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Ribonuclease R (RNase R), 250 U

$995.00

A 3´ to 5´ exoribonuclease that digests all linear RNAs except lariat or circular RNA structures. Specific: Digests all linear RNAs but does not digest lariat or circular RNA structures, or...

NAME SIZE ID AVAILABLITY VENDOR PRICE EX GST $35 FREIGHT FEE PER ORDER
Ribonuclease R (RNase R), 250 U EACH RNR07250 Enquire for stock availability Lucigen $995.00
PRODUCT INFORMATION

A 3´ to 5´ exoribonuclease that digests all linear RNAs except lariat or circular RNA structures.

  • Specific: Digests all linear RNAs but does not digest lariat or circular RNA structures, or doublestranded RNA with 3' overhangs shorter than seven nucleotides
  • Heat Inactivated: Heat at 65°C for 20 minutes to kill enzyme activity
  • Valuable: Use the unique properties of this exoribonuclease to study alternative splicing and gene expression

Ribonuclease R (RNase R) from E. coli is a magnesium-dependent 3´ to ;5´ exoribonuclease that digests essentially all linear RNAs but does not digest lariat or circular RNA structures1,2, or doublestranded RNA with 3´ overhangs shorter than seven nucleotides.2 Most cellular RNAs will be digested completely by RNase R, with the exception of tRNAs, 5S RNA, and intron lariats (Fig. 1). The 3´ tails of lariats will be trimmed by RNase R to the branch point nucleotide, where there is a 2´,5´-phosphodiester linkage. Lariats are produced during pre-mRNA splicing of intron regions and can be isolated from a mixture of total RNA by digestion with RNase R. The MasterPure™ RNA and Yeast RNA Purification Kits are ideal for such total RNA preparations.

Lariat RNAs isolated using this method can be used as a template to produce labeled cDNA as a target for microarrays containing potential intron sequences, or for tiling arrays containing overlapping regions of complete chromosomes or genomes. The cDNA produced will not be a linear representation of the intron, but the sequences contained in it will be intron-derived.

Applications

  • Alternative splicing and gene expression studies.
  • Intron cDNA production.
  • Intronic screening of cDNA libraries.

Unit Definition: One unit of RNase R converts 1 µg of poly(A) into acid-soluble nucleotides in 10 minutes at 37°C under standard assay conditions.

Storage Buffer: RNase R is supplied in a 50% glycerol solution containing 50 mM Tris-HCl (pH 7.5), 100 mM NaCl, 0.1 mM EDTA, 1 mM DTT, and 0.1% Triton® X-100.

RNase R 10X Reaction Buffer: 0.2 M Tris-HCl (pH 8.0), 1 M KCl, and 1 mM MgCl2.

Quality Control: RNase R is function-tested in a reaction containing a mixture of linear and circularised RNA oligonucleotides. Only the linear RNA is digested.

Note: RNase R requires low (0.1-1.0 mM) magnesium concentrations for activity. Low EDTA concentrations in substrate RNA solutions can negatively affect RNase R activity. Additional MgCl2 up to 1 mM final concentration can be used to compensate for EDTA in the substrate. Optimal activity is at 37°C.

rnase r

Figure 1. Schematic overview showing processing of intron lariats by RNase R.