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      Regio-selective chemical-enzymatic synthesis of pyrimidine nucleotides facilitates RNA structure and dynamics studies.

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          Abstract

          Isotope labeling has revolutionized NMR studies of small nucleic acids, but to extend this technology to larger RNAs, site-specific labeling tools to expedite NMR structural and dynamics studies are required. Using enzymes from the pentose phosphate pathway, we coupled chemically synthesized uracil nucleobase with specifically (13) C-labeled ribose to synthesize both UTP and CTP in nearly quantitative yields. This chemoenzymatic method affords a cost-effective preparation of labels that are unattainable by current methods. The methodology generates versatile (13) C and (15) N labeling patterns which, when employed with relaxation-optimized NMR spectroscopy, effectively mitigate problems of rapid relaxation that result in low resolution and sensitivity. The methodology is demonstrated with RNAs of various sizes, complexity, and function: the exon splicing silencer 3 (27 nt), iron responsive element (29 nt), Pro-tRNA (76 nt), and HIV-1 core encapsidation signal (155 nt).

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          Author and article information

          Journal
          Chembiochem
          Chembiochem : a European journal of chemical biology
          1439-7633
          1439-4227
          Jul 21 2014
          : 15
          : 11
          Affiliations
          [1 ] Center for Biomolecular Structure and Organization, Department of Chemistry and Biochemistry, University of Maryland, 1115 Biomolecular Sciences Building, College Park, MD 20782 (USA).
          Article
          NIHMS614743
          10.1002/cbic.201402130
          4127085
          24954297
          9e80d5a6-c56b-4a4d-a2f7-6d4caceda913
          © 2014 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.
          History

          NMR spectroscopy,RNA,dynamics,labeling,structure
          NMR spectroscopy, RNA, dynamics, labeling, structure

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