Conformational Heterogeneity at Position U37 of an All-RNA Hairpin Ribozyme with Implications for Metal Binding and the Catalytic Structure of the S-Turn<sup>,</sup>

Alam, Shabnam; Grum-Tokars, Valerie; Krucinska, J.; Kundracik, M.L.; Wedekind, Joseph E.

doi:10.1021/bi051550i

Cited by 49 publications

(118 citation statements)

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“…recall G8I/2'-OMe A−1 and G8I/2'-dA−1 revealed little change). Overall, subtle changes were observed in the conformation of the A38 base, which mirrored the results of a prior study in which U39 was replaced by a propyl linker (11). A comparison of the N1 positions of A38 from the most active conformation (i.e.…”

Section: Chemical Changes At Position 8 Alter the Scissile Bond Geometrysupporting

confidence: 76%

“…The closest potential Hbond partner is the O4' oxygen of residue A9, but this group is ∼3.6 Å away in the native and variant structures (on average). At present, it is unclear why the native G8 structure does not corroborate the solution data, although a previous structural study of the hairpin ribozyme supported the possibility that the S-turn motif in the crystal structure represented a folding intermediate (11). The G8I substitution itself was reported previously to cause a +2.2 kcal/mol increase in ΔΔG of the hairpin ribozyme during catalysis, as well as a 'strong' effect by NAIM (45,46).…”

Section: G8i Promotes a Cross-strand Loop A Domain Interactionmentioning

confidence: 84%

“…The 4WJ form of the hairpin ribozyme has been solved in complex with vanadate, thereby providing a spatial analogue for the trigonal bipyramidal transition state of this and other ribozyme reactions (10,23,39). A comparison of the vanadate complex to the native G8 , pre-catalytic structure of this and prior studies (9)(10)(11), revealed that τ = 144° for the vanadate mimic ( Figure 6B & Table 2). Although this angle is not ideal for phosphoryl transfer, several features suggest it is the closest available structure to the actual geometry of the reaction intermediate.…”

Section: Comparison Of Position 8 Variants To the Hairpin Ribozyme Vamentioning

confidence: 84%

“…The minute size of this 61-mer ( Figure 1A) enabled the facile incorporation of single-atom point alterations into the sequence by use of solid support chemical synthesis. This approach led to the identification of conformational heterogeneity at position U37 that could be eliminated by incorporation of a U39C point mutant (11). Overall, the structure of the minimal all-RNA variant ( Figure 1B) exhibited a modest 1.3 Å r.m.s.d.…”

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confidence: 99%

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Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer^,

et al. 2005

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The hairpin ribozyme requires functional group contributions from G8 to assist in phosphodiester bond cleavage. Previously, replacement of G8 by a series of nucleobase variants showed little effect on interdomain docking, but a 3-to 250-fold effect on catalysis. To identify G8 features that contribute to catalysis within the hairpin ribozyme active site, structures for five base variants were solved by X-ray crystallography in a resolution range between 2.3 to 2.7 Å. For comparison, a native all-RNA "G8" hairpin ribozyme structure was refined to 2.05 Å resolution. The native structure revealed a scissile bond angle (τ) of 158°, which is close to the requisite 180° 'in-line' geometry. Mutations G8(inosine), G8(diaminopurine), G8(aminopurine), G8(adenosine) and G8(uridine) folded properly, but exhibited non-ideal scissile bond geometries (τ ranging from 118° to 93°) that paralleled their diminished solution activities. A superposition ensemble of all structures, including a previously described hairpin ribozyme-vanadate complex, indicated the scissile bond can adopt a variety of conformations resulting from perturbation of the chemical environment, and provided a rationale for how the exocyclic amine of nucleobase 8 promotes productive, in-line geometry. Changes at position 8 also caused variations in the A−1 sugar pucker. In this regard, variants A8 and U8 appeared to represent non-productive ground-states in which their 2'-OH groups mimicked the pro-R, non-bridging oxygen of the vanadate transition-state complex. Finally, the results indicated that ordered water molecules bind near the 2'-hydroxyl of A−1, lending support to the hypothesis that solvent may play an important role in the reaction. † This work was supported by NIH Grant GM63162 to J.E.W. ‡ Protein Data Bank Codes for the reported structures: 1ZFR (G8), 1ZFT (G8I), 1ZFV (G8A), 1ZFX (G8U), 2BCY (G8AP), 2BB1 (G8DAP), 2BCZ (G8I/dA−1). § Present address: Rosalind Franklin School of Science and Medicine, Dept. Biochem. and Mol. Biol., 3333 Green Bay Road Rd., N. Chicago, IL 60064, USA * To whom correspondence should be addressed: Department of Biochemistry and Biophysics, University of Rochester School of Medicine and Dentistry, 601 Elmwood Ave, Box 712, Rochester, New York 14642 USA. Phone: 585 273-4516; Fax: 585 275-6007; Email: Joseph_Wedekind@URMC.Rochester.edu ∥ These authors contributed equally to this work.Supporting Information Available A stereo diagram of representative electron density maps is provided for the native and position 8 variants of this study (Figure 1). A diagram comparing the G8I/2'-OMe A−1 and G8I/2'-deoxy A−1 variants is also available (Figure 2). The method for HPLC composition analysis of AP8 and DAP8 crystals is reported, as well as elution profiles for the separated hairpin ribozyme strands (Figure 3). This information is provided free of charge at http://pubs.acs.org NIH Public Access The hairpin ribozyme is a small ribozyme whose family members catalyze a reversible, sitespecific phosphodiester bond cleavage reacti...

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Section: Chemical Changes At Position 8 Alter the Scissile Bond Geometrysupporting

confidence: 76%

Section: G8i Promotes a Cross-strand Loop A Domain Interactionmentioning

confidence: 84%

Section: Comparison Of Position 8 Variants To the Hairpin Ribozyme Vamentioning

confidence: 84%

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confidence: 99%

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Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer^,

et al. 2005

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“…The trend in reactivity did not appear to be the result of changes from an N1 to N3 moiety or to be correlated strictly with the substituted group's imino pK a . Moreover, no effort was made to relate the substituted nucleobase to its propensity to favor the syn conformation, which is preferred by Ade38 in the native state (Rupert and Ferré-D'Amaré 2001;Rupert et al 2002;Alam et al 2005;Salter et al 2006;MacElrevey et al 2007;Torelli et al 2007Torelli et al , 2008. Although it is tempting to accept such modifications as pure indicators of chemical functionality, previous studies indicated that single nucleobase changes could evoke large, unforeseen conformational alterations, thus obfuscating the direct assignment of catalytic determinants (Alam et al 2005;Salter et al 2006).…”

Section: Introductionmentioning

confidence: 99%

Structural effects of nucleobase variations at key active site residue Ade38 in the hairpin ribozyme

MacElrevey¹,

Salter²,

Krucinska³

et al. 2008

RNA

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The hairpin ribozyme requires functional groups from Ade38 to achieve efficient bond cleavage or ligation. To identify molecular features that contribute to catalysis, structures of position 38 base variants 2,6-diaminopurine (DAP), 2-aminopurine (AP), cytosine (Cyt), and guanine (Gua) were determined between 2.2 and 2.8 Å resolution. For each variant, two substrate modifications were compared: (1) a 29-O-methyl-substituent at Ade-1 was used in lieu of the nucleophile to mimic the precatalytic state, and (2) a 39-deoxy-29,59-phosphodiester linkage between Ade-1 and Gua+1 was used to mimic a reactionintermediate conformation. While the global fold of each variant remained intact, the results revealed the importance of Ade38 N1 and N6 groups. Absence of N6 resulting from AP38 coincided with failure to localize the precatalytic scissile phosphate. Cyt38 severely impaired catalysis in a prior study, and its structures here indicated an anti base conformation that sequesters the imino moiety from the scissile bond. Gua38 was shown to be even more deleterious to activity. Although the precatalytic structure was nominally affected, the reaction-intermediate conformation indicated a severe electrostatic clash between the Gua38 keto oxygen and the pro-Rp oxygen of the scissile bond. Overall, position 38 modifications solved in the presence of 29-OMe Ade-1 deviated from in-line geometry, whereas variants with a 29,59 linkage exhibited S-turn destabilization, as well as base conformational changes from syn to anti. These findings demonstrate the importance of the Ade38 Watson-Crick face in attaining a reaction-intermediate state and the sensitivity of the RNA fold to restructuring when electrostatic and shape features fail to complement.

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Chemical Mechanisms of the Nucleolytic Ribozymes

Wilson

Lilley

2021

Ribozymes

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Conformational Heterogeneity at Position U37 of an All-RNA Hairpin Ribozyme with Implications for Metal Binding and the Catalytic Structure of the S-Turn^,

Cited by 49 publications

References 56 publications

Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer^,

Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer^,

Structural effects of nucleobase variations at key active site residue Ade38 in the hairpin ribozyme

Chemical Mechanisms of the Nucleolytic Ribozymes

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Conformational Heterogeneity at Position U37 of an All-RNA Hairpin Ribozyme with Implications for Metal Binding and the Catalytic Structure of the S-Turn,

Cited by 49 publications

References 56 publications

Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer,

Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer,

Structural effects of nucleobase variations at key active site residue Ade38 in the hairpin ribozyme

Chemical Mechanisms of the Nucleolytic Ribozymes

Contact Info

Product

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About

Conformational Heterogeneity at Position U37 of an All-RNA Hairpin Ribozyme with Implications for Metal Binding and the Catalytic Structure of the S-Turn^,

Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer^,

Water in the Active Site of an All-RNA Hairpin Ribozyme and Effects of Gua8 Base Variants on the Geometry of Phosphoryl Transfer^,