Metal ion catalysis during group II intron self-splicing: parallels with the spliceosome

doi:10.1101/gad.13.13.1729

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Vol. 13, No. 13, pp. 1729-1741, July 1, 1999

RESEARCH PAPER
Metal ion catalysis during group II intron self-splicing: parallels with the spliceosome

Erik J. Sontheimer,¹^,³ Peter M. Gordon,¹ and Joseph A. Piccirilli¹^,²^,⁴

¹ Department of Biochemistry and Molecular Biology, ² Department of Chemistry, Howard Hughes Medical Institute, University of Chicago, Chicago, Illinois 60637 USA

Abstract

Top
Abstract
Introduction
Results
Discussion
Materials and methods
References

The identical reaction pathway executed by the spliceosome and self-splicing group II intron ribozymes has prompted the ideathat both may be derived from a common molecular ancestor. Theminimal sequence and structural similarities between group IIintrons and the spliceosomal small nuclear RNAs, however, haveleft this proposal in question. Mechanistic comparisons betweengroup II self-splicing introns and the spliceosome are thereforeimportant in determining whether these two splicing machineriesmay be related. Here we show that 3'-sulfur substitution at the5' splice site of a group II intron causes a metal specificityswitch during the first step of splicing. In contrast, 3'-sulfursubstitution has no significant effect on the metal specificityof the second step of cis-splicing. Isolation of the second stepuncovers a metal specificity switch that is masked during thecis-splicing reaction. These results demonstrate that group IIintron ribozymes are metalloenzymes that use a catalytic metalion for leaving group stabilization during both steps of self-splicing.Furthermore, because 3'-sulfur substitution of a spliceosomalintron has precisely the same effects as were observed duringcis-splicing of the group II intron, these results provide strikingparallels between the catalytic mechanisms employed by these twosystems.

[Key Words: Group II intron; spliceosome; ribozyme; metal ion catalysis; 3'-S-phosphorothiolate; phosphotransesterification]

	Introduction

Top Abstract Introduction Results Discussion Materials and methods References

Several classes of intervening sequences (introns) exist in eukaryotic genomes, and each class is removed (spliced) post-transcriptionallyby a distinct pathway. Most introns are removed by a large RNA-proteincomplex called the spliceosome (Nilsen 1998; Burge et al. 1999),but some (group I and group II introns) self-splice by virtueof a catalytic activity resident in the intron RNA itself (Cechand Golden 1999). Excision of group II introns occurs by a two-steptransesterification pathway involving 5' splice site cleavagefollowed by exon ligation; the 2'-hydroxyl group of an adenosineresidue within the intron is usually the first-step nucleophile,leading to excision of the intron in the form of a lariat (Micheland Ferat 1995; Pyle 1996). Although spliceosomes are of muchgreater size and complexity, they catalyze intron removal by thesame chemical pathway, leading to speculation that the spliceosomeis essentially an RNA catalyst that shares a common molecularancestor with group II introns (Sharp 1985; Cech 1986).

The discovery of introns immediately prompted many ideas and questions about the roles of introns in the evolution of genomes(e.g., Gilbert 1978; Darnell 1978; Doolittle 1978). The centralissue has become one of intron antiquity, that is, whether intron-exonstructure predates the divergence of eubacteria, archaebacteria,and eukaryotes. The introns early/late question has been debatedvigorously, and most of the evidence has focused on the conservationof intron positions, the correlation between intron positionsand protein structure, and the distribution of intron phases forspliceosomal introns from genes present in all three kingdoms(for reviews, see Gilbert et al. 1997; Logsdon 1998). Anotherline of inquiry concerns the molecular mechanisms of intron removal $---$ ifthese spliceosomal introns are ancient or are derived from anancient precursor, then the mechanisms by which they are removedmay be ancient as well. Because catalytic RNAs are often thoughtof as `molecular fossils' from an ancient `RNA World' epoch (Gestelandet al. 1999), understanding whether spliceosomal introns are removedby an RNA-based mechanism is important to the debate over intronantiquity. As a result, the possible evolutionary relationshipbetween the spliceosome and the group II ribozymes has receiveda great deal ofinterest.

Evolutionary relationships between macromolecules are often inferred from similarities of sequence and structure. With regardto group II introns and the spliceosomal introns and small nuclearRNAs (U1, U2, U4, U5, and U6), conserved GU dinucleotides at the5' splice sites and AGC trinucleotides within presumptive catalyticdomains (for reviews, see Pyle 1996; Burge et al. 1999) have beennoted, but these similarities are extremely limited and theirsignificance has been questioned (Weiner 1993; Michel and Ferat1995). As for structure, our understanding of these two systemsis still fragmentary, but certain elements of secondary and tertiarystructure bear some resemblance to each other. In the spliceosome,the U6/5' splice site pairing, U2/U6 helix 1 region, U2/branchpointbulged duplex, and U5/exon interactions have been viewed as analogous(and perhaps homologous) to the $epsilon$ - $epsilon$ ' pairing, domain 5, domain6, and EBS-1/IBS1 and $delta$ - $delta$ ' interactions, respectively, in groupII introns (for reviews, see Michel and Ferat 1995; Nilsen 1998).Functional complementation of an EBS1/ $delta$ deletion by the U5 conservedloop has made the latter similarity particularly compelling (Hetzeret al. 1997). Although these similarities are tantalizing, somedifferences exist as well (Michel and Ferat 1995), and the proposedevolutionary kinship between the spliceosome and group II intronsremainsdebatable.

Possible relationships can also be judged by a "mechanistic phylogeny" involving comparisons of reaction pathways and catalyticmechanisms. The only such information obtained for both systemsthus far comes from the analysis of chiral phosphorothioates atthe splice sites. In both the spliceosome (Maschhoff and Padgett1993; Moore and Sharp 1993) and group II introns (Padgett et al.1994), incorporation of an R_P phosphorothioate at either splicesite blocks the reaction, but incorporation of the S_P diastereomerdoes not; furthermore, reaction at each S_P phosphorothioate resultsin inversion of stereochemistry, indicative of direct in-lineS_N2 nucleophilic attack. These results provide additionalevidence for a common reaction pathway catalyzed by both systems,but whether this commonality extends to the catalytic mechanismsthemselves remainsunknown.

We reported recently experiments that bear directly on the catalytic mechanisms employed by the spliceosome (Sontheimer etal. 1997). Incorporation of a 3'-S-phosphorothiolate linkage (inwhich the 3'-oxygen is replaced by sulfur) at the 5' splice sitegives rise to a metal specificity switch for the first step ofsplicing, providing strong evidence that a catalytic metal ionin the spliceosomal active site stabilizes the leaving group bydirect coordination. In contrast, 3'-sulfur substitution at the3' splice site has no effect on the metal specificity of the secondstep of the reaction. This result argues that inner-sphere coordinationof the leaving group by a metal ion may not be required for thisreaction, although a rate-limiting binding or conformational stepmay mask an inhibitory effect on the chemical step of 3' splicesite cleavage and exon ligation. Because of the expectation thatmost catalytic RNAs may use divalent metal ions for catalysis(for review, see Narlikar and Herschlag 1997), the former possibilitywas viewed as weakening the case for RNA catalysis in the secondstep of the spliceosomereaction.

We have now extended this analysis to reactions catalyzed by the ai5 $gamma$ group II intron ribozyme from Saccharomyces cerevisiaemitochondria. We find that 3'-sulfur substitution at the 5' splicesite results in a metal specificity switch for the first reactionstep, demonstrating that group II introns, like the spliceosome,use a catalytic metal ion for leaving group stabilization viainner-sphere coordination. The most striking parallel with thespliceosome, however, is that 3'-sulfur substitution at the 3'splice site has little or no effect on metal ion specificity duringcis-splicing. Therefore, spliceosomal and group II introns exhibitthe same asymmetric response to 3'-sulfur substitution at the5' and 3' splice sites during cis-splicing. To probe further theeffect of 3'-sulfur substitution at the 3' splice site, we isolated3' splice site cleavage and exon ligation from the rest of thecis-splicing pathway using a trans reaction. Under these conditions,a metal specificity switch is uncovered, indicating that a metalion also stabilizes the leaving group in the second step of splicingand suggesting that a conformational change (Chanfreau and Jacquier1996) limits the rate of exon ligation during cis-splicing.

	Results

Top Abstract Introduction Results Discussion Materials and methods References

3'-S-phosphorothiolate diesters have proven to be useful analogs in the analysis of the catalytic mechanisms used by RNA,protein, and ribonucleoprotein enzymes (Sontheimer 1999). Oxygenand sulfur differ in their abilities to occupy the inner ligandsphere of various metal ions (Sigel et al. 1997 and referencestherein); for instance, Mg²⁺ (a "hard" metal) coordinates well to oxygen, but strongly resistscoordination to sulfur. In contrast, "soft" metals such as Mn²⁺, Co²⁺, Zn²⁺, and Cd²⁺ readily accept (and in some cases prefer) sulfur as an inner-sphereligand. For a divalent-metal-dependent reaction that involvesa 3'-oxygen as the leaving group (such as splicing), a changein metal specificity from Mg²⁺ to a softer metal upon 3'-sulfur substitution implicates a directmetal ion-leaving groupinteraction.

Group II introns can self-splice by either of two routes $---$ a "branching" or transesterification pathway or a hydrolytic pathway(Fig. 1A). Both can be relevant in vivo (Podar et al. 1998a);in vitro, either pathway can predominate, depending on the ionicconditions (Daniels et al. 1996). The excised intron is stablein vitro and can catalyze hydrolysis at the exon-exon junctionof the spliced product. This spliced exons reopening (SER) reactionis mechanistically analogous to the reversal of the second stepof splicing (Podar et al. 1995). To test for the presence of catalyticmetal ions in the active site(s) of the group II ribozyme, weused a combination of chemical synthesis (Sun et al. 1997) andenzymatic ligation (Moore and Query 1998) to introduce a 3'-S-phosphorothiolatediester at the site of cleavage for the first (Fig. 1B) and second(Fig. 1C) steps of cis-splicing.

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Figure 1. 3'-Sulfur substitution at the splice sites of a group II intron. (A) The pathways of group II intron self-splicing. Splicing proceeds by either of two pathways, which differ in the identity of the nucleophile during the first step of the reaction. In the branching or transesterification pathway (left), the 2'-hydroxyl group of an adenosine residue attacks the 5' splice site, giving rise to the exon 1 and lariat intron/exon 2 intermediates. In the hydrolytic pathway (right), water or hydroxide attacks the 5' splice site, and the intron/exon 2 intermediate is linear. For both pathways, the second step proceeds by attack of the 3'-hydroxyl group of exon 1 on the 3' splice site, giving rise to spliced exons and releasing the excised intron. As shown at the bottom, released intron can catalyze a SER hydrolytic reaction. (B) 5' Splice site substitution. A simplified depiction of the yeast mitochondrial group II intron ai5 $gamma$ is given at the top; exons are boxed, and each of the six intron domains is indicated. The bulged A residue that acts as a nucleophile in the first reaction step is shown in domain 6. The sequence of the 5' splice junction is given underneath [(C_S) 3'-thiocytidine]. The structure of the 3'-S-phosphorothiolate linkage at the 5' splice site is given at the bottom. (C) 3' Splice site substitution. The diagram is as in B, except that the sequence and the 3'-S-phosphorothiolate linkage are for the 3' splice site [(U_S) 3'-thiouridine].

3'-Sulfur substitution at the 5' splice site of a group II intron results in a metal specificity switch

Self-splicing constructs with a 3'-sulfur substitution (Fig. 1B) or a normal 3'-oxygen at the 5' splice site were constructedand tested for cis-splicing activity in vitro (Fig. 2A) in thepresence of 0.5 M (NH₄)₂SO₄ and 100 mM divalent metal ion (Danielset al. 1996). For the control substrate, no reaction occurredin the absence of divalent metals (Fig. 2A, lane 4), but exon1 and spliced product were both generated in the presence of 100mM MgCl₂ (Fig. 2A, lane 5). When the reactions included 10 or20 mM MnCl₂, CoCl₂, ZnCl₂, or CdCl₂ (Fig. 2A, lanes 6-13), exon1 and spliced product were easily detected, indicating that thepresence of these metal ions allows efficient splicing (althoughCoCl₂, ZnCl₂, and CdCl₂ appear to affect the relative rates ofthe first and second steps, as indicated by the decreased amountsof exon 1 in Fig. 2A, lanes 8-13). For the 3'-sulfur-containingsubstrate, no reaction was observed in the absence of divalentmetals (Fig. 2A, lane 17). Unlike the control substrate, however,no reaction was observed in the presence of 100 mM MgCl₂ (Fig.2A, lane 18). Inclusion of 10 or 20 mM MnCl₂, ZnCl₂, or CdCl₂restored efficient 5' splice site cleavage (Fig. 2A, lanes 19,20, and 23-26), demonstrating a switch in metal specificity forthis reaction. CoCl₂ (10 or 20 mM) was unable to restore 5' splicesite cleavage (Fig. 2A, lanes 21-22). Although MnCl₂, ZnCl₂, orCdCl₂ rescued the first step of the reaction, no spliced productwas generated (Fig. 2A, lanes 19, 20, and 23-26), consistent withthe observation that sulfur is a very poor nucleophile at phosphodiesterlinkages (Pearson 1966; Dantzmann and Kiessling 1996).

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Figure 2. (A) 3'-Sulfur substitution at the 5' splice site of a group II intron results in a metal specificity switch. Self-splicing reactions were performed with ligated substrates containing a 3'-oxygen (lanes 1-13) or a 3'-sulfur (lanes 14-26) at the 5' splice site (see Fig. 1B). (Lanes 1,14) Unspliced RNAs; each substrate was also mock-reacted (lanes 2,15) or reacted (lanes 3,16) with silver(I). Self-splicing reactions were carried out for 1 hr and contained 5 mM EDTA (lanes 4, 17), 100 mM MgCl₂ (lanes 5,18), or 10 or 20 mM MnCl₂, CoCl₂, ZnCl₂, or CdCl₂ (lanes 6-13, 19-26) as indicated at the top of each lane. Reactions in the presence of MnCl₂, CoCl₂, ZnCl₂, or CdCl₂ were supplemented with MgCl₂ so that the total divalent metal ion concentration was 100 mM. Unspliced precursor (1017 nucleotides), exon 1 intermediate (70 nucleotides), and spliced product (130 nucleotides) are indicated on the left, and the sizes of the DNA markers (in nucleotides) are given on the right. The intron/exon 2 intermediates (lariat and linear) and the corresponding excised intron products contain no radiolabel and are therefore not visible. As an additional standard, lane 27 is a silver cleavage reaction of a 3'-sulfur-containing RNA (79 nucleotides) consisting of exon 1 and only 9 nucleotides of intron sequence. (B) 5' Splice site cleavage of the 3'-sulfur-substituted substrate occurs accurately in the presence of Mn²⁺. The strategy for mapping the site of cleavage of the modified RNA is given at the top; the single ³²P-labeled phosphate group is indicated with an asterisk. Samples were digested with RNase T₁, and half of each sample was also treated with iodoacetamide as indicated at the top of each lane. 3'-oxygen and 3'-sulfur products are indicated on the left and right of the gel, respectively. The 8-nucleotide product with a 3'-terminal thiol (lanes 7,9) runs faster than the same fragment with a 3'-terminal hydroxyl (lanes 3,4) because the sulfur is deprotonated under these electrophoresis conditions, adding an extra negative charge.

Treatment of the 3'-sulfur-substituted substrate with silver(I), which induces the specific hydrolysis of the sulfur-phosphorusbond of a 3'-S-phosphorothiolate linkage (Cosstick and Vyle 1990),gave rise to a product of the same size (Fig. 2A, lane 16), confirmingthe presence of the 3'-sulfur modification in the substrate andsuggesting that 5' splice site cleavage occurred accurately. Althoughthe 70-nucleotide exon 1 intermediates and the silver-cleavedproduct comigrated in this 5% polyacrylamide gel, it is possiblethat the resolution was not sufficient to detect very small sizedifferences (1-2 nucleotides). To confirm the accuracy of 5' splicesite cleavage of the modified substrate, unspliced precursor andthe purified products of silver cleavage and Mn²⁺-rescued self-splicing were digested with RNase T₁, which cleavesafter guanosine residues. Unmodified precursor and exon 1 intermediatewere digested in parallel for comparison. We also treated portionsof each sample with iodoacetamide (which reacts with thiols butnot hydroxyls) to test for the presence of the free 3'-thiol (Weinsteinet al. 1996). All samples were then subjected to electrophoresisin a 20% polyacrylamide gel, which provides sufficient resolutionto detect single-nucleotide and even single-functional-group differences.As shown in Figure 2B, the RNase T₁-digested products of silvercleavage (lane 7) and self-splicing (lane 9) comigrated precisely.Furthermore, both fragments reacted quantitatively with iodoacetamide,which decreased their mobilities by exactly the same extent (Fig.2B, cf. lanes 8 and 10). Iodoacetamide did not react with thefragments derived from unspliced precursors or unmodified exon1 intermediate (Fig. 2B, cf. lanes 1, 3, and 5 with lanes 2, 4,and 6, respectively), confirming the specificity of the modificationreaction. These results identify the cleavage site as the sulfur-phosphorusbond of the 3'-S-phosphorothiolate linkage. Similar analyses demonstratedthe accuracy of 5' splice site cleavage of the modified substratein the presence of Zn²⁺ and Cd²⁺ (data notshown).

To confirm that group II ribozyme activity was required for the observed cleavage in the presence of thiophilic metal ions,we took advantage of a trans reaction characterized by Pyle andcoworkers (Fig. 3, top panel). An RNA consisting of exon 1 andintron domains 1, 2, and 3 (ExD123) has no 5' splice site cleavageactivity on its own, but addition of a separate domain 5 RNA (D5)causes specific 5' splice site cleavage (Pyle and Green 1994).This reaction appears to be a faithful mimic of the first stepof self-splicing (Pyle and Green 1994; Peebles et al. 1995; Podaret al. 1995). We incorporated a 3'-S-phosphorothiolate linkageinto the 5' splice site of an ExD123 RNA and tested the abilityof saturating levels of D5 (Pyle and Green 1994) to catalyze thehydrolysis of the sulfur-phosphorus bond. 3'-S-Phosphorothiolatelinkages in RNA undergo base-catalyzed breakdown two to threeorders of magnitude faster than unmodified phosphodiesters, givingrise to cleavage products with 2'-O,3'-S-cyclic phosphorothiolateand 5'-hydroxyl termini (Liu and Reese 1996; Weinstein et al.1996). Therefore, the 70-nucleotide exon 1 resulting from eitherenzymatic hydrolysis or background cleavage differ only in thepresence or absence of a 3'-terminal cyclic phosphorothiolate,and cannot be resolved reliably by gel electrophoresis (data notshown). Because the enzymatic reaction is relatively slow (Pyleand Green 1994), the levels of background cleavage are prohibitivelyhigh to assay D5-catalyzed hydrolysis directly. Therefore, wetreated reaction mixtures with iodoacetamide and RNase T₁ to generatefragments that could be resolved from those derived from unreactedor background-cleaved molecules. This assay has the additionaladvantage of confirming the site of D5-catalyzed 5' splice sitehydrolysis with single-nucleotide accuracy. The reactions areshown in the lower panel of Figure 3. For the 3'-oxygen controlsubstrate, accurate D5-dependent hydrolysis was observed in 100mM MgCl₂ (Fig. 3, lane 3), and inclusion of 10 mM MnCl₂ (Fig.3, lane 5) or 10 mM CdCl₂ (Fig. 3, lane 7) did not impair thereaction. [10 mM ZnCl₂ is insoluble and causes RNA degradationunder the high-KCl conditions of this assay (Pyle and Green 1994), and therefore could not be tested.] Substitution of the 3'-oxygenleaving group with sulfur blocked the hydrolysis reaction whenMg²⁺ was the sole divalent metal ion present (Fig. 3, cf. lanes 3and 11). Inclusion of 10 mM MnCl₂ (Fig. 3, lane 13) or CdCl₂ (Fig.3, lane 15) relieved this negative effect. The Mn²⁺- and Cd²⁺-rescued reactions were D5-dependent (Fig. 3, lanes 12,14) andaccurate, as judged by the comigration with a silver-cleaved,iodoacetamide-modified standard (Fig. 3, lane 9). Therefore, ribozymeactivity is required for 5' splice site cleavage in the presenceof these thiophilic divalent metals.

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Figure 3. Domain 5 of the group II intron acts in trans to catalyze hydrolysis of the 3'-sulfur-substituted 5' splice site in a Mn²⁺- or Cd²⁺-dependent manner. The substrate (ExD123) and enzyme (D5) are diagrammed at the top (the single ³²P-labeled phosphate is denoted as *p). To resolve the product of accurate cleavage from that of background cleavage (see text), all reaction mixtures were treated with iodoacetamide, digested with RNase T₁, and subjected to electrophoresis (bottom) as in Fig. 2B. RNase T₁-digested background cleavage product was run off the bottom of the gel. (Lanes 1,8) Unreacted RNAs; (lane 9) a size standard generated by silver cleavage of the 3'-sulfur-containing substrate. Reactions contained 3 µM D5 RNA (lanes 3,5,7,11,13,15) and 100 mM MgCl₂, 90 mM MgCl₂/10 mM MnCl₂, or 90 mM MgCl₂/10 mM CdCl₂ as shown at the top of each lane. Parallel reactions in the absence of D5 RNA (lanes 2,4,6,10,12,14) were done as controls. 3'-Oxygen and 3'-sulfur products are indicated on the left and right of the gel, respectively.

Mg²⁺ supports the second reaction step of cis-splicing of a group II intron containing a 3'-sulfur substitution at the 3' splice site

To determine whether the second reaction step of self-splicing requires direct coordination of a metal ion to the 3'-oxygenleaving group, we synthesized a self-splicing construct with a3'-sulfur substitution (Fig. 1C) or a normal 3'-oxygen at the3' splice site, and tested them for cis-splicing activity in vitroin the presence of 0.5 M (NH₄)₂SO₄ and 100 mM divalent metal ion(Fig. 4A). Separate aliquots of the same reaction were subjectedto electrophoresis in 5% (Fig. 4A, top) and 20% (Fig. 4A, bottom)polyacrylamide gels. The latter was necessary to visualize thereleased 10-nucleotide exon 2, generated by the hydrolysis ofthe exon-exon junction of the spliced product (spliced exons reopening;see Fig. 1A). For the control substrate, no reaction occurredin the absence of divalent metals (Fig. 4A, lanes 4-7), but intron-exon2 intermediates (both linear and lariat), spliced product, andreleased exon 2 were all generated in the presence of 100 mM MgCl₂(Fig. 4A, lanes 8-11). For the 3'-sulfur-containing substrate,no reaction was observed in the absence of divalent metals (Fig.4A, lanes 19-22). In striking contrast to the results obtainedwith the 5' splice site, however, 100 mM MgCl₂ supported bothsteps of cis-splicing (Fig. 4A, lanes 23-26), as judged by theappearance of lariat intron-exon 2 intermediates, spliced product,and released exon 2. The addition of 10 mM MnCl₂ had no significanteffect on the reaction rate (data not shown). This asymmetry inthe response to 3'-sulfur substitution at the 5' and 3' splicesites is exactly what we observed in the spliceosome (Sontheimeret al. 1997). To diminish the unlikely possibility that the secondreaction step was supported by contaminating traces of thiophilicmetals, we carried out reactions with 110 mM MgCl₂ and 10 mM EDTA(Fig. 4A, lanes 12-15 and 27-30). Because EDTA chelates most thiophilicdivalent metal ions five to eight orders of magnitude more tightlythan it chelates Mg²⁺ (Anderegg 1987), its inclusion would be expected to abolish theability of trace contaminants to support the reaction. The addedEDTA, however, had no effect on the second reaction step withthe 3'-sulfur-substituted substrate (Fig. 4A, cf. lanes 23-26with lanes 27-30), arguing against this possibility. Treatmentof the 3'-sulfur-substituted substrate with silver(I) gave riseto the 10-nucleotide exon 2 fragment (Fig. 4A, lane 18), confirmingthe presence of the 3'-sulfur modification in the substrate. Althoughthe high salt present in the self-splicing reactions distortedthe electrophoretic mobilities of the exon 2 fragments (Fig. 4A,lanes 8-15, 23-30), they appeared to comigrate with the silver-cleavedexon 2, providing a preliminary indication that 3' splice sitecleavage occurred accurately.

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Figure 4. (A) Mg²⁺ supports 3' splice site cleavage and exon ligation of the 3'-sulfur-substituted substrate. Self-splicing reactions were performed with ligated 3'-end-labeled substrates containing a 3'-oxygen (lanes 1-15) or a 3'-sulfur (lanes 16-30) at the 3' splice site (see Fig. 1C). Separate aliquots of each sample were subjected to electrophoresis in a 5% polyacrylamide (top) or 20% polyacrylamide (bottom) denaturing gel. (Lanes 1,16) Unspliced RNAs; each substrate was also mock-reacted (lanes 2,17) or reacted (lanes 3,18) with silver(I). Self-splicing reactions were carried out for 1 hr and contained 10 mM EDTA (lanes 4-7, 19-22), 100 mM MgCl₂ (lanes 8-11, 23-26), or 10 mM EDTA mixed with 110 mM MgCl₂ (lanes 27-30). Samples were incubated for the times (in min) indicated at the top of each lane. Unspliced precursor (967 nucleotides), lariat and linear intron/exon 2 intermediates (897 nucleotides), spliced product (80 nucleotides), and released exon 2 (10 nucleotides) are indicated on the left. The sizes of the DNA markers (in nucleotides) are given on the right. The exon 1 intermediate and the excised intron products (lariat and linear) contain no radiolabel and are therefore not visible. (B) 3' Splice site cleavage of the 3'-sulfur-substituted substrate occurs accurately in the presence of Mg²⁺. The strategy for mapping the site of cleavage of the modified RNA is given at the top, and is similar to that described in Figure 2B. The single ³²P-labeled phosphate in the intron is denoted with an asterisk. Samples were digested with RNase T₁, and half of each sample was treated with iodoacetamide as indicated at the top of each lane. The products are described on the right; the A*pU_SH dinucleotide (lanes 3,5,7) and its acetamide-modified derivative (lanes 4,6,8) are indicated by dots.

To obtain further evidence for the accuracy of 3' splice site cleavage and exon ligation, we mapped the 3'-terminus of theexcised intron RNA directly. The mapping strategy (Fig. 4B, top)involved incorporation of a single ³²P-labeled phosphate adjacent to the 3' splice site, RNase T₁ digestion,iodoacetamide modification, and comparison with the identicallytreated product of silver cleavage. If the correct 3' splice sitewas used, then RNase T₁ digestion should yield the dinucleotideA*pU_SH as the only radiolabeled product, and this dinucleotideshould be modifiable with iodoacetamide. The data are shown atthe bottom of Figure 4B. Silver cleavage generated the A*pU_SHstandard (Fig. 4B, lane 3), which on reaction with iodoacetamideyielded the slower-migrating product A*pU_{SCH₂C(O)NH₂}. In the RNaseT₁ digestions of total RNA from self-splicing reactions in either100 mM MgCl₂ (Fig. 4B, lane 5) or 90 mM MgCl₂/10 mM MnCl₂ (Fig.4B, lane 7), the A*pU_SH dinucleotide is largely obscured by background;however, treatment with iodoacetamide clearly generates the identicalA*pU_{SCH₂C(O)NH₂} modified dinucleotide in both cases (Fig. 4B,lanes 6, 8). This product is absent from the RNA derived fromunspliced precursor (Fig. 4B, lane 2). We conclude that the sulfur-phosphorusbond of the 3' splice site 3'-S-phosphorothiolate linkage is cleavedduring self-splicing in the presence of Mg²⁺. Furthermore, the efficiency of accurate 3' splice site cleavageis not altered by the inclusion of the thiophilic metal Mn²⁺ (Fig. 4B, cf. lanes 6 and 8), providing further evidence againsta metal specificity switch during the second step of cis-splicing.

Isolation of the second step of self-splicing uncovers a metal specificity switch

As with the spliceosome (Sontheimer et al. 1997), the ability of Mg²⁺ alone to support exon ligation with the 3'-splice-site-substitutedsubstrate could indicate that inner-sphere coordination of theleaving group by a metal ion is not required for the reaction.An alternative possibility, however, is that 3'-sulfur substitutiondoes reduce the rate of the chemical step of exon ligation inthe presence of Mg²⁺ alone, but this effect is masked by a rate-limiting conformationalstep (Sontheimer et al. 1997). To distinguish between these possibilities,we assayed the exon ligation reaction in isolation. We took advantageof a recently developed tripartite reaction (A. Bar-Shalom andM. Moore, pers. comm.) in which a 3' splice site oligonucleotideis added separately to an exon 1 oligonucleotide and a ribozymecontaining all but the six 3'-terminal nucleotides of the intron(Fig. 5A). Unlike other group II exon ligation systems (Podaret al. 1998b; Deme et al. 1999), this reaction circumvents therequirement for the inefficient enzymatic ligation step in theconstruction of the 3'-splice-site-containing substrate. We synthesizedand 3'-end-labeled substrate oligonucleotides containing eithera 3'-oxygen or a 3'-sulfur at the scissile phosphate and testedthem in tripartite exon ligation reactions with an exon 1 oligonucleotidecontaining a 3'-terminal 2'-deoxycytidine (E1dC) (Fig. 5B). Althoughthese experiments were done with subsaturating levels of 3' splicesite oligonucleotide (i.e., k_cat/K_M conditions), the rate of thereaction was log-linear with pH (slope ~1 between pH 5.0 and 6.5),which is consistent with the possibility that the rate is sensitiveto the chemical step of the reaction (P.M. Gordon, E.J. Sontheimer,and J.A. Piccirilli, in prep.).

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Figure 5. (A) The tripartite step 2 reaction involves attack of an 18-nucleotide exon 1 RNA with a 3'-terminal 2'-deoxycytidine residue (E1dC) on a 13-nucleotide 3' splice site oligoribonucleotide, catalyzed by an ai5 $gamma$ ribozyme. The 3' splice site oligonucleotides contained either a 3'-oxygen or a 3'-sulfur at the scissile phosphate. The products are the 25-nucleotide spliced exons (labeled) and the 6-nucleotide intron fragment (unlabeled). (B) Isolation of the second step of group II self-splicing uncovers a metal specificity switch. Reactions with the 3'-oxygen (lanes 2-23) and 3'-sulfur (lanes 25-50) substrates are shown in the top and bottom panels, respectively. Reactions were incubated for the times (in min) given at the top of each lane. Parallel reactions in the absence of ribozyme (lanes 16,18,20,22,38-41,43,45,47,49) or the absence of E1dC (lanes 15,42) were done as controls. Reactions contained 10 mM EDTA (lanes 3-6, 26-29), 100 mM MgCl₂ (lanes 7-10, 15-17, 30-33, 43-44), 90 mM MgCl₂/10 mM MnCl₂ (lanes 11-14, 34-42), 90 mM MgCl₂/10 mM CdCl₂ (lanes 18,19,45,46), 90 mM MgCl₂/10 mM CoCl₂ (lanes 20,21,47,48), or 90 mM MgCl₂/10 mM ZnCl₂ (lanes 22,23,49,50).

For the 3'-oxygen control substrate, the reaction in the presence of 100 mM MgCl₂ yielded spliced product (Fig. 5B, lanes7-10) that comigrated with an independently synthesized and purifiedstandard (Fig. 5B, lane 1) under conditions where single-nucleotidedifferences are easily detected. The reaction is dependent onthe presence of divalent metal ions (Fig. 5B, lanes 3-6), E1dC(Fig. 5B, lane 15), and intron ribozyme (Fig. 5B, lane 16). Reactionalso occurred in the presence of 10 mM MnCl₂ (Fig. 5B, lanes 11-14),although the rate was reduced by approximately twofold. Inclusionof 10 mM CdCl₂ (Fig. 5B, lanes 18,19), CoCl₂ (Fig. 5B, lanes 20,21),or ZnCl₂ (Fig. 5B, lanes 22,23) also allowed efficient exon ligationin a ribozyme-dependent manner. For the 3'-sulfur-substitutedsubstrate, no reaction was observed in the absence of divalentmetal ions (Fig. 5B, lanes 26-29), ribozyme (Fig. 5B, lanes 38-41),or E1dC (Fig. 5B, lane 42). In the presence of all reaction components,however, the metal ion dependence was very different from thatobserved in the context of cis-splicing $---$ reaction in the presenceof MgCl₂ alone (Fig. 5B, lanes 30-33) resulted in a rate reductionof 100-fold relative to the 3'-oxygen substrate. Inclusion of10 mM MnCl₂ (Fig. 5B, lanes 34-37) restored the rate to withinthree- or fourfold of that of the 3'-oxygen substrate under thesame conditions (Fig. 5B, lanes 11-14). Furthermore, 10 mM CdCl₂(Fig. 5B, lanes 45,46) or CoCl₂ (Fig. 5B, lanes 47,48) also providedstrong ribozyme-dependent rate enhancements; 10 mM ZnCl₂ had onlya modest effect (Fig. 5B, lanes 49,50). Subsequent experimentswith saturating amounts of ribozyme showed a similar inhibitionin Mg²⁺ and rescue in Mn²⁺ (data not shown). Therefore, isolation of the second step ofself-splicing allowed us to detect a metal ion-leaving group interactionthat is obscured during canonical cis-splicing (Fig. 4A).

Reopening of spliced exons is blocked by 3'-sulfur substitution

Two metal ions have been proposed to catalyze phosphoryl transfer in each step of group II intron self-splicing: one thatfacilitates deprotonation and activation of the incoming 2'- or3'-hydroxyl nucleophile, and one that stabilizes the developingnegative charge on the oxyanion leaving group (Steitz and Steitz1993). Although we have provided strong evidence for the latterin both steps of splicing (see above), there is currently no evidenceregarding the former. Replacement of an oxygen nucleophile withsulfur is not optimal for the detection of metal-nucleophile interactionsbecause of sulfur's weak nucleophilicity at phosphate diesters(Dantzmann and Kiessling 1996; Pearson 1966). The principle ofmicroscopic reversibility (which states that forward and reversereactions must proceed through the same transition state) dictatesthat a metal specificity switch in the reverse reaction is evidencefor a metal ion-nucleophile interaction in the forward reaction.Because the SER hydrolytic reaction (Fig. 1A) is mechanisticallyanalogous to the reverse of the second step of splicing (Podaret al. 1995), 3'-sulfur substitution at the exon-exon junctionof the spliced product allows a direct test of the presence ofthe second metal ion postulated to exist in the group II intronsecond-step active site (Steitz and Steitz 1993).

We constructed 80-nucleotide spliced exons RNAs with a 3'-sulfur substitution or a normal 3'-oxygen at the exon-exon junction.In the presence of the linear intron ribozyme, MgCl₂ supportedmiscleavage at the two unmodified phosphodiester bonds flankingthe exon/exon junction, but no accurately cleaved exon 2 was detected(data not shown). Therefore, substitution of the 3'-oxygen leavinggroup with sulfur blocks the ability of Mg²⁺ to support the accurate SER reaction. We were unable to rescueaccurate exon-exon junction hydrolysis, however, despite testingmultiple concentrations of many different divalent metal ions(data not shown). Although the loss of activity in Mg²⁺ is consistent with the possibility of a direct metal ion interaction,sulfur differs from oxygen in other ways besides metal ion specificity.Accordingly, the absence of rescue by a thiophilic metal meanswe cannot confidently ascribe the inhibition to the disruptionof a metal ion-leaving group interaction, and the proposal fora metal ion-nucleophile interaction in the second step of groupII intron self-splicing (Steitz and Steitz 1993) remainstentative.

	Discussion

Top Abstract Introduction Results Discussion Materials and methods References

We have demonstrated that 3'-sulfur substitution at the 5' splice site causes a metal specificity switch for the first stepof group II intron self-splicing, and that this switch is alsoevident in a first-step intermolecular reaction. Furthermore,we have shown that 3'-sulfur substitution at the 3' splice sitehas no significant effect on the metal specificity of the secondstep of cis-splicing, as observed in the spliceosome (Sontheimeret al. 1997). When the second step is assayed in a tripartitereaction that bypasses the first step, however, a metal specificityswitch becomes evident. These results have significant implicationsfor the mechanism of group II intron self-splicing, and for thepossible relationship between group II introns and thespliceosome.

Metal ion catalysis by group II intron ribozymes

The inhibition of the first step of splicing in Mg²⁺ by 3'-sulfur substitution at the 5' splice site, and the ability of Mn²⁺, Zn²⁺, and Cd²⁺ to relieve this inhibition, provide very strong evidence fora metal ion-leaving group interaction that is essential for 5'splice site cleavage (Figs. 2 and 3). Although we have not determinedwhether this interaction occurs in the ground state or the transitionstate, the latter possibility is more likely (Fig. 6A). Becausethe bridging oxygen of a phosphoester linkage is electropositive(Bourne and Williams 1980), interaction with a divalent cationin the ground state is expected to be weak or even repulsive.This interaction should provide a stabilizing effect only whenthe leaving group develops negative charge during bond breakingin the transition state. This effect has been documented in agroup I intron ribozyme (Piccirilli et al. 1993; Narlikar et al.1995) and may be true for other catalysts that employ a divalentmetal for leaving group stabilization during phosphotransesterification.

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Figure 6. A catalytic metal ion is present in the active site of a group II intron during the first (A) and second (B) steps of self-splicing. The three reactive nucleotides in each step of self-splicing are shown bound to sites 1, 2, and 3 within the group II active sites, as proposed (Steitz and Steitz 1993

). Cataytic Mg²⁺ ions (inferred from this work) directly coordinate the 3'-oxyanion leaving groups (outlined) in the proposed transition states. In the second step (B), an additional catalytic metal ion may coordinate directly to the incoming 3'-oxyanion nucleophile, based on the inhibition of the SER reaction in Mg²⁺ following 3'-sulfur substitution (see text), but the inability to recoveractivity in the prsence of thiophilic divalent metal ions makes this proposal tentative. Adapted from Steitz and Steitz (1993)

It has been shown recently that Mn²⁺ has a marked stimulatory effect on the chemical step of a model reverse-branching reactionwith this ribozyme (Deme et al. 1999). Therefore, the rescue ofthe 3'-thio inhibition by Mn²⁺ could be attributable to a general stimulatory effect on thereaction rather than a specific rescue of the metal ion/leavinggroup interaction. However, 10 mM Cd²⁺ or Zn²⁺ (which also rescue the 3'-thio inhibition) do not stimulate therate of this model reaction (A. Nolte and A. Jacquier, pers. comm.).Furthermore, Mn²⁺ does not generally stimulate the rate of the D5-catalyzed 5'splice site hydrolysis (Deme et al. 1999), despite the fact thatit rescues the hydrolysis of the sulfur-substituted substrate(Fig. 3). We conclude that the relief of 3'-thio inhibition byMn²⁺, Zn²⁺, and Cd²⁺ is not attributable to a general stimulatory effect of thesemetals on the first chemical step of self-splicing.

Because ribozymes appear to be poorly suited for acid-base catalysis (for review, see Narlikar and Herschlag 1997), it hasbeen thought that they usually rely on divalent metal ions forefficient catalysis. The observation that the second step of self-splicingproceeds accurately in the presence of Mg²⁺ alone even after 3'-sulfur substitution at the 3' splice site(Fig. 4) was therefore surprising. The appearance of a metal specificityswitch on isolation of the second reaction step (Fig. 5), however,provides a rationale for this observation: a different step (presumablyconformational) that precedes 3' splice site cleavage and exonligation is likely to limit the rate of the overall reaction,obscuring the metal specificity switch in the subsequent (presumablychemical) phase of the reaction. An interaction ( $eta$ - $eta$ ') that intervenesbetween the two catalytic steps of splicing has been describedby Chanfreau and Jacquier (1996) and likely has a role in sucha conformational change. In the tripartite second-step reaction,a different step likely becomes rate-limiting, and the metal specificityswitch is revealed. This provides strong evidence for a metalion-leaving group interaction that is important for 3' splicesite cleavage (Fig. 6B). The observation that 3'-sulfur substitutionslows the rate of exon ligation at least 100-fold in Mg²⁺ without significantly changing the overall rate of cis-splicingsuggests that the conformational step that occurs during cis-splicingis at least 100-fold slower than the chemical step of exonligation.

The effects of Mn²⁺, Co²⁺, Zn²⁺, and Cd²⁺ were tested on both steps of splicing, and we found that different metal ions rescue cleavageof the 5' and 3' modified substrates to different extents. AlthoughMn²⁺ and Cd²⁺ relieve the inhibition at both sites, Zn²⁺ rescues the 5' splice site far more efficiently than the 3' splicesite, and the reverse is true for Co²⁺, indicating that rescue may be conferred by distinct metal bindingsites with unique coordination environments. This would not beexpected if the sulfur substitution caused the recruitment ofthiophilic metals from solution, leading to non-native cleavageactivity.

The possibility that the group II second-step active site contains a second metal ion that activates the 3'-hydroxyl nucleophile(Steitz and Steitz 1993; Fig. 6B) remains viable, given the stronginhibition of the SER reaction by 3'-sulfur substitution at theexon-exon junction. The inability of thiophilic metals to rescueactivity, however, means that the inhibition cannot yet be attributedto the loss of metal ion-leaving group coordination (Fig. 6B).The inability to rescue this inhibitory effect raises questionsabout the commonality of the active sites for the two steps ofsplicing. The original two-metal-ion model (Steitz and Steitz1993) depicted the two steps of group II self-splicing as forwardand reverse reactions in a single active site, as in group I introns.The effects of chiral phosphorothioates at the splice sites callthis model into question (Padgett et al. 1994) and indicate thatthe two reaction steps are mechanistically distinguishable (Podaret al. 1998b). In the original model (Steitz and Steitz 1993),the same metal ion interacts with the leaving group in the firststep and the nucleophile in the second step. Our experiments documentthat Mn²⁺, Zn²⁺, and Cd²⁺ can serve the first-step function in the context of a 3'-sulfursubstitution (Figs. 2 and 3) but cannot serve the second-stepfunction. Therefore, if a single metal ion serves both functions,the ligand environment that positions this metal ion is likelyto be different for the two steps. Alternatively, there couldbe a single active site that carries out the two steps as parallelrather than reverse reactions; that is, the same metal ion stabilizesthe leaving group in both steps. Although a metal ion-leavinggroup interaction is important for both steps (Fig. 6), differentmetals rescue each step to different extents (Figs. 2 and 5),again arguing for nonidentical ligand environments in the first-stepand second-step active sites. Detailed thermodynamic and structuralanalysis of metal ion function will be required to settle thisissue definitively, and the results described herein provide astarting point for theseanalyses.

Parallels with the spliceosome

The results with a group II intron have a very significant effect on how we view the results obtained previously with thespliceosome (Sontheimer et al. 1997). The identical asymmetricresponses of splice site 3'-sulfur substitution during cis-splicingin the spliceosome and group II introns $---$ a clear metal specificityswitch during the first reaction step, and no apparent metal specificityswitch in the second reaction step $---$ is striking, and provides afundamental parallel in the actual chemical mechanisms of thesetwo systems. Furthermore, it is unnecessary to invoke a proteincatalyst to explain the lack of a metal specificity switch inthe second step of nuclear pre-mRNA splicing, because the sameeffect has now been observed in a true ribozyme that catalyzesthe same chemistry. Two explanations for the asymmetric effectwere noted for the spliceosome: either a rate-limiting conformationalstep masks a metal specificity switch during 3' splice site cleavageand exon ligation, or there is no essential metal ion-leavinggroup interaction during the reaction (Sontheimer et al. 1997).Initially, both explanations were possible for the group II effectsas well. We were able to distinguish between the two possibleexplanations by examining exon ligation in isolation, and we uncovereda metal specificity switch (Fig. 5). The lack of any effect (stimulatoryor inhibitory) of 3'-sulfur substitution at the 3' splice siteduring nuclear pre-mRNA splicing (Sontheimer et al. 1997) stronglysuggests that it too is limited by a conformational change. Becauseit is clear that conformational rearrangements intervene betweenthe two steps of pre-mRNA splicing (Umen and Guthrie 1995), itwill now be important to determine whether a switch can be uncoveredfor the second step in thespliceosome.

It has been argued that in general, catalytic mechanisms will be among the features of enzymes that are most tightly constrainedfrom drifting during evolution (Benner and Ellington 1988). Therefore,it is significant for the debate over a common molecular ancestry,and therefore intron antiquity, that we observe mechanistic parallelsbetween the two systems. Other biochemical similarities continueto accumulate. In addition to the identical reaction pathways,stereochemical requirements, and 3'-S-phosphorothiolate effectson cis-splicing noted above, similar asymmetric responses to 2'-deoxynucleosidesubstitution at the splice sites have also been observed in bothsystems (Moore and Sharp 1992; Griffin et al. 1995; Podar et al.1998b; A. Bar-Shalom and M. Moore, pers. comm.; E.J. Sontheimeret al., unpubl.). Although it is possible that the parallels betweengroup II introns and the spliceosome could have arisen by convergentevolution from two independent lineages, as in mammalian and bacterialserine proteases (Fersht 1985), an increasingly large number ofcoincidences would have to be invoked to explain the cumulativesimilarities in reaction pathways, secondary structural motifs,and now catalyticmechanisms.

	Materials and methods

Top Abstract Introduction Results Discussion Materials and methods References

Plasmids and transcription

All constructs were based on the ai5 $gamma$ group II intron and flanking exons from the mitochondrial COX1 gene from S. cerevisiae.Linear intron ribozyme (D1-6) was transcribed from EcoRV-digestedpKC.D1-6 (a gift from K. Chin and A. Pyle, Columbia University,New York, NY), and domain 5 RNA was transcribed from HpaII-digestedpJDI5'-75 (Jarrell et al. 1988). All constructs for RNA ligationreactions (except for G2.5+10D123 and pG2.1-881/FokI; see below)were derivatives of the pJD20 plasmid (Jarrell et al. 1988). Thefollowing plasmids were constructed, which when linearized andtranscribed with T7 RNA polymerase generate RNAs as indicated:pG2.5+10D1-6Ex (HincII; starting 10 nucleotides downstream ofthe 5' splice site and ending 60 nucleotides downstream of the3' splice site), pG2.3-2ExLD1-6 (NlaIV; starting 293 nucleotidesupstream of the 5' splice site and ending with the second nucleotideupstream of the 3' splice site), pG2.3-2ExSD1-6 (NlaIV; starting70 nucleotides upstream of the 5' splice site and ending withthe second nucleotide upstream of the 3' splice site), and pG2.3-3D1-6(HaeIII; starting with the first intron nucleotide and endingwith the third nucleotide upstream of the 3' splice site). pG2.5+10D123was derived from the pJDI3'-673 plasmid (Jarrell et al. 1988);HindIII digestion and T7 transcription generates an RNA starting10 nucleotides downstream of the 5' splice site and ending 673nucleotides downstream of the 5' splice site, plus an additional37 nucleotides of 3'-terminal polylinker sequence. All of theseplasmids except pG2.3-2ExLD1-6 were made by PCR amplification.PCR products were cloned into pCR2.1 (Invitrogen), sequenced intheir entirety, and subcloned into pSP64 poly(A) (Promega). pG2.3-2ExLD1-6was made by subcloning a fragment of pG2.3-2ExSD1-6 into pJD20.To generate linear intron ribozyme (D1-6/1-881) containing allbut the six 3'-terminal nucleotides of the intron, we made pG2.1-881/FokIby cloning annealed synthetic oligonucleotides into the 3' splicesite of pG2.3-3D1-6; digestion with FokI and transcription withT7 RNA polymerase generates the ribozyme. Finally, 5-3ExS RNA(68 nucleotides), starting 70 nucleotides upstream of the 5' splicesite and ending with the third nucleotide upstream of the 5' splicesite, was transcribed directly from annealed synthetic oligonucleotidesincorporating a T7 promoter. Transcription of the 5+10D123 and5+10D1-6Ex RNAs were done in 100-µl reactions (37°C, 3-5 hr) containing40 mM Tris-HCl (pH 8.0), 2 mM each NTP, 10 mM GMP, 10 mM DTT,20 mM MgCl₂, 2 mM spermidine, 0.6 U/µl RNase inhibitor (Promega),40 ng/µl linearized plasmid DNA, and 0.16 µg/µl T7 RNA polymerase.The fivefold excess of GMP over GTP was included to generate RNAswith a 5'-monophosphate to serve as substrates in the ligationreactions.

Oligonucleotide synthesis

All oligoribonucleotides were synthesized on a Millipore solid-phase DNA/RNA synthesizer. Coupling of unmodified RNA phosphoramidites(Glen Research) followed standard protocols; 3'-S-phosphoramiditeswere synthesized and coupled as described by Sun et al. (1997).All oligoribonucleotides were deprotected following standard techniquesand purified by anion exchange HPLC, except for G2.18/6, whichwas purified by denaturing polyacrylamide gel electrophoresis.The following oligoribonucleotides were used in this study (subscript_S refers to a 3'-S-phosphorothiolate linkage and d refers to a2'-deoxynucleoside): G2.5R (5'-UCGAGCGGUCU-3'), G2.5S (5'-UC_SGAGCGGUCU-3'),G2.3R (5'-UACUAUGUAU-3'), G2.3S (5'-U_SACUAUGUAU-3'), G2.SER (5'-UCACUAUGUAU-3'),G2.SES (5'-UC_SACUAUGUAU-3'), G2.3RTP (5'-CGGGAUACUAUG-3'), G2.3STP(5'-CGGGAU_SACUAUG-3'), E1dC (5'-ACGUGGUGGGACAUUUU(dC)-3'), andG2.18/6 (5'- ACGUGGUGGGACAUUUU(dC)ACUAUG-3').

Construction of substrate RNAs

Full-length RNAs were generated by ligation of synthetic oligoribonucleotides to flanking RNAs, using a bridging oligonucleotideand T4 DNA ligase (Moore and Query 1988). The 5' splice site bridgingoligonucleotide was complementary to the last 22 nucleotides ofexon 1 and the first 28 nucleotides of the intron, the 3' splicesite bridging oligonucleotide was complementary to the last 22nucleotides of the intron and the first 28 nucleotides of exon2, and the spliced exons bridging oligonucleotide was complementaryto the last 20 nucleotides of exon 1 and the first 10 nucleotidesof exon 2. For 5' splice site ligations, the 5'-³²P-phosphorylated G2.5R or G2.5S oligoribonucleotides, bridgingoligonucleotide, and 5-3ExS RNA were annealed and ligated as described(Query et al. 1994), and purified by denaturing polyacrylamidegel electrophoresis. The recovered 79-nucleotide RNA was thenligated to the 5+10D123 or 5+10D1-6Ex RNAs as described (Podaret al. 1995) and gel-purified. 3' splice site ligations were doneessentially as described (Podar et al. 1995), except that theG2.3R and G2.3S oligoribonucleotides were 3'-end-labeled with $alpha$ -³²P-labeled 3'-deoxyadenosine triphosphate (New England Nuclear)and yeast poly(A) polymerase (Amersham Pharmacia), and ligationreactions contained a `disrupter' oligonucleotide (3 µM) complementaryto domain 5 (nucleotides 813-848 of the intron). For RNase T₁mapping of the 3' splice site, the G2.3S oligoribonucleotide was5'-³²P-phosphorylated, and the 3'-end-labeling was omitted. For unknownreasons, yields of 3' splice site ligations were always very low(<1%) and often gave no detectable ligation products, despiteextensive efforts to optimize the reactions. For the SER assay,spliced exons were generated with G2.SER and G2.SES oligoribonucleotidesand 5-3ExS RNAs as described above for the 5' splice site ligations,except that the oligonucleotides were 3'-end-labeled with $alpha$ -³²P-labeled 3'-deoxyadenosine triphosphate and 5'-phosphorylatedwith nonradioactiveATP.

Ribozyme reactions

Cis-splicing assays containing trace radiolabeled substrate, 0.5 M (NH₄)₂SO₄, 40 mM MOPS (pH 7.5), and EDTA or metal ion chloridesas indicated in Figures 2 and 4 were preincubated and reactedat 42°C as described (Daniels et al. 1996). Domain 5-catalyzedhydrolysis reactions of ExD123 containing trace radiolabeled substrate,3 µM D5 RNA, 0.5 M KCl, 40 mM MOPS (pH 7.0), and metal ion chloridesas indicated in Figure 3 were preincubated and reacted for 2 hrat 45°C as described (Pyle and Green 1994). The reactions werethen treated with 40 mM iodoacetamide and 50 mM HEPES (pH 8.0)for 1 hr at room temperature, precipitated with ethanol, and digestedwith RNase T₁ as described below. Electrophoresis was as describedbelow for 5' splice site mapping, except that DTT and the longprerun were omitted. SER reactions containing trace radiolabeledsubstrate, 0.5 µM D1-6 RNA, 1.0 M KCl, 40 mM MOPS (pH 7.5), and100 mM MgCl₂ were preincubated and reacted at 45°C as described(Podar et al. 1995). Tripartite step 2 reactions containing trace3'-end-labeled G2.3RTP or G2.3STP substrate, 0.5 µM E1dC oligonucleotide,0.2 µM D1-6/1-881 RNA, 0.5 M (NH₄)₂SO₄, 40 mM MOPS (pH 7.5), andEDTA or metal ion chlorides as indicated in Figure 5 were doneat 42°C (A. Bar-Shalom and M.J. Moore, pers. comm.). Before reaction,all components except substrate and thiophilic metal ions werepreincubated at 75°C for 2 min and then at 42°C for 90 min. Allribozyme reactions containing EDTA, MgCl₂, and/or MnCl₂ were supplementedwith 10 mM DTT to avoid 3'-thiol oxidation; for reactions containingCoCl₂, ZnCl₂, or CdCl₂, tricarboxyethylphosphine (Strem Chemicals)was used instead to avoid precipitation of metal/DTT complexes.KCl, (NH₄)₂SO₄, and divalent metal ion chlorides (Aldrich) wereof the highest purity available (>99.99%).

Splice site mapping

For mapping the position of 5' splice site cleavage, substrates were subjected to cis-splicing in 90 mM MgCl₂ and 10 mM MnCl₂for 1 hr as described above. A separate 3'-sulfur-substitutedsample was cleaved with silver(I) as described (Sontheimer 1999).The exon 1 intermediates and Ag⁺-cleaved product were purified by electrophoresis in an 8% polyacrylamide:bis(19:1)/0.5× TBE/10 mM DTT gel. Half of each sample (as well asthe corresponding unspliced precursor) was kept frozen in 10 mMDTT, while the other half was treated with iodoacetamide/HEPESas described above. All samples were then digested to completionwith RNase T₁ as described (Sontheimer et al. 1997), and subjectedto electrophoresis in a 20% polyacrylamide:bis (29:1)/0.5× TBE/10mM DTT gel that had been prerun at low wattage (12 W) overnight.The bromophenol blue tracking dye (which runs just ahead of the8- to 9-nucleotide RNase T₁ fragments) was run to the bottom ofa 40-cmgel.

To map the position of 3' splice site cleavage, a 3'-sulfur-substituted substrate with a single ³²P label in the adjacent intron phosphate was prepared as describedabove. Samples were subjected to Ag⁺-cleavage or cis-splicing in 100 mM MgCl₂ or 90 mM MgCl₂/10 mMMnCl₂ for 1 hr as described above; half of each sample (as wellas unspliced precursor) was reacted with iodoacetamide, digestedwith RNase T₁, and subjected to electrophoresis as described abovefor 5' splice sitemapping.

	Acknowledgments

We thank Michelle Hamm and Cecilia Cortez for oligonucleotide synthesis; Barbara Golden, Manyuan Long, Nipam Patel, and ThomasTuschl for comments on the manuscript; and members of the Piccirillilaboratory for advice, discussions, and comments on the manuscript.We are grateful to Barbara Golden for T4 DNA ligase; Richard Padgettfor advice on ligation reactions; and Melissa Moore, Anna MariePyle, and Alain Jacquier for plasmids, discussions, and communicationof unpublished results. E.J.S. was supported in part as a researchassociate of the Howard Hughes Medical Institute. J.A.P. is anassistant investigator of the Howard Hughes MedicalInstitute.

The publication costs of this article were defrayed in part by payment of page charges. This article must therefore be herebymarked `advertisement' in accordance with 18 USC section 1734solely to indicate thisfact.

	Footnotes

Received April 13, 1999; revised version accepted May 21, 1999.

³ Present address: Department of Biochemistry, Molecular Biology and Cell Biology, Northwestern University, Evanston, Illinois60208-3500USA.

⁴ Corresponding author.
E-MAIL jpicciri{at}midway.uchicago.edu; FAX (773) 702-3611.

References

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Abstract
Introduction
Results
Discussion
Materials and methods
References

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RESEARCH PAPER Metal ion catalysis during group II intron self-splicing: parallels with the spliceosome

RESEARCH PAPER
Metal ion catalysis during group II intron self-splicing: parallels with the spliceosome