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Use of terbium as a probe of tRNA tertiary structure and folding.

RNA (New York, N.Y.) (2000-12-06)
M R Hargittai, K Musier-Forsyth
ZUSAMMENFASSUNG

Lanthanide metals such as terbium have previously been shown to be useful for mapping metal-binding sites in RNA. Terbium binds to the same sites on RNA as magnesium, however, with a much higher affinity. Thus, low concentrations of terbium ions can easily displace magnesium and promote phosphodiester backbone scission. At higher concentrations, terbium cleaves RNA in a sequence-independent manner, with a preference for single-stranded, non-Watson-Crick base-paired regions. Here, we show that terbium is a sensitive probe of human tRNALys,3 tertiary structure and folding. When 1 microM tRNA is used, the optimal terbium ion concentration for detecting Mg2+-induced tertiary structural changes is 50-60 microM. Using these concentrations of RNA and terbium, a magnesium-dependent folding transition with a midpoint (KMg) of 2.6 mM is observed for unmodified human tRNALys,3. At lower Tb3+ concentrations, cleavage is restricted to nucleotides that constitute specific metal-binding pockets. This small chemical probe should also be useful for detecting protein induced structural changes in RNA.

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Sigma-Aldrich
Terbium(III)-chlorid Hexahydrat, 99.9% trace metals basis
Sigma-Aldrich
Terbium(III)-chlorid, anhydrous, powder, 99.99% trace metals basis
Sigma-Aldrich
Terbium(III)-chlorid Hexahydrat, 99.999% trace metals basis
Sigma-Aldrich
Terbium(III)-chlorid, anhydrous, powder, 99.9% trace metals basis