Kinetics of Ribosomal Pausing during Programmed -1 Translational Frameshifting

doi:10.1128/MCB.20.4.1095-1103.2000

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Molecular and Cellular Biology, February 2000, p. 1095-1103, Vol. 20, No. 4
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Kinetics of Ribosomal Pausing during Programmed $-$ 1 Translational Frameshifting

John D. Lopinski,¹ Jonathan D. Dinman,² and Jeremy A. Bruenn¹^,³^,^*

Department of Biological Sciences, State University of New York at Buffalo, Buffalo, New York 14260¹; Department of Molecular Genetics and Microbiology, University of Medicine and Dentistry of New Jersey, Robert Wood Johnson Medical School, The Graduate Programs in Molecular Bioscience Rutgers/UMDNJ, and Cancer Institute of New Jersey, Piscataway, New Jersey 08854²; and Hauptman-Woodward Medical Research Institute, Buffalo, New York 14203³

Received 9 August 1999/Returned for modification 21 September 1999/Accepted 16 November 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

In the Saccharomyces cerevisiae double-stranded RNA virus, programmed $-$ 1 ribosomal frameshifting is responsible for translationof the second open reading frame of the essential viral RNA. Atypical slippery site and downstream pseudoknot are necessaryfor this frameshifting event, and previous work has demonstratedthat ribosomes pause over the slippery site. The translationalintermediate associated with a ribosome paused at this positionis detected, and, using in vitro translation and quantitativeheelprinting, the rates of synthesis, the ribosomal pause time,the proportion of ribosomes paused at the slippery site, and thefraction of paused ribosomes that frameshift are estimated. About10% of ribosomes pause at the slippery site in vitro, and some60% of these continue in the $-$ 1 frame. Ribosomes that continuein the $-$ 1 frame pause about 10 times longer than it takes to completea peptide bond in vitro. Altering the rate of translational initiationalters the rate of frameshifting in vivo. Our in vitro and invivo experiments can best be interpreted to mean that there arethree methods by which ribosomes pass the frameshift site, onlyone of which results inframeshifting.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

A 4.6-kb double-stranded RNA (dsRNA) virus, ScV-L-A (also known as ScV-L1), can be found in many laboratory strains of theyeast Saccharomyces cerevisiae. Like most fungal viruses, ScV-L-Ais exclusively cytoplasmic, has no infectious cycle, and is knownto be naturally transmitted only by budding or by cell fusionduring mating (16). It is a member of the Totiviridae, whichare dsRNA viruses with a single essential viral dsRNA (6).

The viral genome has two open reading frames (ORFs) on its plus strand that overlap by 129 bases (Fig. 1). The first ORF isdesignated cap or gag (after the retrovirus nomenclature) andencodes the 76-kDa major capsid polypeptide. The second, pol,encodes the viral RNA-dependent RNA polymerase (12, 14, 21).Translation of pol as a 171-kDa Cap-Pol fusion protein is permittedby a programmed $-$ 1 ribosomal frameshift (12, 14, 21, 40)(Fig. 1). A second, separately encapsidated viral dsRNA (M₁) encodesa secreted polypeptide toxin (k1 killer toxin) that provides aconvenient phenotype for detecting synthesis of Cap and Cap-Pol(4, 34, 37).

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FIG. 1. (A) The 4.58-kb dsRNA genome of ScV-L-A. (B) The two ORFs, cap and pol, of the ScV-L-A plus strand, separated by the $-$ 1 frameshift within the overlapping region. (C) The ScV-L-A 76-kDa 0 frame protein product Cap and the 171-kDa fusion protein Cap-Pol.

Programmed, or directed, ribosomal frameshifting (PRF) is of particular value to viruses that package their plus strands,as it eliminates the need to splice their mRNAs and reduces therisk of packaging defective genomes. It also regulates the ratioof viral proteins synthesized. Examples of the phenomenon (both+1 and $-$ 1 shifts) have been found in a wide range of systems.In addition to the ScV systems, programmed translational frameshiftinghas been identified in retroviruses (17, 23, 30, 32);coronaviruses (5, 20); giardiaviruses, which are also membersof the Totiviridae (41); two bacterial genes (3, 8); bacteriophagegenes (7); astroviruses (28); the yeast EST3 gene (27);and the rat, mouse, Xenopus, and Drosophila ornithine decarboxylaseantizymes (29) (reviewed in references 13 and 18). A significantnumber of cellular genes may utilize $-$ 1 PRF (19).

The ScV-L-A frameshifting site fits a fairly well described motif for promoting a $-$ 1 translational frameshift. There is aheptanucleotide slippery site (bases 1958 to 1964, GGGUUUA) anda region capable of forming a pseudoknot (bases 1969 to 2023)(14, 40) that together comprise the 71-nucleotide (nt) regionthat has been shown sufficient to support frameshifting (40)(Fig. 2). The existence of the stems of the pseudoknot and therequirement of the pseudoknot for frameshifting have been verifiedby mutagenesis (14, 40).

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FIG. 2. Possible structure of the ScV-L-A pseudoknot. The slippery site is in italics starting at base 1958. The second stem is shown with two more base pairs than in some formulations (14).

The proposed mechanism for the $-$ 1 translational frameshift, simultaneous slippage, was verified for Rous sarcoma virus bysequencing the frameshift product (22). In the case of L-A,the model predicts that the tRNA^Gly-tRNA^Leu in the P and A sites of the ribosome slips backward one baseto pair with the Gly-Phe codons of the $-$ 1 pol reading frame (Fig.3). Translation of the Cap-Pol fusion protein can then proceedin the $-$ 1 frame. This predicts a sequence of GLRS through theframeshift site, which has been verified by protein sequencing(T.-H. Tzeng and J. A. Bruenn, unpublished data). This frameshiftingevent has been shown to take place in vitro in rabbit reticulocytelysates approximately 3.5% of the time a ribosome encounters theslippery site (40) and is important in regulating the stoichiometryof Cap and Cap-Pol in vivo (15). The $-$ 1 translational frameshiftingevent has been shown to require a ribosomal pause at the slipperysite (38, 39), presumably because the ribosome is physicallyimpeded by the intact pseudoknot just 3' to the slippery site(39). The 5' end of the ribosome paused at the slippery sitehas been previously mapped to bases 1946 and 1949 (39) by ribosomalheelprinting (42). Analysis of mutants demonstrates that ribosomalpausing is necessary but not sufficient for frameshifting (38,39).

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FIG. 3. Simultaneous slippage model (22) shown here for ScV-L-A. A tRNA^Gly-tRNA^Leu pair in the 0 frame (underlined) P and A site of the ribosome slips back one nucleotide to pair with the $-$ 1 frame (pol) Gly-Phe codons, leaving mispaired nucleotides in the wobble position of each $-$ 1 frame codon.

In this report, the primary pause site is shown to be at base 1945 rather than 1946. The translational intermediate associatedwith a ribosome paused at this position is detected; using invitro translation and quantitative heelprinting, the rates ofsynthesis, the ribosomal pause time, the proportion of ribosomespaused at the slippery site, and the fraction of paused ribosomesthat frameshift are estimated. About 10% of ribosomes pause atthe slippery site in vitro, and some 60% of these continue inthe $-$ 1 frame. Ribosomes that continue in the $-$ 1 frame pause onthe average about half a minute at the slippery site invitro.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Plasmid construction. Plasmid pGEM7ZCTU was constructed as previously described (40). Briefly, an L-A cDNA fragment of 396 bp (1783 to 2179) wasinserted into a HindIII-Csp451 digested pGEM-7Zf(+) vector (Promega).The fragment contained the 71-nt minimal region necessary to supportframeshifting. Plasmid 7zCTUSS was constructed by site-directedmutagenesis according to the method of Kunkel (26), with modificationsas described elsewhere (40). In 7zCTUSS, base 1958 (G) is changedto an A to inhibit the $-$ 1 frameshift by preventing the simultaneousslippage of the tRNA^Gly-tRNA^Leu backward into the pol reading frame. Mutants 7ZCTUm3, a disruptionof stem 1 of the pseudoknot, 7ZCTUm5, an inverted restorationof stem 1, and 7ZCTUd9, a deletion of the L-A bases beyond 2012,which truncates stem 2 of the pseudoknot, were constructed asdescribed elsewhere (40).

In vitro transcription. Transcripts for in vitro translations and heelprint analysis were made as described by Kreig and Melton (25) from the plasmidsdescribed above linearized with SspI (Bethesda Research Laboratories).Transcription for protected fragment analysis used [³²P]UTP (specific activity, 3,000 Ci/mmol) at a final concentrationof 1 µM and nonradioactive UTP at 0.1 mM. Transcripts for thepulse-chase translations and the heelprint showing artifacts (Fig.5) were done with SspI-linearized pGEM constructs that yieldeda 1,114-base message. Transcripts for the heelprint in Fig. 6,the translations in Fig. 8, and the protected fragment analysiswere made with XbaI-linearized pGEM constructs that gave a 480-basetranscript.

In vitro translation. Translations were performed with rabbit reticulocyte lysates as previously described (39). A standard translation was at26°C for 25 min without a chase with nonradioactive methionine.Translation products were expected to be 75 amino acids long (slippersite stop [SST] product), 110 amino acids 0 frame stop [0ST] product,and 234 amino acids (frameshift [FS] product) for SspI-linearizedtemplate transcripts of 1,114 bases. XbaI-linearized templatesgive a runoff translation FS product of 160 amino acids, whilethe SST and 0ST products are the same. For [³⁵S]Met-labeled translations, the final volume of the reaction was50 µl, of which 33 µl was lysate. Protected fragment translationswere done in a 25-µl volume, of which 17.5 µl was lysate. In eachtranslation, the FS and SST products have a single methionine(at the N terminus), while the 0ST product has threemethionines.

Heelprinting. Heelprinting (see Fig. 4) was performed as described elsewhere (39, 42), with additional modifications as follows in laterheelprints. The final reaction volume was 25 µl, of which 17.5µl was lysate. All translations and heelprints were done at roomtemperature and used about 3 µg of RNA. The Flexi (Promega) rabbitreticulocyte system was used. The nuclease digestion to degradeall RNA not protected by ribosomes was performed in 40 µl of 1mM cycloheximide-3.5 mM magnesium acetate-3 mM CaCl₂, first withmicrococcal nuclease (final concentration, 10 U/µl; BoehringerMannheim) at room temperature for 10 min, then with RNase V1 (Pharmacia)at a concentration of 17.5 U/ml for 10 min, and then with pancreaticRNase A (25 µg/ml) for an additional 5 min. The heelprinting reactionwas completed as described previously (39) except that the nuclease-liberatedmonosomes with protected fragments were spun through the sucrosecushion at 70,000 rpm in a Beckman TLA 100.3 rotor for 30min.

Protected fragment quantification. Protected RNA fragments were generated by translation of gel-purified [³²P]UTP-labeled RNA combined with cold transcripts generated fromthe same template. The transcription reactions containing the[³²P]UTP were run on an 8 M urea-4.5% polyacrylamide gel. The positionsof the full-length transcripts were visualized with a MolecularDynamics PhosphorImager, after which they were cut from the geland eluted. Approximately 10⁶ cpm of the purified transcript was then combined with 3 µg ofthe corresponding cold transcript and used to program the rabbitreticulocyte translations. The reactions were then taken throughthe heelprinting procedure described above to the point whereribosome-protected RNA fragments were precipitated in ethanol.The fragments were then dissolved in 8 µl of diethyl pyrocarbonate-treatedH₂O and subjected to a modified version of the RNase reactiondescribed by Myers et al. (31). In this procedure, 2 µl of protectedfragments was added to each of three separate reactions containing27 µl of a solution of 80% formamide, 40 mM piperazine-N,N'-bis(2-ethanesulfonicacid) (PIPES; pH 6.4), 0.4 M NaCl, and 1 mM EDTA; 2 µg of a 76-baseoligonucleotide identical to the minus strand of L-A from bases1985 to 1910 was added to one of the three reactions for eachmutant. The SS hybridizations used an oligonucleotide identicalto this with the single change of C to T at 1958. Each reactionwas then brought to a final volume of 30 µl, heated to 90°C for2 min, and placed at 45°C for 30 min to ensure hybridization ofthe RNA fragments to the oligonucleotide. The samples were spunbriefly and then diluted to 60 µl with a solution containing 20mM Tris-HCl (pH 7.5), 2 mM EDTA, 400 mM NaCl, and 200 mM LiCl.To one of the reactions with RNA fragments and no oligonucleotideand to the reaction with RNA fragments and oligonucleotide, 0.06µg of pancreatic RNase (RNase A) was added. The reaction mixtureswere incubated at room temperature for 20 min, after which 1 µlof 3' RNAsin was added to each. The samples were phenol-chloroform-isoamylalcoholextracted twice, made to 0.3 M sodium acetate, diluted twofoldwith cold ethanol, incubated at $-$ 20°C for at least 1 h, spun for20 min at 4°C, rinsed with 70% ethanol, and vacuum dried. Thesamples were then dissolved in 4 µl of 1× sequencing gel loadingbuffer (36), boiled for 2 min in a water bath, and resolvedon an 8 M urea-8% polyacrylamide gel next to a DNA sequencingreaction as a size marker. The resulting bands for each mutantwere quantified relative to that of the controls for that mutant,using a Molecular DynamicsPhosphorImager.

In vivo frameshifting assays. Wild-type (WT) killer⁺ cells were transformed with a series of plasmid-based GCN2^c-constitutively active alleles of the eIF-2^c kinase, which inhibit translational initiation to various degreesfrom strong to weak (33) (kindly provided by A. Hinnebusch andT. Dever). PRF was measured with the tester pTI25 (0 frame control),pF8 or pJD104 ( $-$ 1 or +1 ribosomal frameshift tester respectively),or pT124 ( $-$ 1 frameshift suppression) (2, 14).

Statistics. Standard errors in rates or ratios of rates were determined by calculating the limits of intercepts or slopes of straightlines with the statistical program StatView. Standard errors ofindividual values were determined from repeatedmeasurements.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

A number of parameters of pausing can be estimated in vitro. From the rate of in vitro translation and the time it takes allribosomes to finish translating in the $-$ 1 frame after a chasewith nonradioactive methionine, it is possible to estimate themaximum time a ribosome pauses at the slippery site. An independentestimate of the average pause time can be made from heelprinting.From the heelprinting data and from the ratio of the rates ofsynthesis of the SST and FS products, it is possible to deriveindependent estimates of the fraction of paused ribosomes thatframeshift. Similarly, by altering the rates of initiation, itis possible to estimate the fraction of paused ribosomes thatframeshift invivo.

Heelprinting. Heelprinting experiments with ribosomes translating the L-A message were repeated in order to develop conditions for makingquantitative measurements of paused ribosomes. The heelprintingtechnique (outlined in Fig. 4) is designed to map the 5' positionof some factor (in this case a ribosome) that protects mRNA fromnuclease digestion. The same primer and template are used to generatethe sequencing ladder and the primer extension that becomes theheelprint. Where the primer extension is inhibited by a protectedRNA fragment hybridized to the template, a band results, migratingon the gel to a position corresponding to the most 5' nucleotideof the message protected by a ribosome from nuclease digestion.The position is identified by comparison with the adjacent sequencingladder.

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FIG. 4. Heelprinting technique (42). In step 1, translating ribosomes are stopped on the template with cycloheximide and EDTA and unprotected mRNA is digested away, liberating monosomes. In step 2, the monosomes are collected through a sucrose cushion and the ribosomal proteins are stripped away, yielding protected RNA fragments. In step 4, the fragments are annealed to an ssDNA that has a region complementary to the message used in the translation. The heteroduplexes stop the extension of a primer at the 5' ends of the RNA fragments that were protected from nuclease by the ribosome. In step 5, the primer extensions are elaborated next to a DNA sequencing ladder generated with the same primer on the same ssDNA template, thereby mapping the 5' end of the protected RNA fragment.

While this is primarily a mapping tool, the relative differences in intensities of bands at any particular position indicatequalitatively the number of ribosomes paused at the position inquestion within the population of messages being translated. Themicrococcal nuclease heelprinting experiment shown in Fig. 5 includesthe previously unpublished heelprint for the slippery site (SS)mutant which has base 1958 (G) altered to an A in order to preventthe $-$ 1 slippage of the ribosome into the pol reading frame. Thismutant shows less than 1% of the frameshifting efficiency of theWT (14). The SS heelprint differs from the remaining lanes primarilyat base 1945, misread as 1946 in reference 39, where a distinctband can be observed. This indicates that the 5' end of the pausedribosome was positioned at base 1945. Since it is known that therabbit reticulocyte ribosomes protect a region of mRNA of about30 bases (39), this result is consistent with a ribosome beingpositioned with its P and A sites over the slippery site (1958)and verifies previous data showing that pausing is necessary butnot sufficient for frameshifting (38, 39). Construct d9 truncatesthe pseudoknot at base 2012, thereby greatly diminishing the ribosome'spropensity to pause at the slippery site (39). While the heelprintsof the SS and d9 constructs have many bands in common, they clearlydiffer at position 1945, where the band present in the SS heelprintis entirely missing in the d9 heelprint.

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FIG. 5. Heelprinting results with micrococcal nuclease. Lanes represent the SS and d9 mutants, control with mRNA left out of translation, and control with no reticulocyte or RNA used in the heelprinting reaction (no frag).

The bands they do share can be identified as artifacts of two kinds: bands derived from adventitious hybridization of RNAfragments (probably from rRNA), and bands derived from preferredstops of the T4 DNA polymerase used for the primer extension.The latter variety of artifact is illustrated by the "no frag"lane: a heelprint performed on the single-stranded DNA (ssDNA)template without any reticulocyte or RNA used in the reaction.Note that in this negative control the T4 DNA polymerase usedin the reaction has a tendency to stop at bases 1946, 1949, 1953,1956, and 1963. Additionally, longer stop products can be seenin all lanes. The negative controls were repeated many times toensure that the cause of the artifactual bands was not contaminatedreagents. Artifactual stops seem to increase with the age of thepolymerase (unpublished data). These appear to be the result ofnatural pauses by the T4 DNA polymerase on the template, and themajor bands occur at pyrimidines just preceding A residues (bases1949, 1953, 1956, and 1963). The authentic heelprint at base 1945is a G preceding a pyrimidine. Additional bands, primarily ofsmaller size, are present in the "no RNA" lane (a heelprintingreaction carried out with an unprogrammed reticulocyte lysate).These are greatly reduced by more extensive RNase digestion ofprotected fragments (see below) and are therefore probably theresult of adventitious hybridization of fragments of RNA fromthe reticulocyte lysate, presumablyrRNAs.

Figure 6 shows the heelprint of the WT construct along with the SS mutant, M3 (disruption of stem 1 of the pseudoknot), M5(pseudoknot restoration), d9 (pseudoknot truncation), and a negativecontrol with no RNA protected fragments added to the heelprint.As in Fig. 5, the heelprint is at position 1945. The WT, SS, andM5 constructs all show a pronounced heelprint at base 1945. Disruptionsof the pseudoknot (M3) and deletions of the pseudoknot (d9) yieldmuch less signal at 1945, consistent with decreased ribosomalpausing in the absence of the pseudoknot. Many of the low-molecular-weightartifactual bands are missing from this set of heelprints, becausetheir protected RNA fragments were produced by sequential digestionwith micrococcal, V1, and pancreatic RNases. The artifactual bandsresulting from T4 DNA polymerase hard stops are still visibleat bases 1949, 1953, 1956, and 1963. It is clear from these datathat the only position at which ribosomes are frequently pausedon this message is over the slippery site, because the only prominentheelprint (after eliminating artifactual bands) is at base 1945.

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FIG. 6. WT and mutant heelprints and a heelprint without added RNA ( $-$ ).

Quantification of ribosome-protected fragments. Using conditions such that the majority of ribosome-protected fragments are derived from ribosomes paused at the slipperysite, it is possible to determine what proportion of ribosomespausehere.

We measured the protected RNA that could result from one or two ribosomes paused behind the pseudoknot i.e., from bases 1913to 1989, a span which covers slightly more than the minimum 60bases that two stacked ribosomes should cover. However, very fewexperiments show a heelprint in the vicinity of 1913, so underthese conditions, few messages have more than one ribosome pausedat the slippery site (notshown).

The molar fraction of RNA being translated which is in protected fragments from the region in which the heelprint occurs (f)is the fraction of ribosomes paused at the slippery site. Thequantity f is estimated by PhosphorImager quantification froma gel in which the input fragments run through a mock hybridizationand the input fragments hybridized to the 76-base region are elaboratedon a sequencing gel (Fig. 7). f is the ratio of the amount ofRNA in lane c divided by the amount of RNA in lane a. This isthe fraction of ribosomes that are paused at the slippery site(see below) and turns out to be 0.132, or 13.2% ± 1.6%, in theWT, approximately the same in the SS mutant, and less in M3, asexpected. If the amount of hybridization in the M3 control istaken as the background due to random isolation of fragments fromthis region, then the fraction of ribosomes paused at the slipperysite is (13.2% ± 1.6%) $-$ (6.7% ± 0.9%) = 6.5% ± 2.5%. This experimentwas performed twice for each mutant and three times for the WT.The result agrees well with the proportion of paused ribosomesestimated from the relative rates of synthesis of the SST andFS products of 10.6% ± 2% (see below).

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FIG. 7. Quantitative protected fragment recovery. Protected RNA fragments from the WT, SS, and M3 constructs are shown after recovery from the hybridization procedure (see Materials and Methods) with no DNA oligonucleotide and no RNase (lanes a), no DNA with RNase (lanes b), or with DNA and with RNase (lanes c).

From the fraction f, the average pause time can be determined. In the heelprint experiments, the message is 480 bases longand contains 110 codons in the 0 frame. If ribosomes are randomlydistributed along the message, this means that a ribosome shouldbe located on any particular codon about 1/110 of the time. Weare assuming that all ribosomes are in the 0 frame for this calculation;since 92 to 98% are in the 0 frame, little error should be introducedby this assumption. Since the rate of translation is 28.2 ± 7amino acids/min (see below), this means that a ribosome shouldspend about 0.035 min/codon. However, about 6.5% of the ribosomeson the mRNA are located over the first slippery site codon. Henceribosomes pause (0.065)/(1/110) = 7.2 times longer here than theyshould if dispersed randomly. Hence the average pause time is(0.035)(7.2) = 0.25 ± 0.07 min. If the ribosomes continuing inthe 0 frame have a negligible pause and about 60% of the ribosomescontinue in the $-$ 1 frame (see below), then the average pause isabout 0.42 ± 0.11 min (0.25/0.6) for ribosomes in the $-$ 1frame.

Identification of translation products. Ribosomal pausing during $-$ 1 translational frameshifting has also been demonstrated by in vitro translation using the coronavirusinfectious bronchitis virus pseudoknot (38). A transient translationalintermediate of a size expected for a ribosome paused at the pseudoknotwas identified. Ribosomal pausing (albeit at reduced levels) usinga simple stem-loop with the same base pairs as the pseudoknotis also demonstrable. While ribosomes did pause in the latterconstruct, they did not frameshift, indicating that pausing maybe required but is insufficient for frameshifting, as also demonstratedby heelprinting (39).

A similar translational analysis of L-A mRNAs from the WT, SS mutant pseudoknot disruptant mutant (M3), and pseudoknot restorations(M5 and M6) is shown in the standard translation of Fig. 8 (nochase with nonradioactive methionine). The 0ST product is themajor product in each translation. The product resulting froma $-$ 1 frameshift (FS) is present only in the constructs capableof frameshifting (WT, M5, and M6). There is one additional product(SST) of the right size to be a peptide halted at the slipperysite. The putative SST is present only where expected, in theSS, WT, M5, and M6 translations. It is not detectable in the M3translation. The predicted and measured sizes of the translationproducts in the longer transcripts are as follows: 0ST (measured,11.8 kDa; predicted, 12.0 kDa), FS (measured, 26.9 kDa; predicted,27.8 kDa), and SST (measured, 8.4 kDa; predicted, 8.4 kDa). Theidentification of the FS product was confirmed by translatinga shorter message (shown in Fig. 8), truncated at the XbaI site,producing an FS product with a predicted size of 18.4 kDa.

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FIG. 8. Standard translation of WT, SS, M3, M5, and M6 constructs. Positions of 0ST, SST, and FS products are indicated. These translations had no chase with nonradioactive methionine.

Kinetics of synthesis of translation products. Translations of WT, SS, and M3 mRNAs terminated after 20 min are shown in the first lanes in Fig. 9. Immediately after thezero point was taken, the reaction was divided into two halves,one of which was brought to 40 µM cold methionine to chase transientproducts. The other half of the reaction was allowed to continuewithout dilution of the labeled methionine, and aliquots weretaken from each half of the reaction as indicated. As in Fig.8, the WT construct clearly shows the production of the FS, 0ST,and SST proteins, while the SS mutant shows the SST and 0ST productsbut not the FS product. The presence of the SST in both the WTand SS constructs but its absence in M3 is predicted by the heelprintshown in Fig. 6, which indicates that there is a ribosomal pauseat the slippery site (heelprint at 1945) for the WT and SS constructsbut not for M3. By PhosphorImager analysis, the accumulation ofthe translation products 0ST, SST, and FS shown in Fig. 9 canbe quantified and the rate of synthesis can be estimated. Therate of synthesis of any in vitro translation product should beproportional to the number of ribosomes translating it. Hence,the frameshift efficiency can be estimated either from the relativerates of synthesis of the FS and 0ST products, corrected for themolarity of methionine in the products, or from the molar ratioof the total amounts of FS and 0ST that accumulate during synthesis.(The 0ST product has three methionines, while the SST and FS productseach have only one, so the 0ST product is three times more intenseper mole.) From the kinetics of synthesis of the FS and 0ST products(Fig. 10 and 11), the relative ratio of rates of synthesis, correctedfor methionine content in the products, gives a frameshift efficiencyof 6.1% ± 0.7%. From the accumulation of translation productsafter 60 min of synthesis (in the absence of a methionine chase),still in the linear portion of the curve, the molar proportionof FS product to total products is 5.2%, fairly close to measuredin vivo rates of frameshifting (see below).

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FIG. 9. Pulse-chase in vitro translations. Reaction mixtures were incubated for 20 min and divided in half. One half was chased with cold methionine, and aliquots were taken from each half (with [+] or without [ $-$ ] Met) at the indicated time points. Positions of the SST, 0ST, and FS products are indicated.

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FIG. 10. Kinetics of synthesis of the WT 0ST product from the data of Fig. 9. The ordinate is relative molar units, generated by the PhosphorImager volume report but divided by 3 to account for the difference in the number of methionines between the 0ST and the FS and SST products. The equation for the least squares line calculated is given.

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FIG. 11. Initial kinetics of synthesis of the WT SST product and FS product, as in Fig. 10, from the same experiment as that of Fig. 10, in relative molar amounts.

After 20 min of synthesis with labeled methionine and 60 min of chase (a total of 80 min of synthesis) (from the data of Fig.9), the molar ratio FS/(FS + 0ST + SST) approaches a value of8.1%. This is probably by virtue of the delayed synthesis of alreadyinitiated FS product, while initiation of 0ST has decreased dueto inactivation of ribosomes. This supposition is confirmed byexamining the proportion of FS product synthesized after the chasecompared to the total products synthesized after the chase, whichis 9.1%.

Fraction of ribosomes that are paused from in vitro translations. As above, the number of ribosomes translating an in vitro translation product should be proportional to its rate of synthesis.Hence the percentage of ribosomes that pause at the slippery sitecan be calculated from the relative initial molar rates of accumulationof the SST and 0ST products. From Fig. 10 and 11, this is 14.5%± 2.2%. However, not all of this represents paused ribosomes.It is clear from Fig. 9 that not all of the SST product can bechased into FS or 0ST; some of it persists, presumably due toincorrect termination of ribosomes and release of SST (1, 24),which is not degraded as it would be invivo.

The percentage of ribosomes which incorrectly terminate at the slippery site can be estimated from the amount of SST synthesizedafter the chase as a fraction of total synthesis. Any paused ribosomesthat do continue synthesis result in product that appears in theFS and 0ST, and so only the incorrectly terminating ribosomescontribute to the amount of SST synthesized after the chase. Theamount of SST synthesized after the chase is 3.9% of the totalprotein synthesized. Consequently, the rate of accumulation ofSST by ribosomes that will continue past the slippery site eitherin the $-$ 1 frame or in the 0 frame is 14.5% ± 2.2 $-$ 3.9% = 10.6%± 2.2% of the rate of synthesis of total products, or the correctedfraction of ribosomes paused at the slippery site is 10.6% ± 2.2%.About a quarter of the SST synthesized is not a transient productbut a termination product. This calculation of the fraction ofribosomes that pause assumes that synthesis of a terminal SSTproduct generates an SST product but not a discernible pause.This value of 10.6% ± 2.2% compares well with the calculationfrom quantification of ribosome-protected RNA fragments (6.5%± 2.5%; see above), supporting the assumption that the generationof terminal SST products does not create a discernible ribosomalpause.

Percentage of paused ribosomes that frameshift. The relative numbers of paused ribosomes that pause and that go on in the $-$ 1 frame can be estimated from the ratio of ratesof synthesis of FS and SST from Fig. 11. The percentage of pausedribosomes that frameshift at the slippery site is the ratio ofFS rate to SST rate times 100 = 100 × (6.1 ± 0.7)/(10.6 ± 2.2)= 57.5% ± 23%. This assumes that all ribosomes translating inthe $-$ 1 frame have undergone a detectable pause at the slipperysite, an assumption justified by the demonstrable dependence offrameshifting on pausing (Fig. 5, 6, and 8).

Translation rate. A number of calculations depend on knowing the actual rate of in vitro protein synthesis under our conditions. The averagerate of translation can be estimated from the initial time ofappearance of products of known size. The initial times of appearanceof the control protein (luciferase, 552 amino acids) and the 0STproduct (110 amino acids) are 33.5 ± 3 min (not shown) and 17.8± 0.5 min (Fig. 10), respectively. If both have the same initialdelay before synthesis (mainly due to the time it takes to equilibratethe tRNA^Met with labeled methionine), a rate of 28.2 ± 7 amino acids/minin the in vitro translation (considerably slower than in vivo)is calculated. A similar answer results from making the same assumptionabout the synthesis of luciferase and the SST. The initial delayis calculated to be 13.9 min, which agrees well with data obtainedby chasing with nonradioactive methionine (seebelow).

Estimate of pause time from translation rates. The minimum pause time in the $-$ 1 frame can be estimated from the intercepts of the SST and FS synthesis lines (Fig. 11). TheSST is first visible at about 10 min (10.2 ± 1 min), and the FSappears at about 20 min (20.2 ± 2 min). Hence, it takes about10 min (10.1 ± 3 min) minus the time it takes to translate theremaining 159 amino acids, or 10.1 ± 3 $-$ (159/28.2 ± 7) = 4.5± 5 min, minimum, to resolve the paused ribosome at the slipperysite in the $-$ 1 frame. The standard deviation here is very large,and the minimum pause time is not significantly different fromzero.

The maximum pause time is estimated from the difference between clearance times of ribosomes translating the 0ST and FS productsby measuring translation activity remaining (Fig. 12) after chasefor the WT and M3 mutant constructs. It takes 30 min to clearall ribosomes capable of making the FS product. It takes 20 minto clear all ribosomes capable of making the 0ST (in the M3 mutant,in which the stop is eliminated).

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FIG. 12. Translation activity remaining during the chase with nonradioactive methionine for the M3 0ST (m3 ST) and WT FS. The percent activity remaining (AR) is calculated from the plateau value of the PhosphorImager volume report for the FS or 0ST (P) and the value at 0 to 50 min after the chase of the volume report (V), as follows: AR = 100[(P $-$ V)/P].

Note that most of this time is the time it takes for equilibration of nonradioactive methionine: the maximum time to clearthe 0ST message of ribosomes (without a pause, as in M3) wouldbe the time it takes to translate the entire 0ST message: [110/(28.2± 7)] = 3.9 ± 1 min. So 20 $-$ 3.9 ± 1 = 16.1 ± 1 min (with standarderror minimized [see below]) is the time for the methionine poolto reach equilibrium. This agrees well with the estimate of 13.9min for tRNA^Met pool equilibration calculated by assuming the same rates of synthesisof luciferase and the 0ST (seeabove).

The maximum time a ribosome pauses at the SST is 10 min minus the difference in time it takes to translate from the 0 frametermination codon to the $-$ 1 frame termination codon, or 10 $-$ [(234 $-$ 110)/(28.2 ± 7)] = 5.6 ± 1.5 min. Since the 10-min differencein clearance times has no easily calculated standard error, thestandard error of 1.5 min is a minimumestimate.

Estimate of average pause time from translation chases. The small percentage of ribosomes continuing on in the $-$ 1 frame takes much longer to clear, and the average pause time forthese can also be calculated (Fig. 12) from the time it takes halfof them to clear (16.5 min) minus the time it takes half the 0STribosomes to clear (6 min). Again, as above, subtracting the timeit takes to translate from the 0 frame termination codon to the $-$ 1 frame termination codon gives 10.5 $-$ (4.4 ± 1.5) = 6.1 ± 1.5min for an average pause time. A meaningful standard error cannotbe calculated for either the maximum or average pause times derivedfrom Fig. 12, but the maximum pause time of 5.6 ± 1.5 min calculatedabove is not significantly different from the average pause time.The relatively long time necessary to equilibrate the tRNA^Met pool makes this estimate of average pause time inherently inaccurate,but these translational measurements place an upper limit on thepausetime.

Average pause times, estimated by two independent methods, for ribosomes continuing in the $-$ 1 frame were 6.1 ± 1.5 min (range,4.5 ± 5 to 5.6 ± 1.5 min) calculated by in vitro translation and0.42 ± 0.11 min calculated byheelprinting.

Ribosome spacing in vivo. It is also possible to perturb $-$ 1 PRF in vivo in order to measure some of its characteristics. Since the RNA pseudoknot mustdenature to allow passage of the ribosome, the passage of subsequentribosomes will be affected by (i) the relative rates of pseudoknotrenaturation, (ii) ribosome transit speeds, and (iii) the temporaldistance between elongating ribosomes. If pseudoknot renaturationrates and ribosome transit speeds are constant, then mutationsor conditions affecting initiation rates could result in changesin the temporal spacing between elongating ribosomes. This wouldchange the amount of time available for renaturation of the pseudoknot(which was denatured by a prior transiting ribosome) before itencountered the next transiting ribosome. Therefore, those conditionswhich decrease rates of translational initiation would resultin elongating ribosomes being spaced further apart. Consequently,the pseudoknot would have more time to renature, leading to anincrease in the percentage of ribosomes that encounter the renaturedpseudoknot, increasing the percentage of paused ribosomes andthereby increasing the overall efficiency of $-$ 1 ribosomal frameshifting.Conversely, mutations or conditions which increase initiationrates would yield lower efficiencies of $-$ 1 ribosomal frameshifting.Further, since Ty1-directed +1 ribosomal frameshifting and frameshiftsuppression are independent of an RNA pseudoknot, changing thetemporal spacing between elongating ribosomes should have no effecton thesemechanisms.

We tested the general validity of this hypothesis by transforming WT killer⁺ cells with a series of plasmid-based GCN2^c constitutively active alleles of the eIF-2^c kinase, which inhibit translational initiation to various degreesfrom strong to weak (33) (kindly provided by A. Hinnebusch andT. Dever). The results are summarized in Table 1. Examinationof the data reveals that the ribosome spacing hypothesis is essentiallytrue in that these mutations specifically affect programmed $-$ 1but not +1 ribosomal frameshifting or frameshift suppression.Interestingly, the increases in $-$ 1 ribosomal frameshift efficienciesare only twofold in cells harboring the GCN2^c alleles, regardless of the severity of the initiation defect.This result can be interpreted in at least two ways: (i) thatin vivo the leading ribosome resolves the pseudoknot for immediatelytrailing ribosomes or (ii) that in vivo ribosome stacking at thepseudoknot prevents frameshifting (see Discussion).

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TABLE 1. Summary of experiments using different GCN2^c alleles on URA3 CEN vectors to test the effects of initiation defects on ribosomal frameshifting^a

The in vivo rates of frameshifting (3.5% ± 0.7% in the WT) are similar to those measured in vitro (6.1% ± 0.7%).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We have determined, by heelprinting and by analysis of in vitro translation products, that about 10% of ribosomes normallypause at the L-A slippery site and that many fewer pause whenthe downstream pseudoknot is disrupted. These measurements assumethat ribosomes that incorrectly terminate at the pseudoknot donot detectably pause. By these same assumptions, about 60% ofpaused ribosomes frameshift. The extent of the pause at the slipperysite can be calculated by several methods from in vitro translationdata, all of which arrive at a pause of minutes, with some uncertainty.A calculation from the fraction of paused ribosomes, assuminga random distribution of ribosomes in the absence of pausing,gives a more exact pause time of about half a minute in vitro.All calculations of ribosomal pause time exceed by at least 10-foldthe time it takes to make a single peptidebond.

Our in vitro experiments can best be interpreted to mean that ribosomes may suffer three fates at the frameshift site in L-AmRNA.

Fate 1. About 10% of ribosomes pause at the pseudoknot. Another 4% of the ribosomes prematurely terminate. The remaining ribosomespass the pseudoknot before it causes an obstruction. This couldoccur in two ways: the first ribosome translating the messagecould resolve the pseudoknot, and all subsequent ribosomes couldencounter the unwound pseudoknot before it could re-form; or asubset of the Mof proteins or the translational surveillance complex(SC) (35) could recognize and resolve these RNA structures independentof elongatingribosomes.

Ribosomes that encounter the pseudoknot either pause at the pseudoknot or terminate there. Paused ribosomes may continue translationin two ways: either by a melting of the pseudoknot and a resumptionof 0 frame translation or by a $-$ 1 translational frameshift (about60% of the time invitro).

Fate 2. In the second mechanism, which permits a resumption of 0 frame translation after ribosomes are already paused at the pseudoknot,the MOF gene products seem to be involved, since altering theireffectiveness alters the frequency with which the third methodof passing the pseudoknot is chosen. Consequently, MOF gene productsare probably involved in both the first and second mechanismsby which ribosomes pass thepseudoknot.

Fate 3. The third form of resolution, which is of most interest, requires both the pseudoknot and the slippery site. The pseudoknotis necessary since a simple secondary structure of similar stabilitycauses pausing but not frameshifting (38) and because a mutantwith two to four bases of the second stem deleted (depending onhow the pseudoknot is drawn) demonstrates ribosomal pausing butnot frameshifting (39). The slippery site is necessary, as shownby the present results, since the SS mutant shows essentiallynormal pausing both by heelprint analysis and by in vitro translationyet reduces frameshifting to very low levels. Therefore, thisthird mechanism of resolution of the ribosome-pseudoknot complexmust require a specific interaction between the pseudoknot andsome component(s) of the translation machinery not yet defined.This resolution may be a lengthy process, since ribosomes pause(in vitro) for at least 10 times as long as it takes to make asingle peptidebond.

Relationship between in vitro and in vivo $-$ 1 PRF. The one experiment we have performed to change the kinetics of $-$ 1 PRF in vivo tells us that there are some differences betweenframeshifting in vivo and in vitro. Our preferred interpretationof the results is that decreasing the initiation rate resultsin an increase in frameshifting efficiency because the leadingribosome no longer clears the pseudoknot for trailing ribosomes;the pseudoknot now re-forms before a trailing ribosome arrives.The fact that there is a ceiling on frameshifting efficiency,twice the basal rate, regardless of how low the rate of initiationis most simply interpreted to mean that normally 50% of ribosomespause at the pseudoknot, while with limited initiation, essentiallyall ribosomes pause. However, this would imply that only 7% ofthe paused ribosomes shift frame in vivo, while 60% do so invitro.

The disparity between in vivo and in vitro results may be explained by the role of the Mof proteins. It is becoming clearthat the process of remodeling nuclear to cytoplasmic ribonuclearparticles is a key step in determining the posttranscriptionalfate of mRNAs (11). There is evidence to support the notionthat RNP remodeling by the first translating ribosome and itsassociated SC also plays a role in programmed $-$ 1 ribosomal frameshifting.For example, we have demonstrated that mutants of at least threefactors present in the SC, Upf1p/Mof4p, Upf3p, and Sui1p/Mof2p,affect programmed $-$ 1 ribosomal frameshift efficiencies (9,10, 35). We propose that one of the functions of the SC isto recognize and resolve complex tertiary mRNA structures. Forexample, one of the factors in the SC may specifically recognizethe pseudoknot and recruit another (e.g., the Upf1p RNA helicase)to unwind this structure. Additionally, other, yet to be characterizedMof proteins, either components of the SC or integral ribosomalproteins that are part of the intrinsic ribosomal helicase, mayplay a role in recognizing and resolving the pseudoknot. By thismodel, resolution of the pseudoknot by the first ribosome or SCis part of the nuclear-to-cytoplasmic RNP remodeling process.Given that the nonsense-mediated mRNA decay machinery is not functionalin translationally competent cell extracts (i.e., reticulocytelysates), it is probable that the pseudoknot-resolving activityof the SC is also not functional in the in vitro system. Thiswould explain why the frameshifting of paused ribosomes is somuch higher in the reticulocyte system that in intactcells.

A second interpretation of the increased frameshifting in vivo with decreased initiation rates is that when ribosomes stackup behind the pseudoknot, the first ribosome (on the slipperysite) cannot move backward one base because of the ribosome behindit. The significance of the ceiling of twice the usual frameshiftingefficiency would be that in yeast in vivo, under normal initiationconditions, 50% of the time ribosomes are stacked, but that asignificant decrease in initiation rate results in no stackingat all. Again, the in vivo result is different from what one wouldexpect in vitro, since there are very few ribosomes translatinga message in vitro. In fact, in our system, we calculate fewerthan two ribosomes per mRNA (results not shown). This would explainthe absence of stacking as detected by heelprinting in vitro.This explanation makes no predictions about what fraction of ribosomespause in vivo and so is not inconsistent with the in vitrodata.

Pause time in vivo. The time ribosomes spend paused at the pseudoknot is estimated by two independent methods, both of which arrive at a pausein the range of minutes. If the relationship between the pausetime in vitro and the pause time in vivo is the same as the relativerates of translation, this would correspond to several secondsin vivo. However, since the slow rate of translation in vitrois probably due to the diffusion-limited accessibility of chargedtRNAs and other components, which are probably closely associatedwith the translation complex in vivo, and since frameshiftingprobably requires only components closely associated with theribosome both in vivo and in vitro, it is not clear that directextrapolation of in vitro pause times to the in vivo situationis correct. It may be that pause times in vivo are more like thoseobserved in vitro. At any rate, the pause time in vivo is a minimumof several seconds, or at least an order of magnitude longer thanthe time it takes to complete a single peptidebond.

	ACKNOWLEDGMENTS

We thank A. Hinnebusch and T. Dever forplasmids.

We thank the NIH (grant GM58859 to J.D.D. and grant GM22200 to J.A.B.) and the NSF (grant MCB9727630 to J.A.B.) forsupport.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biological Sciences, State University of New York at Buffalo, Buffalo,NY 14260. Phone: (716) 645-2868. Fax: (716) 645-3776. E-mail:cambruen{at}nsm.buffalo.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Kinetics of Ribosomal Pausing during Programmed 1 Translational Frameshifting

Kinetics of Ribosomal Pausing during Programmed $-$ 1 Translational Frameshifting