 

Principle

Treating cDNA with RNase H prior to PCR can improve sensitivity as RNA bonded to the cDNA template may prevent binding of the amplification primers in a PCR reaction. RNase H treatment is often necessary when amplifying longer, full-length cDNA targets. In addition, RNase H is useful for removing poly(A) tails on mRNAs after hybridization with oligo(dT) and for the site-specific enzymatic cleavage of RNA.

Procedure

Quality Control

Protein purity is evaluated using Coomassie Blue detection assay by SDS-PAGE electrophoresis resulting in >90% purity. The relevant procedures have confirmed the absence of DNase, RNase and protease activity.


RNase and DNase contamination is evaluated by assessing RNase activity through gel electrophoresis following the incubation of RNA at 37°C.


Protease activity is also determined by SDS-PAGE electrophoresis.


Usage


Use 5 U of the enzyme to remove RNA from an RNA:DNA duplex after reverse transcription in a 20 μL reaction. If a 50 μL reaction is desired, 12.5 U of the enzyme is recommended.


The reaction mixture should be incubated at 37⁰C for 20 minutes.

 

Applications

This is used for applications such as:

  • Removal of RNA after first strand cDNA synthesis (RT-PCR and qRT-PCR)
  • Removal of mRNA prior to synthesis of second strand cDNA
  • Removal of the poly(A) sequences of mRNA after hybridization with oligo(dT)
  • Site-specific cleavage of RNA
  • Studies of in vitro polyadenylation reaction products

 

Resources

Certificates of Analysis (1)