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Literature DB >> 12060694

A universal method to produce in vitro transcripts with homogeneous 3' ends.

Heike Schürer¹, Kathrin Lang, Jens Schuster, Mario Mörl.

Abstract

A method is described that allows a general drawback of in vitro transcription assays to be overcome: RNA polymerases tend to add extra nucleotides to the RNA 3' end that are not encoded in the linearized DNA template. Furthermore, these polymerases show a considerable rate of premature termination close to the RNA's 3' end. These features lead to a decreased yield of full-length transcripts and often make it difficult to determine and isolate the correctly transcribed full-length RNA. The hammerhead ribozyme is frequently used in cis to cleave off these extra nucleotides. However, the upstream sequence requirements of this ribozyme restrict its general usability. In contrast, the hepatitis delta virus ribozyme has no such requirements and can therefore be applied to any RNA sequence in cis. Due to the catalytic activity of the ribozyme, the desired transcript is released as an RNA molecule with a homogeneous 3' end. The resulting 2',3'-cyclo-phosphate group of the released RNA can be easily and efficiently removed by T4 polynucleotide kinase treatment. The presented method can be applied for virtually any sequence to be transcribed and is therefore superior to other ribozyme strategies, suggesting possible applications in every field where transcripts with homogeneous 3' ends are required.

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Year: 2002 PMID： 12060694 PMCID： PMC117298 DOI： 10.1093/nar/gnf055

Source DB: PubMed Journal: Nucleic Acids Res ISSN： 0305-1048 Impact factor: 16.971

18 in total

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Authors: M D Been
Journal: Trends Biochem Sci Date: 1994-06 Impact factor: 13.807

9. Use of exonuclease III to determine the site of stable lesions in defined sequences of DNA: the cyclobutane pyrimidine dimer and cis and trans dichlorodiammine platinum II examples.

Authors: B Royer-Pokora; L K Gordon; W A Haseltine
Journal: Nucleic Acids Res Date: 1981-09-25 Impact factor: 16.971

10. In vitro and in vivo comparison of hammerhead, hairpin, and hepatitis delta virus self-processing ribozyme cassettes.

Authors: B M Chowrira; P A Pavco; J A McSwiggen
Journal: J Biol Chem Date: 1994-10-14 Impact factor: 5.157

68 in total

A universal method to produce in vitro transcripts with homogeneous 3' ends.

Review 1. Crystallization of RNA.

2. Differential role of the intermolecular base-pairs G292-C(75) and G293-C(74) in the reaction catalyzed by Escherichia coli RNase P RNA.

3. 3'-Phosphatase activity in T4 polynucleotide kinase.

4. In vitro RNA synthesis with SP6 RNA polymerase.

5. Preparation of specific ribosomal RNA fragments.

6. Synthesis of small RNAs using T7 RNA polymerase.

7. Direct chemical method for sequencing RNA.

Review 8. Cis- and trans-acting ribozymes from a human pathogen, hepatitis delta virus.

9. Use of exonuclease III to determine the site of stable lesions in defined sequences of DNA: the cyclobutane pyrimidine dimer and cis and trans dichlorodiammine platinum II examples.

10. In vitro and in vivo comparison of hammerhead, hairpin, and hepatitis delta virus self-processing ribozyme cassettes.

1. Exponential growth by cross-catalytic cleavage of deoxyribozymogens.

2. A simple and cost-effective method for producing small interfering RNAs with high efficacy.

3. Superior 5' homogeneity of RNA from ATP-initiated transcription under the T7 phi 2.5 promoter.

4. General plasmids for producing RNA in vitro transcripts with homogeneous ends.

5. Rapid preparation of RNA samples for NMR spectroscopy and X-ray crystallography.

6. A novel 4-base-recognizing RNA cutter that can remove the single 3' terminal nucleotides from RNA molecules.

7. Structure and function of the 3' terminal six nucleotides of the west nile virus genome in viral replication.

8. Generating in vitro transcripts with homogenous 3' ends using trans-acting antigenomic delta ribozyme.

9. An inhibitory C-terminal region dictates the specificity of A-adding enzymes.

10. Small RNA binding to the lateral surface of Hfq hexamers and structural rearrangements upon mRNA target recognition.