RNase H cleavage for processing of in vitro transcribed RNA for NMR studies and RNA ligation.
- 1 March 1996
- journal article
- Vol. 2 (3) , 289-96
Abstract
Large quantities of RNA for study by NMR and X-ray crystallography can be produced by transcription reactions in vitro using T7 bacteriophage RNA polymerase. A limitation on producing RNA with this polymerase has been the strong dependence of the yield of the transcription reaction on the sequence at the 5' end of the RNA produced. We report a procedure for obtaining large quantities of enzymatically synthesized RNA from T7 RNA polymerase that has no dependence on the 5' end sequence of the target RNA. Ribonuclease H has been shown previously (Inoue H, Hayase Y, Iwai S, Ohtsuka E, 1987, FEBS Lett 215:327-330) to cleave RNA site specifically using 2'-O-methyl RNA/DNA chimeras to direct the cleavage site. We show that 2'-O-methyl RNA nucleotides on the 5'-side of the DNA nucleotides in the chimera are not essential for site-specific cleavage. This allowed us to design the method such that the same 2'-O-methyl chimera may be used to process any RNA sequence. We have adapted this reaction to the cleavage of NMR-scale quantities of RNA at high yield. RNA is synthesized using T7 RNA polymerase with a 15-nt high-yielding leader sequence at the 5' end, and then this sequence is cleaved off with the RNase H cleavage reaction. The cleaved RNA has 3'-hydroxyl and 5'-phosphate ends, so that the products can be used directly as substrates for ligation by T4 DNA ligase. We show that the cleavage reaction occurs efficiently in solution and on a solid streptavidin/agarose matrix. We report an example in which we are able to improve transcription yield by more than five-fold using this technique in the synthesis of a 15N isotopically labeled hairpin found in the Crithidia fasciculata spliced leader RNA. We are able to obtain a 0.5-mM NMR sample from this inherently poorly transcribing sequence, while minimizing the amount of isotopically labeled rNTPs used to produce it. The NMR spectroscopic results are consistent with the predicted RNA secondary structure.This publication has 14 references indexed in Scilit:
- Assignment of NH resonances in nucleic acids using natural abundance 15N‐1H correlation spectroscopy with spin‐echo and gradient pulsesFEBS Letters, 1993
- Synthesis and purification of large amounts of RNA oligonucleotides.1991
- Construction of a novel RNA-transcript-trimming plasmid which can be used bothin vitroin place of run-off and (G)-free transcriptions andin vivoas multi-sequences transcription vectorsNucleic Acids Research, 1991
- Rapid and simple purification of T7 RNA polymeraseNucleic Acids Research, 1991
- [5] Synthesis of small RNAs using T7 RNA polymerasePublished by Elsevier ,1989
- ompT encodes the Escherichia coli outer membrane protease that cleaves T7 RNA polymerase during purificationJournal of Bacteriology, 1988
- Sequence‐dependent hydrolysis of RNA using modified oligonucleotide splints and RNase HFEBS Letters, 1987
- Oligoribonucleotide synthesis using T7 RNA polymerase and synthetic DNA templatesNucleic Acids Research, 1987
- Cloning and expression of the gene for bacteriophage T7 RNA polymerase.Proceedings of the National Academy of Sciences, 1984
- Isolation and Characterization of an Endonuclease from Escherichia coli Specific for Ribonucleic Acid in Ribonucleic Acid·Deoxyribonucleic Acid Hybrid StructuresJournal of Biological Chemistry, 1973