Uridylate Addition and RNA Ligation Contribute to the Specificity of Kinetoplastid Insertion RNA Editing

doi:10.1128/MCB.20.22.8447-8457.2000

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Molecular and Cellular Biology, November 2000, p. 8447-8457, Vol. 20, No. 22
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Uridylate Addition and RNA Ligation Contribute to the Specificity of Kinetoplastid Insertion RNA Editing

Robert P. Igo Jr., Setareh S. Palazzo, Moffett L. K. Burgess, Aswini K. Panigrahi, and Kenneth Stuart^*

Seattle Biomedical Research Institute, Seattle, Washington 98109

Received 10 May 2000/Returned for modification 21 June 2000/Accepted 24 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

RNA editing in Trypanosoma brucei inserts and deletes uridylates (U's) in mitochondrial pre-mRNAs under the direction of guideRNAs (gRNAs). We report here the development of a novel in vitroprecleaved editing assay and its use to study the gRNA specificityof the U addition and RNA ligation steps in insertion RNA editing.The 5' fragment of substrate RNA accumulated with the number ofadded U's specified by gRNA, and U addition products with morethan the specified number of U's were rare. U addition up to thenumber specified occurred in the absence of ligation, but accumulationof U addition products was slowed. The 5' fragments with the correctnumber of added U's were preferentially ligated, apparently byadenylylated RNA ligase since exogenously added ATP was not requiredand since ligation was eliminated by treatment with pyrophosphate.gRNA-specified U addition was apparent in the absence of ligationwhen the pre-mRNA immediately upstream of the editing site wassingle stranded and more so when it was base paired with gRNA.These results suggest that both the U addition and RNA ligationsteps contributed to the precision of RNAediting.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Kinetoplastid RNA editing is a form of mitochondrial (mt) mRNA maturation in which uridylate residues (U's) are inserted anddeleted (for recent reviews, see references 1, 26, 27).It is an essential step in the maturation of most mt RNAs in kinetoplastidprotozoa since it creates start and stop codons and determinesthe mature coding sequence, often accounting for more than halfof the sequence. The mature mRNA sequence is specified by smallguide RNAs (gRNAs), which contain sequences complementary to shortregions of edited mRNA, allowing G · U base pairs (6).

In vitro studies using mt extract from the kinetoplastid Trypanosoma brucei (8, 15, 25) indicate that RNA editing occursby a series of enzymatic reactions, including endonucleolyticcleavage, U addition or removal, and RNA ligation (6). Initially,gRNAs form an anchor duplex with the pre-mRNA immediately downstreamof the sequence to be edited. The pre-mRNA is cleaved at a pointupstream and adjacent to the anchor duplex, thus selecting theediting site (ES). This cleavage produces a 5' fragment with a3'-terminal hydroxyl and a 3' fragment with a 5' phosphate (20,25). The 5' cleavage fragment may be tethered to the 3' regionof the gRNA, and the gRNA in turn is stably associated to the3' fragment by the anchor duplex and also perhaps by associationwith one or more proteins. Tethering of the 5' fragment may involvethe 3' oligo(U) tail of gRNA, by interaction with purine-richsequences in the 5' fragment and/or by RNA-protein interactions.During insertion editing, one or more U's from free UTP are addedto the 3' end of the 5' cleavage fragment (15), while U's areremoved during deletion to generate free UMP (13). Finally,the processed 5' cleavage fragment is rejoined to the 3' fragmentextending the anchor duplex in the 5' direction and yielding RNAedited at one ES. Kinetoplastoid RNA editing is catalyzed by amultiprotein complex, called the editosome or editing complex,that contains the RNA endonuclease, terminal uridylyl transferase(TUTase), 3' U-specific exonuclease, and RNA ligase activitiesthat catalyze the steps of editing (2, 10, 21, 22).

The insertion of U's appears to be directed by the guiding A's and, less often, G's, in gRNAs (6). However, how the numberof U's inserted is specified by gRNAs is unknown. We exploredwhich step(s) during U insertion editing determines the numberof inserted U's. The cleavage step determines the site selectedfor editing, but it cannot directly specify the number of U'sthat are inserted. Hence, the precision in the number of U's thatare inserted is likely to arise during the steps subsequent tocleavage $---$ the U addition and RNA ligation steps. We developed anovel in vitro precleaved insertion editing assay that allowsseparate assessment of the U addition and ligation steps. Thisassay, which is an extension of an earlier in vitro assay (15),presents the pre-mRNA as two separate molecules that correspondto the 5' and 3' cleavage fragments. Using this system we havecharacterized the roles of U addition and RNA ligation in determiningthe number of U's added at the ES during insertionediting.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Preparation of RNAs. All RNAs used in this study were prepared by T7 polymerase (Promega) transcription of PCR-generated templates, except forthe 3' fragments 3'CL13pp and 3'CL3'p, which were purchased asRNA oligonucleotides from Oligos, Etc. Since T7 polymerase generatesRNA transcripts with heterogeneous 3' ends (19), the total lengthand the identity of the 3'-terminal G of 5'CL18 were verifiedby RNase T₁ digestion of the T4 ligation product of 5'CL18 and3'CL13pp. The presence of the 3' phosphate on 3'CL13pp was verifiedby the inability to ligate [5'-³²P]pCp to the 3' end of this molecule using T4 ligase and usingthe same oligonucleotide lacking the 3' phosphate as acontrol.

Template DNA for transcription was prepared by PCR from oligonucleotide pair templates. The transcription template for 5'CL18,the 5' fragment used in these experiments, was prepared by PCRof 5'CL18-Tmp1 (5'-GGCGGAATTCTGTAATACGACTCACTATAGGAAGTATGAGACGTAGG-3'and complementary sequence) using primers EcoRI T7 (5'-CGGCGGAATTCTGTAATACGACTCACTATAG-3')and 5'CL18-3' (5'-CCTACGTCTCATACTTCCTATAG-3'). Transcription templatesfor gRNAs gPCA6-0A, -1A, -2A, -3A, -4A, and -5A were preparedby PCR of gPCA6-3A-Tmp1 (5'-CGGCGGAATTCTGTAATACGACTCACTATAGGATATACTATAACTCCGATAAACCTACGTCTCATACTTCC-3'and complementary sequence) with primers EcoRI T7 and gPCA6-0A-3',-1A-3', -2A-3', -3A-3', -4A3', and -5A3', respectively (5'-GGAAGTATGAGACGTAGG[T]_nATCGGAGT-3',where n equals the number of guiding A residues indicated in thename of the gRNA). Transcription templates for A6AC and A6AC5'CLwere prepared by PCR of DNA encoding the pre-mRNA A6e-ES1 (15)with primers A6 Shorter (5'-GTAATACGACTCACTATAGGAAAGGTTAGGG-3'),containing the T7 promoter, and A6AC-3' (5'-CTATAACTCCAATCAGTACTTTC-3')and A6AC5'CL-3' (5'-CAGTACTTTCCCTTTCTTCT-3'), respectively. Transcriptiontemplates for gA6[14]USD-1A, -2A, and -3A were prepared by PCRof plasmid pgA6[14]wt (15) with primers EcoRI T7 and gUSD-1A3',-2A3', and -3A3', respectively (5'-AAAGAAAGGGAAAACTTCG[T]_nATTGGAGTTATAG-3').Radiolabeling of RNA at the 5' terminus was performed either bycapping, using [ $alpha$ -³²P]GTP (DuPont NEN) and guanylyltransferase (Gibco-BRL), or byphosphorylation of alkaline-phosphatase-treated RNA with T4 polynucleotidekinase (Gibco-BRL) in the presence of [ $gamma$ -³²P]ATP (DuPont NEN). Radiolabeling at the 3' terminus was performedby ligation of [5'-³²P]pCp (27). For RNA sequencing, a 10× preparative reaction wasperformed, and relevant RNA species were excised from the gel,eluted in 0.3 M NaOAc (pH 5.2)-0.1% sodium dodecyl sulfate (SDS)-1mM EDTA, and precipitated. RNAs were sequenced using the Pharmaciaenzymatic RNA sequencingkit.

Preparation of mt extract. Mitochondria were isolated from procyclic T. brucei brucei strain IsTat 1.7a as previously described (14). Editing complexeswere enriched from a 0.5% Triton X-100 mt lysate (21) by sequentialSP Sepharose cation-exchange and Q Sepharose anion-exchange chromatography(A. K. Panigrahi et al., submitted for publication). Cleared mtlysate was bound to a 1-ml SP Sepharose column (Bio-Rad) in SPSepharose buffer A (10 mM Tris HCl [pH 7.0], 10 mM MgCl₂, 50 mMKCl, 1 mM dithiothreitol [DTT]), and fractions were eluted bya linear step gradient from 50 to 1,000 mM KCl. Fractions correspondingto 150 to 300 mM KCl were pooled and equilibrated to pH 8.3. Proteinsin the pooled fractions were bound to a 1-ml Q Sepharose columnin Q Sepharose buffer A (same as SP buffer A with 10 mM Tris [pH8.3] replacing Tris-HCl [pH 7.0]) and eluted by another 50 to1,000 mM KCl linear step gradient. Insertion-editing activityelutes from the Q Sepharose column at approximately 200 mM KCl(Panigrahi et al., submitted for publication). The fold purificationof precleaved insertion-editing activity varied among preparations,but it was generally about 100-fold greater than in cleared mtlysate (Panigrahi et al., submitted for publication; R. P. Igo,Jr., unpublishedresults).

Assays for insertion editing of precleaved and uncleaved pre-mRNAs. Editing reactions were performed in a total volume of 30 µl in a final concentration of 25 mM HEPES (pH 7.9)-10 mM Mg(OAc)₂-5mM CaCl₂-50 mM KCl-0.5 mM DTT-1 mM EDTA. UTP was also presentat 100 µM unless otherwise indicated. Editing reactions contained50 fmol of labeled 5' fragment, 0.5 pmol of gRNA, and 1 pmol of3' fragment. Substrate RNAs and gRNA were annealed prior to thereaction by incubation at 65°C for 2 min and then at room temperaturefor 15 min. Editing reactions were stopped by addition of 2 µlof 260 mM EDTA-2.5% SDS. Ligation during editing assays was preventedby addition of 4 mM pyrophosphate to the reaction mix 15 min priorto the addition of the RNAs or by use of a 3' fragment with no5' phosphate, 3'CL3'p. To prevent interactions between labeledproducts and gRNA during electrophoresis, 25 pmol of nonradioactiveA6PC (ligation product of 5'CL18 and 3'CL13) competitor RNA wasadded. After phenol-chloroform extraction and precipitation, theRNA was resuspended in 7 M urea-1× Tris-borate-EDTA containing0.05% bromophenol blue and 0.05% xylene cyanol dyes, incubatedat 100°C for 2 min, and immediately loaded on 18% (wt/vol) denaturingpolyacrylamide gels. Reaction products were visualized on a StormPhosphorImager (Molecular Dynamics). Quantification was performedusing ImageQuaNTsoftware.

Insertion editing of the intact (uncleaved) A6AC pre-mRNA was assayed in reactions containing 0.25 pmol of pre-mRNA and 0.5pmol of gRNA, under the same reaction conditions as for the precleavedassay, except that ATP was added to a final concentration of 10µM. Ligation activity during a full round of insertion editingwas prevented by the presence of 0.4 mM pyrophosphate. Productsof editing of uncleaved or precleaved A6AC RNA were separatedon 9% (wt/vol) polyacrylamidegels.

Ligation reactions. Assays for RNA ligation activity were performed in the same manner as editing assays, except that UTP was omitted from thereactions. T4 ligation reactions, used as an RNA size standard,contained the same quantities of 5'CL18, 3'CL13pp, and gPCA6-2Aas in the insertion-editing reactions, plus 8 U of T4 RNA ligase(Gibco-BRL). These reactions were in a total volume of 10 µl ofT4 ligase buffer (25 mM HEPES [pH 8.3], 5 mM MgCl₂, 25 µM ATP,1.6 mM DTT, 15% glycerol, 10% dimethyl sulfoxide) and were incubated3 h at 4°C before phenol-chloroform extraction and RNAprecipitation.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Editing of precleaved RNA. The ability of preedited RNA that is presented as separate 5' and 3' fragments (Fig. 1) to be accurately edited in vitro wastested, since this would be useful for studies of the individualenzymatic steps of editing. The two fragments were designed tomimic the pre-mRNA cleavage products that result from the editing-associatedendonuclease, and thus we refer to this as the precleaved editingassay. The fragments were based on the A6 pre-mRNA that was usedto develop the in vitro editing system (15). The sequence ofthe 3' fragment, 3'CL13pp, matches that of A6 pre-mRNA editedat ES1 (A6-eES1). It has a 5' monophosphate like the 3' cleavagefragment that is produced during editing (15, 23, 25), buta 3' phosphate was added to prevent U addition to the 3' terminusby TUTase activity during in vitro incubation. The sequence ofthe 5' fragment, 5'CL18, has the same nucleotide composition butnot the same sequence as the upstream region of pre-A6 mRNA; itis shorter than the 5' fragment produced by cleavage of A6-eES1(15) in order to maximize resolution of the products of editingon polyacrylamide gels. The sequences of the 5' region of gPCA6gRNAs match that of gA6[14] and thus can form the same anchorduplex with the 3' fragment as in the native RNAs.

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FIG. 1. (A) Structure of the precleaved insertion-editing substrate RNAs aligned with gRNA. The 5' cleavage fragment 5'CL18 and 3' cleavage fragment 3'CL13pp are shown aligned with gRNA gPCA6-2A, which directs insertion of two U's at the ES. The asterisk denotes a ³²P-labeled monophosphate or [ $alpha$ -³²P]GTP cap. The ES is marked by an arrow, and guiding nucleotides are underlined in lowercase. 5'CL18 contains a 3' hydroxyl group. 3'CL13pp contains a 5' and 3' monophosphate; the latter prevents U addition to the 3' end of 3'CL13pp by TUTase activity. (B) Structure of A6AC pre-mRNA aligned with gRNA gA6[14]USD-2A. ES2 is indicated by an arrow, and guiding nucleotides are in lowercase. The potential base pair upstream of ES2 is indicated by a dashed line. The sequence of A6AC differs from that of pre-A6 mRNA edited at ES1 (4) in that a GU sequence 4 nt upstream of ES2 was replaced by AC. The information region of gA6[14] (17) was truncated and replaced with an oligopyrimidine sequence complementary to part of the upstream purine-rich region of A6AC.

Incubation of the 5' and 3' fragments with gRNA and mt extract containing active editing complexes under conditions that supportin vitro insertion editing of pre-A6 mRNA (Fig. 2) resulted inedited RNA and products with added U's (U addition products) (Fig.3A and B). The species marked U1, U2, and U3 in Fig. 3A representthe products of U addition to the 3' end of the 5' fragment, sincethey were generated in the presence but not the absence of UTPand were generated when the 5' end of 5'CL18 was blocked by GTPcapping (Fig. 3B, lanes 1 and 7; data not shown). In addition,no U's were added during this reaction to a 3'CL13 RNA labeledat its 3' end with [5'-³²P]pCp, showing that the 3' phosphate of 3'CL13pp was not removed.Products marked E1, E2, and E3 in Fig. 3A had the correct mobilityfor edited RNA containing 1, 2, and 3 U's inserted at the ES,respectively. The identity of these edited products was confirmedby RNA sequencing (data not shown). The accurately edited product,containing the number of U's specified by the number of guidingA's in gRNA, represented more than 90% of the total ligation productsof editing reactions containing a gRNA with 1, 2, or 3 guidingA's. Thus, the separate 5' and 3' fragments were accurately editedin a gRNA-directed fashion. Of the U addition products, thosewith the number of added U's specified by their respective gRNAsaccumulated to the highest level. Addition products with fewerU's than specified by gRNA were also observed but were substantiallyless abundant. No addition products with more U's than specifiedby the gRNA were observed. Thus, there was preferential accumulationof addition products with the number of U's specified by the gRNA.

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FIG. 2. Insertion editing activity of T. brucei mt extract partially purified by SP and Q Sepharose chromatography. A6AC RNA was 3' end labeled and incubated with gA6[14]USD-1A (A), -2A (AA), or -3A (AAA) in insertion-editing assays as described in Materials and Methods, and the reaction products were separated on a 9% (wt/vol) polyacrylamide gel along with a partial alkaline hydrolysis ladder (right lane). An arrow indicates the input RNA, and E1, E2, and E3 indicate edited products containing one, two, and three inserted U's, respectively. The one-U insertion product is incompletely resolved from the input.

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FIG. 3. Accurate, gRNA-directed insertion editing of precleaved RNA substrates. Editing reactions, assembled as described in Materials and Methods and with variations as described below, were incubated 3 h at 28°C. The RNA products were separated in an 18% denaturing polyacrylamide gel. The input 5'CL18 is indicated by an arrow. Products with one, two, or three added U's are indicated as U1, U2, or U3, respectively. L indicates ligated 5'CL18 and 3'CL13pp. Edited RNA with one, two, or three U's inserted at the ES are indicated as E1, E2, or E3, respectively. Lanes labeled T4 contain T4 ligase reactions with 5'CL18 and 3'CL13pp, as a size standard. (A) Products of precleaved editing reactions containing gPCA6-1A (A), gPCA6-2A (AA), and gPCA6-3A (AAA) (see Materials and Methods). (B) gRNA and substrate RNA requirements for precleaved editing. Conditions were as follows: lane 1, 5'CL18 RNA and UTP omitted; lane 2, 5'CL18 only; lane 3, 5'CL18 and 3'CL13pp RNAs and gRNA omitted; lane 4, 5'CL18 and gPCA6-2A RNAs and 3' fragment omitted; lane 5, complete reaction with 5'CL18, 3'CL13pp, and gPCA6-2A RNAs (same as lane AA in panel A; see Materials and Methods); lane 6, complete reaction with 0.3 mM ATP; lane 7, complete reaction with UTP omitted; lane 8, complete reaction with mt extract omitted. Lane 10, partial alkaline hydrolysis ladder of A6 pre-mRNA, as a size standard. (C) Products of precleaved editing of A6AC pre-mRNA. Reactions were performed omitting mt extract, gRNA, or UTP, and complete reaction mixtures contained gA6[14]USD-1A (A), -2A (AA), and -3A (AAA). Reaction products are labeled as in panels A and B. Alk, partial alkaline hydrolysis ladder.

As expected, neither edited RNA nor the addition products were generated in the absence of UTP or mt extract containing activeediting complexes (Fig. 3B, lanes 1, 7, and 8). Little +2-U additionproduct was produced when the 3' fragment was omitted; indeed,the +1-U product was more abundant than the +2-U product (Fig.3B, lane 4). Omission of the gRNA resulted in major products with1 to 4 added U's, in descending order of abundance, plus a lessabundant population of products with 10 to 40 added U's (Fig.3B, lanes 2 and 3). It cannot be resolved from these data whetherthe products with few U's result from the simple addition of afew U's or the addition of many U's followed by the removal ofmost of them by U-specific exonuclease (18). None of these productswas due to ligation with the 3' fragment, since the products appearedin the absence of this fragment (lane 2), nor were they the resultof circularization, since they appeared when the 5' fragment wasGTP capped (data not shown). The nucleotide addition activitywas highly specific for U; addition of G's or A's was barely detectableeven at 5 mM GTP or ATP, and addition of C's occurred with muchlower efficiency than addition of U's (R. P. Igo, Jr., et al.,unpublished data). Thus, accurate U insertion required all threeRNA components, UTP, and mt extract containing active editingcomplexes.

Insertion editing of the A6AC pre-mRNA precleaved at ES2 (Fig. 1B) was also examined. U addition to the 5' fragment of A6ACin the absence of gRNA yielded a very abundant product with oneadded U and much less abundant products with more than one addedU. The preponderance of the +1-U-addition product remained inthe presence of a gA6[14]USD gRNA containing 1, 2, or 3 guidingA residues. Some of this +1-U product was ligated in the presenceof a gRNA with 2 or 3 guiding A residues. Nevertheless, the mostprominent ligated product contained the number of U's specifiedby gRNA, as did the most prominent nonligated product besidesthe +1-U product. Thus, although U addition to precleaved A6ACwas less gRNA specific than to a smaller substrate (Fig. 3A),it still appeared to be responsive to the gRNAsequence.

Insertion editing of precleaved A6-eES1 RNA was extremely inefficient and not always detectable, when directed by wild-typegA6[14] gRNA (15; data not shown). However, substantial editedRNA was generated when a stable Watson-Crick duplex between thegRNA and the 5' fragment was allowed (Fig. 2). Edited RNA wasalso produced in the presence of gA6[14]COMP gRNA, in which theU tail of gA6[14] is replaced by a sequence which can form sucha duplex (8), and in the presence of a 5' fragment with basesubstitutions that allowed a duplex with the gRNA immediatelyupstream of the ES (data not shown). Editing of A6-eES1 RNA bythe complete insertion reaction was also very inefficient in thepresence of gA6[14], but it was 14-fold more efficient when theU tail of this gRNA was replaced by a sequence that was complementaryto the 5' fragment (data not shown). Thus, the ability to forma stable upstream duplex enhanced the ability of the RNA to beedited.

Under some conditions, ligation products of 5'CL18 and 3'CL13pp other than the accurately edited RNAs were observed. A smallamount of the simple ligation product of 5'CL18 and 3'CL13pp withno inserted U's, designated L, was generated when UTP was omittedfrom the reaction (Fig. 3B, lane 7). However, a substantial amountof this ligation product was generated when 0.3 mM ATP was added,even in the presence of UTP (Fig. 3B, lane 6). The identity ofthis ligation product was confirmed by RNA sequencing (data notshown). In the absence of added ATP, the production of editedRNA with the sequence specified by the gRNA (Fig. 3B, lane 5)presumably reflected the activity of adenylylated (charged) ligasein the editing complex (see below). Charged ligase could alsogenerate the very low level of ligated RNA (L) in the absenceof UTP (Fig. 3B, lane 7). Thus, the inclusion of ATP appearedto have primarily stimulated nonspecific ligation, i.e., ligationof 5' fragments without the number of added U's specified by thegRNA. The specific ligation activity was especially evident inthe SP Sepharose-Q Sepharose fraction (see Materials and Methods).The active editing fractions from glycerol gradients and fromSuperdex-200 gel filtration chromatography had very low editingactivity in the absence of added ATP, but the addition of ATPstimulated both accurate editing and nonspecific ligation (R.P. Igo, Jr., et al., unpublished results). The stimulation ofnonspecific ligation in the presence of ATP may also have accountedfor the production of a small amount of edited RNA with one insertedU, rather than the two specified by the gRNA (Fig. 3B, lane 6).While the efficiency of editing, as a percentage of total input,was similar when ATP was either present or absent, a prominentnonligated +2-U-addition product was not observed when ATP wasincluded, suggesting that all of the available +2-U product wasincorporated into edited RNA (Fig. 3B, compare lane 6 with lane5). Overall these results suggested that RNA with the number ofU's specified by the gRNA was preferentially ligated in the absenceof ATP, presumably by charged ligase in the editingcomplex.

Time course of precleaved insertion editing. The accumulation kinetics of the products of precleaved editing provided information on gRNA specificity. Using gRNAs specifyinginsertion of 1, 2, or 3 U's, the 5' fragments with added U's appearedand accumulated early in the reaction and then reached or nearlyreached a steady-state level within 1 h (Fig. 4). This paralleledthe kinetics of accumulation of U addition products in an assayin which the pre-mRNA is cleaved by the editing complex (15).The edited RNA appeared after the 5' fragments with added U'sand continued to accumulate over the entire 3-h course of theincubation. Thus, the order of appearance and accumulation ofU addition and ligation products closely resembled that of substratesthat are cleaved during a full round of in vitro editing (15,25). Accumulation of edited RNA continued at a gradually slowingrate for 16 h, although significant degradation of the input RNAoccurred after 3 h (data not shown). Importantly, the nonligatedproduct with the number of added U's specified by the gRNA accumulatedto a higher level than did those products with fewer added U's.Furthermore, the products with fewer U's accumulated before thosewith more added U's and more quickly reached a steady-state level,suggesting stepwise U addition. These experiments further supportedthe hypothesis that the gRNA sequence determines the number ofU's that are added during this step of editing, although U removalmay also contribute to the preferential accumulation of the gRNA-specifiedproduct by removing U's added beyond the specified number.

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FIG. 4. Time course of precleaved insertion. Precleaved editing reactions, with gPCA6-1A (A), gPCA6-2A (B), or gPCA6-3A (C), were incubated for various time periods at 28°C before adding stop buffer. Panels at right show denaturing polyacrylamide gels of the reaction products. U addition products and edited RNA are labeled as in Fig. 2. Graphs at left show the accumulation of products over time. Accurately edited RNAs are depicted by filled symbols and solid lines, while U addition products are depicted by open symbols and dashed or dotted lines (see legends of graphs).

The relative abundance of the products with added U's reflected the rate of ligation of each product. For each gRNA tested,the 5' fragment with the number of added U's specified by thegRNA became most abundant, and the edited RNA which resulted fromthe ligation of that fragment accumulated to a much higher levelthan the other ligated products (compare Fig. 4A, B, and C), ina manner resembling RNA ligase activity observed in Leishmaniatarentolae (5). Indeed, while the simple ligation product ofthe 5' and 3' fragments appeared within 2 min, its abundance didnot increase appreciably over the course of the experiments despitethe substantial abundance of the input 5' fragment. The levelof U addition products with more U's than specified by gRNA wasless than 0.5% of input or undetectable throughout the time course(Fig. 4, right-hand panels). The formation of edited product initiallyclosely followed the formation of the U addition product of thelength specified by gRNA and continued after the specific U additionproduct reached a steady-state abundance. The order of appearanceof the various intermediates and edited RNA was consistent withthe smaller U addition products being intermediates in the reactionand the gRNA-specified U addition product being the immediateprecursor of editedRNA.

U addition to the 5' cleavage fragment without ligation. The U addition step was examined in the absence of ligation, since the kinetic data suggested that products with the numberof added U's specified by the gRNA may be the end product of thisstep. Ligation was prevented by pretreatment of the extract withpyrophosphate to deadenylylate the charged RNA ligase in the editingcomplex (22, 24) or by using a 3' fragment that lacks the5' phosphate (5), unlike the 3' fragment that is generatedby the editing-associated endonuclease (20, 25). Pretreatmentof mt extract with 4 mM pyrophosphate (Fig. 5, lanes 4 and 8)prevented ligation in reactions containing 5'CL18 and 3'CL13ppmRNA fragments and gRNA gPCA6-1A or gPCA6-2A. This indicated thatligation during precleaved editing in the absence of ATP was catalyzedby adenylylated ligase. Similarly, use of the 3' fragment whichlacked the 5' phosphate, 3'CL3'p, rather than 3'CL13pp, also preventedligation in editing reactions (Fig. 5, lanes 3 and 7). In addition,accumulation of gRNA-specified U addition products was reducedunder both experimental conditions. There was a 25 to 35% reductionin the accumulation of the nonligated +1-U-addition product withgPCA6-1A (Fig. 5, compare lane 3 with lane 2) and an 80% reductionof the nonligated +2-U product with gPCA6-2A (Fig. 5, comparelane 7 with lane 6). When the edited products derived from theseU addition products were included, the overall reductions of gRNA-specifiedaddition products (ligated and nonligated) were greater than 85and 95% with gPCA6-1A and gPCA6-2A, respectively. Pyrophosphatetreatment itself inhibited U addition. In the absence of the 5'phosphate, an additional inhibition of 75% occurred after pyrophosphatetreatment (Fig. 5, compare lane 3 with lane 5 and lane 7 withlane 9). However, as mentioned previously, omission of the 5'phosphate from the 3' cleavage fragment by itself also reducedaccumulation of gRNA-specific U addition products. With gPCA6-2Ain the absence of the 5' phosphate, the major U addition productcontained only one U (Fig. 5, lane 7). Nevertheless, the maximumnumber of added U's was that specified by gRNA; the shift in themajor U addition product was likely a result of slower U addition(see below). Products with added U's were reduced to barely detectablelevels when the 3' fragment with no 5' phosphate was used alongwith the pyrophosphate pretreatment (Fig. 5, lanes 5 and 9); theaccumulation of U addition products was reduced by more than 75%compared with omission of the 5' phosphate alone (Fig. 5, comparelane 5 with lane 3 and lane 9 with lane 7). Although blockingligation inhibited U addition, the addition was still clearlydirected by the sequence of gRNA even in the absence of ligation,since no products with more U's than specified by gRNA accumulatedin the absence of ligation.

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FIG. 5. Uridylate addition to the 5' fragment 5'CL18 in the absence of ligation. The 5'-end-labeled 5' fragment, 5'CL18, was incubated for 3 h with gPCA6-1A (lanes 1 through 5) or gPCA6-2A (lanes 6 through 9), which specifies insertion of one or two U's, respectively. Ligation was prevented by pretreatment with 4 mM pyrophosphate for 15 min at 28°C (PP_i) and/or by use of a 3' fragment with no 5' phosphate, 3'CL3'p (No 5' P), as indicated. The input 5'CL18 (arrow), resultant addition products (U1 and U2), ligation product with no inserted U's (L), and RNA edited by the insertion of one (E1) or two (E2) U's are indicated. UTP was omitted in the negative control (lane 1). Partially hydrolyzed A6 pre-mRNA was used for sizing (lane 10).

Pyrophosphate also inhibited full-round insertion editing of A6AC RNA (Fig. 6A). The production of 3' cleavage fragments at40 µM pyrophosphate, which substantially inhibited editing, indicatedthat the loss of editing activity did not occur at the cleavagestep. Pyrophosphate did partially inhibit cleavage at and above400 µM. U addition did occur to the 5' fragment of 5'-end-labeledA6AC during full-round editing, although the addition productswere not abundant, most likely reflecting partial inhibition ofcleavage and U addition by pyrophosphate (Fig. 6B). Importantly,the major U addition products contained the number of added U'sspecified by gRNA or fewer. Products with more U's than specifiedwere very low in abundance or not detectable. U addition to the5' fragment of precleaved A6AC RNA in the presence of pyrophosphatewas also gRNA specific, although less so (Fig. 6C). Although alow level of multiple-U addition occurred in the presence of gRNA,the most prominent addition product, besides the +1-U product,contained the number of added U's specified by gRNA. Therefore,the inhibition of editing of the uncleaved A6AC pre-mRNA by pyrophosphateresulted from prevention of the ligation step, and U additionwas still responsive to the gRNA sequence under conditions inwhich ligation did not occur.

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FIG. 6. U addition to the 5' fragment of A6AC RNA without ligation. (A) Inhibition of insertion editing by pyrophosphate. Editing reactions containing 3'-end-labeled A6AC and gA6[14]USD-2A were preincubated for 15 min at 28°C in the presence or absence of pyrophosphate. The input A6AC (arrow), edited product containing two inserted U's (E2), and the 13-nt 3' cleavage fragment (3') are indicated. (B) U addition to the 5' fragment of A6AC during the uncleaved editing assay. Reactions contained 5'-end-labeled A6AC and no gRNA, gA6[14]USD-1A (No UTP and A), -2A (AA), or -3A (AAA) and were preincubated with 400 µM pyrophosphate. Lane T₁ is a partial RNase T₁ digest of 5'-end-labeled A6AC. The ES2 cleavage site is marked by an arrow. Cleavage fragments with no added U's (U0), and one (U1), two (U2), and three added U's (U3) are indicated. (C) U addition to the 5' fragment of precleaved A6AC. Reaction conditions were the same as described in panel B. Reaction products are marked as in Fig. 3C.

Time course of U addition without ligation. In order to analyze further the specificity of U addition without ligation, kinetic assays similar to those of Fig. 4 wereperformed under conditions that prevented ligation (Fig. 7). Productswith added U's did not reach a steady-state level during a 3-hincubation, and they accumulated more slowly in experiments using3'CL3'p, a 3' fragment that lacks the 5' phosphate, than whenthe 5' phosphate was present (compare Fig. 7 to Fig. 4). The productswith the number of U's specified by the gRNAs accumulated to amuch lower level in the absence of the 5' phosphate during thecourse of the experiment. However, products with fewer U's thanspecified by the gRNAs accumulated to a higher level by 3 h (compareFig. 7 to Fig. 4). Thus, the rate of accumulation rather thanthe ultimate level was reduced by omission of the phosphate. Nevertheless,omission of the 5' phosphate did not impair the gRNA-specificityof the U addition reaction since U addition terminated with thenumber of U's specified by the gRNA (Fig. 7, right-hand panels).

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FIG. 7. Time course of U addition in the absence of ligation. Precleaved insertion reactions were performed as described in the legend of Fig. 3, except that 3'CL3'p, lacking the 5' phosphate, was used in place of 3'CL13pp. Symbols and lines for nonligated U-addition products are the same as in Fig. 3. The solid lines without symbols show nonligated U-addition products formed in the presence of the 5' phosphate, from Fig. 3. Note differences in scale from Fig. 3 in the graphs at left.

gRNA specificity of ligation. We studied the gRNA specificity of RNA ligation in the absence of U addition by performing editing reactions in the absenceof UTP. Ligation of 5'CL18 and 3'CL13pp was measured as a functionof the length of "gap" between the ligatable RNA termini bridgedby gRNA (Fig. 8A) (5). The gap consists of the guiding A nucleotides,which separate the ES termini of the cleavage fragments annealedto the upstream and downstream regions of the gRNA. The precleavedsubstrate was ligated most rapidly when splinted by a gPCA6 gRNAcontaining no A residues at the ES (gPCA6-0A), presumably by bringingthe RNA termini into close apposition (Fig. 8B, gap length 0).Accumulation of ligated RNA in the presence of this gRNA was linearfor the first 15 min of incubation (data not shown); thus, wechose this length of time for measuring the effect of gap length.In reactions containing 0.3 mM ATP (Fig. 8B, +ATP), ligated productwas generated most quickly when no gap was present between the3' and 5' termini, and this activity decreased with each increasein gap length up to 5 nucleotides (nt). Significant ligation occurredeven with a 5-nt gap. In the absence of exogenous ATP (Fig. 8B,-ATP), the efficiency of ligation dropped off much more steeplywith increasing distance between the ligatable RNA termini. WithoutATP, the ligation product was undetectable when the gap was greaterthan 3 nt in length. These results confirm those of Fig. 3B, inwhich addition of ATP to the precleaved insertion reaction increasedthe production of ligation products with the number of insertedU's other than that specified by the gRNA. By this direct analysisof ligation activity, ligation occurring across a gap of at least1 nt was analogous to the formation of improperly edited products.Overall, increased gap length decreased the efficiency of ligation,as was seen for the L. tarentolae mt RNA ligase (5), indicatingthat preferential ligation of 5' cleavage fragments of the correctlength contributed to accuracy during precleaved editing.

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FIG. 8. RNA ligation in the absence of UTP. (A) Pre-mRNA fragments aligned with gRNA, diagramming an n-nucleotide "gap" between 5'CL18 and 3'CL13pp. (B) Precleaved ligation reactions, in the presence (lanes 1 through 6) and absence (lanes 7 through 12) of 0.3 mM ATP, were performed as described in Materials and Methods. The input (arrow) and ligated (L) RNA species are indicated. The efficiency of ligation in each reaction is indicated below the ligated product, and it is expressed as the percentage of total input 5'CL18.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

This study reports the development of a precleaved in vitro editing system, in which the pre-mRNA was provided as two fragments,and its use to examine the U addition and ligation steps of RNAediting. The 5' fragments with the number of added U's specifiedby the gRNA preferentially accumulated during in vitro editing.The 5' fragments with the number of U's specified by the gRNAwere preferentially ligated with the 3' fragment to produce accuratelyedited RNA. Thus, both the U addition and RNA ligation steps actedin concert to contribute to the specificity of the editedsequence.

The precleaved assay displayed all of the features of kinetoplastid insertion RNA editing consistent with the cleavage ligationmodel for editing (6). The reaction required gRNA, UTP, andmt extract that contained active editing complexes which werecapable of catalyzing a full round of in vitro editing (Fig. 3B).It catalyzed the addition of U's to the 3' end of the 5' pre-mRNAfragment and generated accurately edited RNA by ligation withthe 3' fragment of 5' fragments that had the correct (i.e., gRNA-specified)number of added U's (Fig. 3A). The kinetics of this editing reaction(Fig. 4) were similar to those of in vitro U-insertion-editingreactions that use pre-mRNAs which must be cleaved by the editingcomplex (15). In addition, the precleaved assay was efficient.Typically, 15 to 20% of input 5' fragment was processed into accuratelyedited RNA, which was severalfold as efficient as in vitro editingof A6 pre-mRNA, which was not precleaved. This suggested thatthe endonucleolytic cleavage step can limit the rate of editingin vitro. Cleavage appeared to be rate limiting, using the SPand Q Sepharose purified mt extract, since a full round of editingof A6-eES1 RNA was no more efficient using this extract than thatpurified by glycerol gradient sedimentation (data not shown).The precleaved insertion activity also cofractionated, by severaldifferent purification strategies, with the activity that accuratelyedited RNA which was not precleaved, even though the individualTUTase and RNA ligase activities have different profiles in somecases (Panigrahi et al., submitted for publication). The U additionand ligation activities observed here remain to be conclusivelyshown to be components of the editingcomplex.

The efficiency of editing was very low for A6-eES1 precleaved at ES2, when gA6[14] was used, but it was more robust when theU-tail was replaced with a sequence designed to form a stableduplex with the 5' fragment. A stable upstream duplex has beenshown to enhance the efficiency of complete editing reactionsas well (8, 16). In addition, partially purified mt RNA ligasefrom L. tarentolae requires an upstream duplex of 7 nt for optimalligation of two substrate RNAs splinted by a complementary RNAmolecule (5). Furthermore, a strong upstream duplex can counteractinhibition of insertion editing caused by modification of the3' end of gRNA (8). Finally, a stable duplex immediately upstreamof the ES dramatically increases editing efficiency of NADH dehydrogenasesubunit 7 RNA by crude L. tarentolae mt extract (16). Theseobservations suggest that stable interactions between the 3' regionof gRNA and the 5' pre-mRNA fragment enhance the efficiency ofediting. This greater efficiency may be due to more closely tetheringthe 5' fragment to gRNA, preventing chimera formation and alsoreducing religation (without U addition) by promoting base pairingof added U's withgRNA.

The step of U addition to the 3' end of the 5' pre-mRNA fragment appeared to be gRNA specific. Abundant products with thenumber of added U's specified by the gRNA accumulated (Fig. 2and 3). This activity was highly specific for U; other nucleotideswere added very inefficiently, if at all, even in the presenceof complementary "guiding" nucleotides. Thus, the observed U additionwas unlikely to have been the result of an RNA-dependent RNA polymerase.In addition, prevention of ligation by using a 3' fragment thatlacks a 5' phosphate or by pyrophosphate treatment reduced therate of U addition but did not prevent the accumulation of 5'fragments with the correct number of added U's (Fig. 7). The basisfor specific gRNA-directed U addition is unclear. It may be controlledby stopping U addition beyond the number of guiding nucleotidesin gRNA, suggesting that it is a property of the enzyme that addsU's. Alternatively, it may occur by trimming of excess U's bya 3' U-specific endonuclease (1). A robust U-specific exonucleaseactivity is present in the mt extract used in this study (Panigrahiet al., submitted for publication; D. Weston and S. Lawson, unpublisheddata) and may remove 3' terminal U's not protected by base pairing(18). We did not observe ligation of 5' cleavage fragments withmore added U's than specified by gRNA, as was seen in L. tarentolae(9). This difference may reflect our direct analysis of intermediatesand edited RNA rather than the indirect (i.e., primer extension)analysis of reverse transcription-PCR products of edited RNA.The differences may also be explained by differences in activitybetween L. tarentolae and T. brucei editing complexes or betweencrude mt extract (9) and our partially purified extract. However,our results would be consistent with the conclusions drawn inthat study (9), if the removal of excess U's occurred veryrapidly in our mtextract.

U addition in the precleaved assay appeared to be more gRNA specific than that previously observed in the complete insertion-editingreaction (15), in which the gRNA-specified addition productwas not the most prominent nonligated addition product and inwhich U's appeared to be added beyond the gRNA-specified number.However, accumulation of U addition products appeared to be substantiallyrestricted to those with the gRNA-specified number of added U'sor fewer in A6AC RNA after cleavage during a complete editingreaction in which ligation was prevented (Fig. 6B). Nonligatedaddition products with more than the specified number of addedU's were also observed in the precleaved A6AC editing reaction(Fig. 6C). This may reflect the weaker tethering of the 3' terminusof the 5' fragment to the gRNA, thus allowing TUTase to add multipleU's to the 5' fragment (see below). In addition, the lower specificityobserved earlier (15) may have resulted from the use of lesspure mt extract. Although the specificity of U addition seemedto vary among substrate RNAs, accumulation of U addition productsappeared to be responsive to the sequence of gRNA even in theabsence of ligationactivity.

The U addition activity was greatly affected by the presence of the 3' fragment, 5' phosphorylation of the 3' fragment, andthe ability of the ligase to ligate the two fragments. Dephosphorylationof the 3' fragment or deadenylylation of the ligase slowed theU addition overall and also resulted in an increased accumulationof products with fewer U's than specified by the gRNA, comparedto the correct addition product (Fig. 5). Omission of the 3' fragmentresulted in preferential accumulation of 5' product with onlya single added U using gRNA specifying the addition of two U's(Fig. 3B); this was also the consequence of slowing of U addition(data not shown). The accurate and efficient U addition that reliedon the presence of a 3' fragment with a 5' phosphate may reflectthe interactions among the pre-mRNA, gRNA, and editing complex.Indeed, removal of U's from a 5' fragment in the presence of agRNA specifying U deletion is also slowed in the absence of the5' phosphate (D. Weston, unpublished data), perhaps reflectinga similar effect of altered RNA-complex interaction. The importanceof the gRNA in the specificity at the addition step is clearlyillustrated by the production of a ladder of 5' products withincreasing numbers of added U's upon the omission of the gRNA(Fig. 3). This may reflect the altered context of the 5' fragment,since its 3' terminus is presumably single stranded in the absenceof complementary gRNA. Alternatively, the 5' fragment may notbe bound by the editing complex and hence may not be associatedwith gRNA. Indeed, U addition without gRNA may simply be due toa TUTase activity not involved with editing, possibly the TUTasewhich adds U's to the gRNAtail.

The RNA ligation step also appeared to contribute to the accuracy of the edited RNA. The experiments presented here and elsewhere(15) show that although a family of 5' fragments may differin the number of U's produced during editing, those with the numberspecified by the gRNA are preferentially ligated to form editedRNA. The simplest explanation for this specificity is that basepairing of the correct 5' fragment with the gRNA will place theRNA termini to be ligated in closer proximity than would be thecase with incorrect 5' fragments. The incorrect 5' fragments couldbe ligated but appeared to do so at a lower efficiency (Fig. 6).Ligation of incorrect 5' fragments appeared to be more efficientin the absence of the correct fragment (Fig. 3B, compare lanes5 and 7). These characteristics of the RNA ligase activity inour mt extract were similar to those of partially purified mtRNA ligase from L. tarentolae (5). Potentially this preferencereflects accessibility of the RNA termini to the active site ofthe editing-associatedligase.

The production of accurately edited RNA from the precleaved substrate occurred in the absence of added ATP. This is likelyto have been due to the action of adenylylated ligase (11, 22,24), since treatment with pyrophosphate eliminated the ATP-independentligation activity (Fig. 5). Deadenylylation of RNA ligase in mtextract with 8 mM pyrophosphate during purification, before theQ Sepharose fractionation step, also greatly reduced ATP-independentligation. However, ligation was unaffected in its gRNA specificitywhen ATP was added to deadenylylated RNA ligase, producing approximatelyequal levels of gRNA-specific and -nonspecific ligation products(R. P. Igo, Jr., unpublished results). The addition of low tomoderate levels of ATP (<1 µM to 0.3 mM) stimulated ligation activitybut only of incorrect pre-mRNA fragments, i.e., those with feweradded U's than specified by the gRNA (Fig. 2B and data not shown).Ligation of U addition products of correct length was unaffectedby ATP (Fig. 3B), as was ligation of RNA termini with no gap (Fig.8B). Cruz-Reyes et al. (11, 12) found that procyclic mitochondriacontain 0.1 to 1 mM ATP and that increased ATP reduced the productionof RNA that is accurately edited in vitro by U insertion. Theyconcluded that this effect resulted from inhibition of endonucleolyticcleavage by ATP. However, unlike the precleaved assay, editingassays that rely on endonucleolytic cleavage of the pre-mRNA donot detect ligated fragments to which no U's are added (or removed),since these molecules have the same mobility as the input pre-mRNA.Hence the reduced editing observed by Cruz-Reyes et al. can alsobe explained by ATP-stimulated religation of 5' fragments withoutadded U's, which would reduce the pool of available 5' cleavagefragments for U addition. The effect of ATP on precleaved editingreflects an increase in ligation activity but not U addition activity,as indicated by the reduction in nonligated U addition products(Fig. 3A, lane 6). The increased ligation may reflect activationof an RNA ligase that is not involved in editing or an editingRNA ligase that is not associated with the editing complex. Alternatively,it may reflect an inappropriate ATP-dependent step, such as mistimedadenylylation of the editing ligase or a conformational changein an editing complex protein allowing more efficient ligationbut with reducedspecificity.

Previous results indicate that ATP is required for accurate in vitro insertion editing using a 20S glycerol gradient fractionas the source of the editing complex (15). However, the 20Sfraction has very low precleaved insertion activity in the absenceof ATP (ca. 0.25% of input) compared to the fraction from SP Sepharoseand Q Sepharose chromatography (15 to 20% of input), which containsmore concentrated and more highly purified editing complexes (A.K. Panigrahi et al., submitted for publication). The SP Sepharose-QSepharose fraction has much more ligase activity in the absenceof added ATP than does the 20S fraction (S. S. Palazzo, unpublishedresults). In addition, the less pure glycerol-gradient extractmay contain inhibitors of ligase adenylylation or ligase activity,since the adenylylation activity of this extract increased afterdilution of the extract (10). The increased accuracy of insertioncompleted by adenylylated ligase could indicate that RNA ligaseis adenylylated prior to assembly of active editing complexesand that misedited products in the presence of abundant ATP areligated by RNA ligase not associated with such complexes. We arecurrently characterizing the precharged ligase to determine whetherit is identical to the adenylylated ligase described by Sabatiniand Hajduk (24).

The results presented here show that the U addition and ligation steps act in concert to contribute to the generation of accuratelyedited RNA. The former adds the number of U's specified by thegRNA, and the latter preferentially ligates the 5' fragment withthe number of added U's specified by gRNA. However, several importantissues are not yet resolved. Additional study is needed to determinethe RNA structure that the editing-associated U addition enzymerequires for substrate recognition. Does the enzyme add U's tothe 5' fragment only when the 3' terminal nucleotide is base pairedwith the gRNA, as the current results suggest, or does it polymerizeU's which can form base pairs with the guiding A's or G's in gRNA,regardless of the RNA structure at the terminus? It is also unclearwhether the activity that adds the U's to the 5' fragment is thesame as the U addition activity that occurs in the absence ofgRNA (Fig. 3B) and which is measured in various assays for TUTaseactivity (3, 10, 22). The relationship of the activitythat adds oligo(U) tails to gRNA (7) to the U addition seenhere is also unknown. Our results also hint that adenylylationof RNA ligase may occur in a controlled fashion, perhaps withthe participation of other factors, and hence be important tothe mechanism and control ofediting.

The precleaved assay is useful for elucidating the characteristics of the specific steps of editing. The relatively high efficiencyof the reaction allows accurate, quantitative analysis of theeffects of various editing conditions on the production of editingintermediates and end products under different experimental conditions,thus facilitating analysis of the factors that contribute to accurateediting during the U addition and ligation steps. Additionally,the independence from endonucleolytic cleavage allows study ofthe effects of gRNA and pre-mRNA sequences in and around the editingsite that would normally disrupt cleavage. Such work is in progressin ourlaboratory.

	ACKNOWLEDGMENTS

We thank RoseMary Reed, Barbara Morach, and Nicole Carmean for their assistance in preparation of T. bruceimitochondria.

This work was supported by NIH grant GM42188 and HFSPO grant RG/97 to K.S. and NIH postdoctoral fellowship AI10312 to R.P.I.

	FOOTNOTES

^* Corresponding author. Mailing address: Seattle Biomedical Research Institute, 4 Nickerson St., Seattle, WA 98109. Phone: (206)284-8846 x316. Fax: (206) 284-0313. E-mail: kstuart{at}u.washington.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Panigrahi, A. K., Gygi, S. P., Ernst, N. L., Igo, R. P. Jr., Palazzo, S. S., Schnaufer, A., Weston, D. S., Carmean, N., Salavati, R., Aebersold, R., Stuart, K. D. (2001). Association of Two Novel Proteins, TbMP52 and TbMP48, with the Trypanosoma brucei RNA Editing Complex. Mol. Cell. Biol. 21: 380-389 [Abstract] [Full Text]

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