Reverse Sanger sequencing of RNA by MALDI-TOF mass spectrometry after solid phase purification

doi:10.1093/nar/gnh089

Nucleic Acids Research 2004 32(12):e97; doi:10.1093/nar/gnh089

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Published online 7 July 2004

Reverse Sanger sequencing of RNA by MALDI-TOF mass spectrometry after solid phase purification

Beatrice Spottke, Julia Gross², Hans-Joachim Galla¹ and Franz Hillenkamp^*

Institute for Medical Physics and Biophysics and ¹ Institute for Biochemistry, University of Münster, Münster, Germany and ² Department of Chemistry, Washington University, St Louis, MO 63130, USA

^* To whom correspondence should be addressed. Tel: +49 251 83 55103; Fax: +49 251 83 55121; Email: hillenk{at}uni-muenster.de

Received April 27, 2004; Revised and Accepted June 4, 2004

Several DNA/RNA sequencing strategies have been developed usingmatrix-assisted laser desorption ionization mass spectrometry(MALDI-MS). In the reverse Sanger sequencing approach ${alpha}$ -thiophosphate-containingNTPs are employed. Sequencing ladders are produced by the subsequentexonuclease cleavage, which is inhibited by the ${alpha}$ -S-NTP at the3' terminus. Here the reverse Sanger sequencing of RNA is described.The stability of RNA during the UV-MALDI process is higher relativeto DNA, and RNA can be easily synthesized by transcription usingbacteriophage RNA polymerase. ${alpha}$ -S-rNTP was added to the reactionin a ratio of 1:3 to the native rNTPs and was incorporated statisticallyby the RNA polymerase. Four separate sequence ladders were produced,to avoid the problem of the only 1u mass difference betweenuridine and cytidine. However, it was shown that RNA transcriptiondoes not produce homogeneous transcripts. Therefore isolationof the full-length transcript is required to attain a non-ambiguousinterpretation of cleavage spectra. This is achieved by theexclusive immobilization of the full-length transcript on asolid phase. The full-length transcripts were hybridized tomagnetic beads, coated with short universal sequences, complementaryto the in vitro RNA. After purification and isolation the RNAfull-length transcript is cleaved by snake venom phosphodiesterase(SVP) and the obtained sequence ladder is analyzed by MALDI-MS.

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