Alteration of hairpin ribozyme specificity utilizing PCR. | Zendy

Paula Degrandis | Zendy; Arnold Hampel | Zendy; Scott Galasinski | Zendy; James Borneman | Zendy; Andy Siwkowski | Zendy; M. Altschuler | Zendy

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Alteration of hairpin ribozyme specificity utilizing PCR.

Author(s) -

Paula Degrandis,

Arnold Hampel,

Scott Galasinski,

James Borneman,

Andy Siwkowski,

M. Altschuler

Publication year - 1994

Publication title -

genome research

Language(s) - Uncategorized

Resource type - Journals

SCImago Journal Rank - 9.556

H-Index - 297

eISSN - 1549-5469

pISSN - 1088-9051

DOI - 10.1101/gr.4.3.139

Subject(s) - biology , ribozyme , computational biology , hairpin ribozyme , genetics , evolutionary biology , gene , rna

We have developed a method by which a researcher can quickly alter the specificity of a trans hairpin ribozyme. Utilizing this PCR method, two oligonucleotides, and any target vector, new ribozyme template sequences can be generated without the synthesis of longer oligonucleotides. We have produced templates with altered specificity for both standard and modified (larger) ribozymes. After transcription, these ribozymes show specific cleavage activity with the new substrate beta-glucuronidase (GUS), and no activity against the original substrate (HIV-1, 5' leader sequence). Utilizing this technique, it is also possible to produce an inactive ribozyme that can be used as an antisense control. Applications of this procedure would provide a rapid and economical system for the assessment of trans ribozyme activity.

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