The phenotype of many independently isolated +1 frameshift suppressor mutants supports a pivotal role of the P-site in reading frame maintenance.

The main features of translation are similar in all organisms on this planet and one important feature of it is the way the ribosome maintain the reading frame. We have earlier characterized several bacterial mutants defective in tRNA maturation and found that some of them correct a +1 frameshift mutation; i.e. such mutants possess an error in reading frame maintenance. Based on the analysis of the frameshifting phenotype of such mutants we proposed a pivotal role of the ribosomal grip of the peptidyl-tRNA to maintain the correct reading frame. To test the model in an unbiased way we first isolated many (467) independent mutants able to correct a +1 frameshift mutation and thereafter tested whether or not their frameshifting phenotypes were consistent with the model. These 467+1 frameshift suppressor mutants had alterations in 16 different loci of which 15 induced a defective tRNA by hypo- or hypermodifications or altering its primary sequence. All these alterations of tRNAs induce a frameshift error in the P-site to correct a +1 frameshift mutation consistent with the proposed model. Modifications next to and 3' of the anticodon (position 37), like 1-methylguanosine, are important for proper reading frame maintenance due to their interactions with components of the ribosomal P-site. Interestingly, two mutants had a defect in a locus (rpsI), which encodes ribosomal protein S9. The C-terminal of this protein contacts position 32-34 of the peptidyl-tRNA and is thus part of the P-site environment. The two rpsI mutants had a C-terminal truncated ribosomal protein S9 that destroys its interaction with the peptidyl-tRNA resulting in +1 shift in the reading frame. The isolation and characterization of the S9 mutants gave strong support of our model that the ribosomal grip of the peptidyl-tRNA is pivotal for the reading frame maintenance.

Introduction

Evolution of the translation apparatus involved in transfer of the genetic message stored in mRNA into proteins was an early event [1]. In the beginning of life translation made many missense errors and it was not possible to translate long mRNAs due to difficulties in maintaining the reading frame. Thus, the evolution of how translation avoids missense and reading frame maintenance errors must have occurred early and before the three domains of life emerged. Therefore, its basic mechanism is most likely similar in all organisms [1]. Many missense errors are not harmful and they occur in cells of to-day at a frequency of about 4×10−4 per codon [2] although it varies widely at different sites in bacteria and in yeast [3], [4]. Even if this error level is low, it would still result in that only 78% of the molecules of a 500 amino acid protein having no missense error [5]. Therefore, in a cell many proteins are not faithfully decoded and contain missense errors. Since many of these errors are in non-critical positions of proteins and influence their activity and stability in only minor ways, such an error level is apparently acceptable for the cell. However, every processivity error, such as a frameshift error, is harmful, since ribosomes shifted into the wrong frame will generally soon encounter a stop codon and terminate and thereby generate a truncated peptide. Accordingly, the frequency of processivity error should be lower than missense errors although the estimates of such spontaneous frameshift errors have been difficult to assess [5]. Parker suggested that the frameshift errors may be 10−5 or less [2] and thus at least 10-fold less than the level of missense errors.

Although we have learnt much about the mechanism of translation, especially about the 3D structure of the decoding center and how the tRNA is located on the ribosome at the various steps of translation [6]–[8], the mechanism of how the reading frame is maintained is still not known (reviewed in [9]). In some cases there are special sites, the programmed frameshifting sites, at which frameshifting occurs at high frequency due to the presence of various stimulators [10]–[13]. However, at a much lower frequency, frameshift errors may also occur at sites with no apparent nearby stimulators. Such frameshift errors seem to require that the ribosome stalls due to imbalances in any of the steps in the translation elongation process. One way to avoid frameshift errors would be that each step in the elongation cycle occurs at a uniform rate. Indeed, the various aminoacylated tRNA combined with elongation factor Tu (EF-Tu) functions equivalently in translation suggesting that tRNA and its cognate amino acid have co-evolved [14]. Moreover, modified nucleosides, which are present in tRNAs in all organisms, uniform the function of the tRNA [15]. Indeed, mutants isolated as deficient in various modified nucleosides with vastly different chemical structures, present in many different positions of tRNA, and in different tRNA species, induce frameshift errors [16] [17]–[23]. Structural changes of tRNA as well as alterations in elongation factors and rRNA also induce frameshift errors [9], [11]. Moreover, starvation of amino acids, presence of rare or stop codons, or over-expression of tRNA also induce such errors [24]–[27] [28], [29]. Therefore, imbalances in the supply of aminoacylated tRNA and certain sequences in the mRNA upset the maintenance of the reading frame. Accordingly, changes in the environment may also induce errors in reading frame maintenance and indeed, cells in stationary phase have an intrinsic increased rate of frameshift error rate [30], [31].

Transfer RNAs with an extra nucleotide in the anticodon loop suppress certain +1 frameshift mutations [32]. From analysis of such altered tRNAs it was inferred that the frame error induced by an inserted nucleotide in the mRNA was corrected by a tRNA having an apparent four nucleotide anticodon. Such an anticodon was suggested to read four bases, allowing a quadruplet translocation and thereby moving the ribosome into the zero frame [32]. This explanation supported the suggestion that the normal tRNA having a three nucleotide anticodon was used as yardstick in reading frame maintenance by monitoring the three nucleotide translocation required for reading frame maintenance [33]. Although the yardstick model was attractive, it was shown not to be valid for the classical frameshift mutations sufA6 and sufB2, which both have an extra G-nucleotide in the anticodon loop of proK and proL , respectively [34]. It was suggested that these tRNAs suppress a +1 frameshift mutation by being defective in A-site entrance and thereby being out-competed by the near-cognate proM . Following a normal three nucleotide translocation, this near-cognate peptidyl-tRNA slips forward one nucleotide thereby moving the A-site codon into the zero frame. In accordance with this model, many base substitutions in the body of proL , of which the sufB2 tRNA is a derivative, as well as in the anticodon, also suppress certain +1 frameshift mutations and the frameshift event occurs in the P-site [35]. Based on these observations and how deficiency of many different modified nucleosides imposes a +1 frameshift, an explanatory model was suggested [16], [36]. In the proposed model (Figure 1) the ribosomal grip of the peptidyl-tRNA is a key feature in reading frame maintenance [36]. There are several ways that a defective tRNA can induce frameshifting, e.g.: Fig. 1, A; the ternary complex with the defective tRNA is so slow entering the A-site that it allows a ternary complex containing a near-cognate tRNA to decode the A-site codon. After a normal three nucleotide translocation to the P-site, the peptidyl-near-cognate tRNA is prone to slip into an overlapping reading frame. Fig. 1, B; the ternary complex with a defective tRNA decodes the codon in the A-site efficiently, but once the defective tRNA has been translocated into the P-site it may slip on the mRNA. Fig. 1, C; the ternary complex containing a defective tRNA is so slow entering the A-site that it causes a pause which allows the wild type peptidyl-tRNA to slip. Note, that various physiological conditions may reduce the level of charged tRNA or the degree of modification and thereby induce a frameshift error according to this model. Basically, as soon as the kinetics of the entry to the A-site and the translocation is not in balance, the ribosome may stall allowing the peptidyl-tRNA to shift frame. This model of frameshifting is similar in many features to other models suggesting P-site slippage [24], [34], [35], [37]–[40] or models proposing that the aberrant peptidyl-tRNA induces a binding of the aa-tRNA in the A-site to the correct frame [39], [41]. In addition we may also expect according to the model that changes in the P-site environment of the ribosome may also induce frameshift errors.

Figure 1

The ribosomal grip of the peptidyl-tRNA is pivotal in reading frame maintenance.

The figure shows three ways (A, B and C) how certain events may induce slippage by the peptidyl-tRNA and thereby a frameshift error. It is the ternary complex (aa-tRNA*EfTu*GTP) which enters the A-site and interacts with the codon but in the figure we have symbolized it with “aa-tRNA” to save space. A. A defective cognate tRNA (red diamond) is slow (broken arrow) entering the A-site allowing a near-cognate aa-tRNA (blue wobble nucleoside) to decode the A-site codon. After a 3 nucleotide translocation the near-cognate peptidyl-tRNA may slip into the +1 frame. B. A defective cognate aa-tRNA (red diamond) decodes efficiently the codon in the A-site. After a 3 nucleotide translocation the defective cognate peptidyl-tRNA may be prone to slip into the +1 frame. C. The defective aa-tRNA (red diamond, yellow tRNA) is slow entering the A-site mediating a pause allowing the cognate wild type peptidyl-tRNA to slip into the +1 frame. Not depicted in the figure, alterations in the ribosomal P-site environment may also induce a frameshift error if the alteration changes the ribosomal grip of the peptidyl-tRNA. The figure is adopted from [36] with permission. Indeed, as shown in this paper a truncation of ribosomal protein S9, which interacts with the peptidyl-tRNA induces an error in reading frame maintenance (See Fig. 6). Moreover, the occupancy of the E-site also improves reading frame maintenance [80], [86]–[88], perhaps by strengthening the ribosomal grip of the peptidyl-tRNA. Therefore, a defective tRNA may also increase frameshifting by altering the dissociation rate of it from the E-site.

An unbiased test of the proposed model (Fig. 1) would be to first select many independent mutants able to suppress various +1 frameshift mutations and then genetically and biochemically characterize such mutants to see whether or not their frameshift phenotypes are consistent with the model. Here we address this question by isolating and characterizing many (467) independently isolated +1 frameshift suppressor mutants. These 467+1 frameshift suppressor mutants had alterations in 16 different loci. According to the model we expected that many loci would, in some way, influence the structure and the activity of a tRNA. Indeed 15 of these 16 loci were in this class and the mechanism how they induce frameshifts to correct the consequences of the +1 frameshift are all consistent with the model (Figure 1). Interestingly, two mutants had a defect in a loci not altering any tRNA but changing the P-site environment. These two mutants (rpsI) had a C-terminal truncated ribosomal protein S9, which C-terminal contacts the peptidyl-tRNA and thereby is part of the ribosomal grip of the peptidyl-tRNA. The isolation and characterization of these rpsI mutants gave a strong support of our model that the ribosomal grip of the peptidyl-tRNA is pivotal for the reading frame maintenance.

Materials and Methods

Bacteria and Growth Conditions

The bacterial strains used were derivatives of Salmonella enterica serovar typhimurium and Escherichia coli (Table 1). As rich media Luria-Bertani (LB) was used [42].The minimal solid medium was made from the basal medium [43] with 15g of agar per liter and supplemented with 0.2% glucose and required amino acids and/or vitamins [44]. TYS-agar (10g of Trypticase Peptone, 5g of yeast extract, 5g of NaCl, and 15g of agar per liter) was used as solid rich medium.

Table 1

S. enterica and E.coli strains used in this study.

Strains	Genotype	References
Salmonella enterica
GT853	hisO1242, hisC3737	Laboratory collection
GT5796	his-152, a deletion from the end of hisD to the beginning of hisI	[83]
GT6315	LT2/pKD46	Laboratory collection
GT6372	(TT17437) pNK2881 (miniTn10 tranposase helper plasmid)/his-644,serA790,lys-554	[82]
GT6374	Pool of 35000 colonies with random Tn10dTc insertions in GT6372	This study
GT6402	proL2231(G2A), hisO1242, his C3737, stm2220-2546::Tn10dTc,	This study
GT6408	mnmA1(W38stop), hisO1242, hisC3737,stm1254-2553::Tn10dTc	This study
GT6463	hisC10106, zdd-2532::cat, hisO1242	This study
GT6536	hisC10109, hisO1242	This study
GT6579	pSMP24/his-152	This study
GT6588	Pool (170000 colonies) of EZ-R6 gamma KAN, his-152, pSMP24)	This study
GT6795- GT6804,GT6806,GT6810	As GT6805 but with glnU alleles as shown in Table 4	This study
GT6805	glnU1538 (G4C), stm0672-2539::Tn10dTc, hisC3737, hisO1242	This study
GT6807	hisD10110, hisO1242, zdd-2532::cat	This study
GT6828	hisD10111, zdd-2532::cat, hisO1242	This study
GT6995	proK2236 (G added in AC), hisD10110, hisO1242, zdd-2532::cat	This study
GT7128	pKD46/hisD-2540::tetRA, zdd2532::cat, hisO1242	This study
GT7170	mnmA2(S33F), hisO1242, hisD10111,stm1221-2545::Tn10dTc	This study
GT7279	proM2219 (G31A), hisD10111, hisO1242, zdd-2532::cat, stm3930-2547::MudSacI	This study
GT7318	iscS56 (S184I), hisC3737, hisO1242, stm2545-2548::Tn10dTc	This study
GT7321	hisD10122, zdd-2532::cat, hisO1242	This study
GT7398	rpsI2 (deletion from R109 to the C-terminal end), stm3333-2543::Tn10dTc, hisD10122, zdd-2532::cat, hisO1242	This study
GT7432	tusE30 (K128stop), stm1091-2549::Tn10dTc, hisD10122, zdd-2532::cat	This study
GT7436	mnmE13 (del aa247-271), stm3848/3849-2542::Tn10dTc, hisD10122, zdd-2532::cat, hisO1242	This study
GT7440	mnmA3(G24D), hisD10122, stm1221-2545::Tn10dTc, zdd-2532::cat, hisO1242	This study
GT7453	tusB27, stm3453-2550::Tn10dTc, hisD10122, zdd-2532::cat, hisO1242	This study
GT7458	hisT10128 (deletion), stm2375-2552::Tn10dTc hisD10122, zdd-2532::cat, hisO1242	This study
GT7478	mnmG19 (gidA, 58 bp deletion from A402), stm3848/3849-2542::Tn10dTc, hisD10122, zdd-2532::cat, hisO1242	This study
GT7484	ybbB219 (G67R), sfbA-2537::MudSacI hisD10122, zdd-2532::cat, hisO1242	This study
GT7644	Deletion between tusD (A35) and tusC (S41), hisD10111, stm3453-2554::Tn10dTc, hisO1242	This study
GT7690	trmD39 (D150G), hisO1242, hisD10111, zdd-2532::cat	This study
GT7747	rpsI3 (deletion from E99 to the C-terminal end), stm3346-2551::Tn10dTc, hisD10122, zdd-2532::cat, hisO1242	This study
GT7775	proL2240, stm2235-2541::Tn10dTc, hisD10122, hisO1242, zdd-2532::cat	This study
GT7829	mnmG20 (gidA, G340stop) pstA2544::Tn10dTc, hisD10122, zdd-2532::cat, hisO1242	This study
GT7901	tusA32 (C19Y), hisD10122, hisO1242	This study
GT7988	proL2241 (G10A), hisO1242, hisD10111, zdd-2532::cat, zej-2555::Tn10dTc	This study
Escherichia coli
DH5alfa	fhuA2 Δ(argF-lacZ)U169 phoA glnV44 Φ80 Δ(lacZ)M15 gyrA96 recA1 relA1 endA1 thi-1 hsdR17	Laboratory collection
pNTR-SD-trmD	trmD under IPTG-inducible promoter	[54]
pNTR-SD-mnmA	mnmA under IPTG-inducible promoter	[54]
pNTR-SD-iscS	iscS under IPTG-inducible promoter	[54]

Genetic Procedures

Transduction with phage P22 HT105/1 (int-201) [45] was performed as previously described [44]. DNA sequencing was performed on chromosomal DNA or PCR products following the manual of Applied Biosystems ABI PRISM Cycle Sequencing Ready Reaction Kit Big Dye™.

Systems Used to Isolate +1 Frameshift Suppressor Mutants

We have used different +1 frameshift mutations in the hisC or the hisD genes (Table 2) constructed as described below. The hisC3737 mutation was used earlier to obtain several of the classical frameshift suppressor mutants [46] and apparently only very small amount of the HisC enzyme is required to enable a mutant to form colonies within a day or two without histidine in the growth medium. We also introduced other frameshift mutations at the same site as in hisC3737 to widen our possibilities to obtain various frameshift suppressor mutants. Several frameshift mutations in the hisD gene were constructed, since only 1% of the HisD enzyme is enough to make a cell His+ within a day [47]. Thus, only a fraction of a percent suppression of a frameshift mutation in the hisD gene is required to make enough of a functional HisD enzyme to allow a colony to appear within a few days. Monitoring suppression of a frameshift mutation in the hisD gene would be a sensitive way to detect mutations mediating very weak suppressor activity. Indeed, monitoring frameshifting as growth on a plate lacking histidine is a more sensitive way to monitor +1 frameshift suppression than monitor the suppression of the same +1 frameshift mutation in the lacZ gene which encodes β-galactosidase [36].

Table 2

Sequence of the various frameshifts sites in the his-operon used in the selection of 460 independent frameshift suppressor mutants.

Allele number	Sequence of the frameshift window
hisC3737	AUG-(NNN)124-GTA-GAG-(NNN)31-CCC-CAA-UAA
hisC10106	AUG-(NNN)124-GTA-GAG-(NNN)31-CCC-AUG- UAA
hisC10109	AUG-(NNN)124-GTA-GAG-(NNN)31-CCC-UGG- UAA
hisD10110	AUG-(NNN)4-CUG-AUU-GAC-UGG-AAC-AGC-UGU-CCC-UAU-UGA-ACA-GCA-G
hisD10111	AUG-(NNN)4-CUG-AUU-GAC-UGG-AAC-AGC-UGU-CCC-AAG-UGA-ACA-GCA-G
hisD10122	AUG-(NNN)4-CUG-AUU-GAC-UGG-AAC-AGC-UGU-CCC-CAA-UGA-ACA-GCA-G

1. The sequences of (NNN)124 and (NNN)31 in hisC3737, C10106 and C10107 are: agc act gaa aac act ctc agc gtc gct gac tta gcc cgt gaa aat gtc cgc aac ctg gta ccg tat cag tct gcc cgc cgt ctg ggc ggt aac ggc gat gtc tgg ctg aac gcg aat gaa ttc ccg aca gcg gtg gag ttt cag ctc acc caa caa acg ctt aac cgc tac ccg gaa tgc cag cca aag gcc gtg att gaa aac tac gcg caa tat gct ggc gta aag ccg gag cag gtg ctg gtc agc cgc ggc gcg gat gaa ggg atc gag ctg gtg atc cgc gcc ttc tgt gaa ccg ggg aaa gac gcc att ctc tac tgt ccg ccc act tac ggt atg tac agc gtc agc gcc gaa acc att ggc and: gta gag cgc cgg acg gtt ccc gcg ctt gaa aac tgg cag ctg gat cta cag ggg att tcc gac aac ctt gac ggc aca aaa gtg gtg ttc gtt tgt agc ccc caa taa [84], respectively.

2. The sequence of (NNN)4 in hisD10110, hisD10111 and hisD10122 is: AGC-UUC-AAU-ACC.

Constructions of Various +1 Frameshift Mutations in the hisC and hisD Genes

The frameshift mutation hisD10122 was constructed as follows: The tetracycline resistance genes tetA and tetR from Tn10dTc were first inserted into the hisD gene in strain GT6808 (zdd-2532::cat, hisO1242) generating strain GT7127 (hisD10132::tetRA, zdd-2532::cat, hisO1242) to which plasmid pKD46 from strain GT6315 (LT2, pKD46) was introduced resulting in strain GT7128 (pKD46/hisD10132::tetRA, zdd-2532::cat, hisO1242). This latter strain was transformed with a 60 nt DNA oligonucleotide designed to replace the tetracycline resistance cassette with the designed frameshift mutation selecting tetracycline-sensitive recombinants [48]; e.g. to construct the frameshifting site CCC-CAA-U present in hisD10122 mutant the codons 13–14 (AGC-CCU) of hisD were replaced by CCC-CAA-U. In order to produce a functional HisD protein from the mRNA of this mutant, the ribosome has to shift to the +1 reading frame before the UGA (stop) codon, which is in the zero frame and placed just after the CCC-CAA sequence. In hisD10122 a +1 shift occurs when is in the ribosomal P-site at the CCC codon resulting in a mutant peptide sequence (-Cys-Pro-Asn-Glu-). The hisD10110 and hisD10111 were constructed similarly by replacing the codons 13–14 (AGC-CCU) of hisD with the codons CCC-UAU-U and CCC-AAG-U, respectively, using 60 bp oligonucleotides with the mutated codons in the middle of the oligonucleotides. The complete frameshift windows used in this study are listed in Table 2.

The hisC3737 mutation is 31codons from the start codon and it creates a CCC-CAA- sequence upstream of the stop codon UAA in the zero frame (See Table 2). The sequence CCC-CAA of hisC3737 was replaced by CCC-AUG- and CCC-UGG in hisC10106 and hisC10109, respectively, by using the suicide plasmid pDM4 as described [49]. Two complementary 20-mers containing the desired mutation and two primers just outside the hisC gene, were used to generate by crossover PCR a fragment that was cloned into a T/A overhang vector. Then the entire hisC fragment with the mutation was cut out and ligated into the suicide vector pDM4, which contains the sacB gene, and cannot survive on plates with 5% sucrose. The construct was conjugated into S. enterica and a derivative, in which the integrated suicide vector had recombined out of the chromosome, were selected by adding 5% sucrose to the agar plates. Transconjugants surviving on plates with 5% sucrose were chosen and correct frame shift construction was confirmed by PCR and sequencing.

Mutagenesis to Obtain +1 Frameshift Suppressor Mutants

Mutagenesis of the strain GT6588 [pool of EZ-R6 gamma KAN, his-152 (deletion of the his-operon), pSMP24], which contains plasmid pSMP24 harboring dinB, was performed by inducing the expression of DinB [50], [51] from plasmid pSMP24 [52]. An over-night culture of strain GT6588 was diluted 2×106-fold and inoculated into 500μl of LB+100 µg carbenicillin (Cb)/ml +0.08% L-arabinose. After 24 hours of growth at 37°C, phage P22 was added to make phage lysates. The phage lysates were used to infect strains containing the different frame shifting sites and His+ clones were collected every day for nine days and saved for further analysis.

To mutagenize with hydroxylamine a phage P22 lysate prepared from strain GT6374 [pool of random Tn10dTc insertions in strain GT6372 (containing a deletion of the hisD and hisC genes (his-644), thus avoiding recombination with wild type his-operon in transductions)] was treated with hydroxylamine as described [53] until approximately 0.1 per cent infectious phage P22 particles remained. This lysate was used to transduce strains with a +1 frameshift mutation as described in Table 2.

Nitrosoguanidine (NG) induced mutations were obtained by placing a crystal of NG on a lawn of the donor strain with either a deletion of the his-operon or with the same +1 frameshift mutation as the recipient strain; e.g. hisD10122 on an agar plate, which was incubated over night at 37°C. Around the NG crystal a ring of growing bacteria emerged that contains bacteria with mutations induced by NG. Bacteria were scraped off from several fractions of the bacterial ring and resuspended in 1 ml of LB and allowed to grow for 1–2 hours before phage P22 was added to make lysates. As above the phage lysate was used to infect His- strain harboring a suitable +1 frameshift mutation in the his-operon and His+ clones were collected as above. To avoid siblings only one mutant from each phage stock was saved. To locate the extragenic +1 suppressor mutation in each His+ clone, a Tn10dTet was placed close to the mutation by using a phage P22 stock grown on a random pool of Tn10dTet in strain GT6374 as donor and the His+ clone as recipient. TetR clones were selected and His- clones were screened. These clones have most likely the +1 frameshift mutation exchanged by the wild type allele from the donor. Following verification that the Tn10dTet was close to the +1 frameshift suppressor mutation, the location of the Tn10dTet was determined by DNA sequencing directly on purified chromosome and with primers binding in the transposon and pointing outwards. The chromosome was purified by Qiagen Tip100/G as described by the manufacturer.

Complementation Analysis

A set of mobile plasmids containing most of the ORFs from E. coli with the expression controlled by Ptac/lacIq, was a kind gift from National Institute of Genetics, Mishima, Shizuoka 411–8540, Japan [54]. A plasmid, which contained the wild type copy of the structural gene for the potential mutated gene in the +1 frameshift suppressor mutant, was introduced to this mutant. The frameshift suppressor phenotype was scored as growth on plates lacking His and in several cases the modification of tRNA was established by HPLC. If the plasmid reversed the suppressor phenotype to the wild type phenotype (i. e from His+ to His-), the mutant was defective in the gene harbored on the plasmid. This was verified by determining the DNA sequence of the mutated gene on the chromosome.

Analysis of tRNA Levels

Strains were grown in 10 ml LB medium at 37°C to about 4×108 cells/ml. Following centrifugation the pellet was suspended in 1 ml of ice-cold water. Cells were collected by centrifugation and resuspended in 400 µl of 10 mM Tris-EDTA, pH 7.5. The same amount of acid phenol was added and the mixture was vigorously shaken for 10 sec, incubated for 45 min at 65°C with occasional shaking before the phases were separated by centrifugation. To the water phase 400 µl chloroform was added and the mixture was shaken after which the water phase was transferred to a clean test tube. The RNA was precipitated by adding 40 µl of 3M sodium acetate, pH 5.3 and 1 ml of 100% ethanol. The precipitated RNA was washed once with 70% ethanol, centrifuged, and dissolved in 50 µl of water. About 5 µg of RNA was applied to 8% polyacrylamide gel containing 8M Urea in 89 mM Tris-borate buffer pH 8.2 containing 2 mM EDTA. The gel was transferred to a Zeta probe membrane and the RNA was UV cross-linked to the membrane. The tRNAs were detected by Northern hybridization using radioactive oligonucleotides complementary to tRNAArg or .

Determination of Aminoacylation of in vivo

Cells were grown in 30 ml LB medium at 37°C to about 4×108 cells/ml and cells were collected by centrifugation. Cells were resuspended in 1 ml of water, washed once with 1 ml of water, and finally resuspended in 500 µl of cold 0.1 M NaAc (pH 4–5) containing 10 mM EDTA. To the suspension of cells, 200 µl of glass beads and 500 µl of 25:24:1 phenol-chloroform-isoamylalcohol mixture was added and the mixture was vortexed four times for one minute with a one minute on ice between the shakings. Following centrifugation, the supernatant was transferred to a new tube and RNA was precipitated by adding 3 volumes of ethanol. The RNA was dissolved in 50 µl of 10 mM NaAc pH 4.5 containing 1 mM EDTA. Half of the sample was diluted with equal volume of 0.5M Tris HCl, pH 9.0 for 20 min at 37°C. The deacylated and non-treated samples were run on an acidic gel containing 8% polyacrylamide, 8 M urea, 0.1 M NaAc pH 5.0. RNA was transferred to Zeta probe membrane and was detected as above.

Analysis of Modified Nucleosides in tRNA

Bacterial strains were grown over night in LB medium, diluted 100 times in 100 ml of the same medium and grown at 37°C to 100 Klett units (approximately 4×108 cells/ml). Cells were lysed and total RNA was prepared [55] and dissolved in 2 ml buffer R200 (10 mM Tris-H3PO4, pH 6.3, 15% ethanol, 200 mM KCl) and applied to a Nucleobond® AX500 column (Macherey-Nagel Gmbh & Co., Düren, Germany), pre-equilibrated with the same buffer. The column was washed once with 6 ml R200 and once with 2.5 ml R650 (same composition as R200, except for 650 mM KCl instead of 200 mM KCl). Finally, tRNA was eluted with 7 ml R650, precipitated by 0.7 volumes isopropanol, washed twice with 70% and dissolved in water. tRNA was digested to nucleosides by nuclease P1 followed by treatment with bacterial alkaline phosphatase at pH 8.3 [56]. The hydrolysate was analyzed as described earlier [57] using a Supelcosil C-18 column (Supelco) with a Waters Alliance HPLC system.

Determination of the Amino Acid Sequence of the Slippage Junction

To monitor ribosomal slippage and to purify the slippage product, a previously described system was used [58], [59]. It employs a fusion protein consisting of maltose-binding protein (MBP) fused to glutathione-S-transferase (GST) at its N-terminus and having six histidine residues (6×His) at its carboxy terminus (GST-MBP-6×His). The full-length GST-MBP-His6 fusion proteins were expressed from plasmid pUST290 (CCC-CAA-), pUST292 (UUU-CAA), pUST310 (CCC-CAA) or pUST311 (CCC-AAG). These plasmids were constructed by cloning a DNA fragment containing the frameshift sequence into the BamHI and EcoRI sites of vector pGHM57 [58]. Ligated plasmids were transformed into strain DH5α, analyzed by sequencing the insert, and retransformed by electroporation into different S. enterica strains. The fused GST-MBP-6xHis protein expressed from these plasmids were purified essentially as described by Atkins et al [58], except the Ni-NTA purification was omitted and the MBP-His6 part of the fusion was released by digestion with PreScission Protease (GE Healthcare), while the GST part was still bound to Glutathione-Sepharose. The MBP-His6 peptides were separated by SDS polyacrylamide (15%) gel electrophoresis and electroblotted to a Sequi-Blot PVDF membrane (Bio-Rad). The bands corresponding to the MBP-His6 peptides were excised from the membrane and subjected to N-terminal sequence analysis by Edman degradation. A +1 reading frame shift when tRNAPro is in the P-site at the CCC codon in pUST310 would result in the sequence GPLGILICPNDK. Unmodified cysteine is too reactive during N-terminal sequencing and is usually only seen indirectly as the absence of an amino acid in one cycle. The confirmation of the presence of cysteine has been described earlier [36].

Nomenclatural Acts

The electronic edition of this article conforms to the requirements of the amended International Code of Zoological Nomenclature, and hence the new names contained herein are available under that Code from the electronic edition of this article. This published work and the nomenclatural acts it contains have been registered in ZooBank, the online registration system for the ICZN. The ZooBank LSIDs (Life Science Identifiers) can be resolved and the associated information viewed through any standard web browser by appending the LSID to the prefix “http://zoobank.org/”. The LSID for this publication is: urn:lsid:zoobank.org:pub: XXXXXXX. The electronic edition of this work was published in a journal with an ISSN, and has been archived and is available from the following digital repositories: PubMed Central, LOCKSS [author to insert any additional repositories].

Results

1. Systems and Procedures Used to Isolate Many Independent +1 Frameshift Suppressor Mutants

According to our frameshift model [16], [36] the shift in frame occurs not by an error in the A-site as e.g. suggested by the quadruplet translocation model, but by an error in the P-site: i.e it is the peptidyl-tRNA that slips forward one nucleotide resulting in a +1 frameshift (Fig. 1). There are several ways that may induce a shift in frame (see Introduction). To extensively test the model in an unbiased way, we here present the characterization of many independently isolated mutants able to suppress various +1 frameshift mutations. These were, after the initial selection, subjected to a careful analysis of their frameshift suppressing phenotype. Such an analysis would reveal whether or not their frameshifting phenotypes were consistent with the model.

We have used different +1 frameshift mutations in the hisC and hisD genes (Table 2) to isolate extragenic +1 frameshift suppressors. As described in the Materials and Methods, monitoring frameshifting as growth on a plate lacking histidine is a very sensitive way to isolate weak +1 frameshift suppressor mutants allowing us to isolate a wide range of different +1 frameshift suppressor mutants and thereby extensively test our frameshift model. Furthermore, we placed the frameshift mutations (both the hisC and hisD derivatives) on the chromosome (not on a plasmid!) ensuring a “wild type balance” of various factors involved in reading frame maintenance. We feel this is important since overexpression of mRNA, as is the case if the test gene containing the frameshift mutation is residing on a plasmid, or unbalanced tRNA pools may induce translation errors [[60], [61]discussed by Atkins and Björk [9]]. Therefore, we expected these systems to be good tools to extensively test our model.

To isolate many independent frameshift suppressor mutants, a strain having a partial deletion of the his-operon (his-152) was mutagenized by overproduction from the plasmid pSMP24 (dinB) of DinB, which induces random mutations of various kinds [50]. Alternatively, we mutagenized cultures of strains harboring one of the indicated his-mutations or a his deletion by nitrosoguanine (NG). Phage P22 were grown on such cultures and used to infect strains having one of the his-mutations shown in Table 2. His+ transductants were selected at 37°C following several days of incubation to allow the appearance of weak suppressor mutants. Care was taken to avoid siblings by saving only one unique mutant from each phage stock. Thus, all mutants characterized (Table 3) are of independent origin even if the mutation resulted in the same nucleotide substitution. Next, we placed a Tn10dTc transposon close to each +1 frameshift suppressor mutation by crossing out the suppressor phenotype (the His+ phenotype of the suppressor mutant changed to the parent phenotype His- when the transposon is located close to the suppressor mutation). The location of the transposon on the chromosome was determined by DNA sequencing out from the transposon and into the nearby chromosomal region. To link the His+ phenotype with the mutated gene, we transduced it back to the parental strain (His-) by selecting TetR. Frequency of co-transduction between the transposon and the suppressor phenotype (His+) indicated which gene mediated the +1 frameshift suppressor phenotype. If DNA sequencing showed that the suspected gene contained a mutation, we introduced a plasmid harboring a wild type copy of the mutated gene to complement the mutation and thereby further demonstrate the link between the mutated gene and the +1 frameshift suppressor ability. In this way we obtained and characterized 467 independent mutants harboring an extragenic suppressor to the different +1 frameshift mutations in the his-operon. These 467+1 frameshift suppressor mutations present in the mutants were distributed in 16 different loci (Table 3).

Table 3

Summary of all mutants selected as suppressors to various frameshift mutations in the his-operona.

Gene mutated	His mutationused	No of mutants obtained	Molecules affected	Comments	Mechanism of frameshifting (See Fig. 1)
mnmA	D10122	39 (24b)	Synthesis of mnm5s2U34	Induces s2-deficiency of mnm5s2U34	Alt. C in Fig. 1
----« ----	C3737	1	----« ----	----« ----	----« ----
----« ----	D10111	1	----« ----	----« ----	----« ----
tusA	D10122	2	----« ----	----« ----	----« ----
tusDCB	D10122	15	----« ----	–– « –----	----« ----
----« ----	D10111	1	––« ----	––« ––	----« ----
tusE	D10122	1	----« ----	----« ----	----« ----
iscS	C3737	7	----« ----	----« ----	----« ----
mnmE	D10122	2	----« ----	Induces lack of mnm5-sidechain of mnm5s2U34	----« ----
gidA	D10122	1	----« ----	----« ----	----« ----
–« –	D10111	2	----« ----	----« ----	----« ----
ybbB	D10122	1	Adds a geranyl group to the s2-group of mnm5s2U34	Results in decreased level of charged	----« ----
hisT	D10122	10 (7b)	Synthesis of Ψ at postion 38, 39 and 40 i some tRNAs	Induces lack of Ψ in e.g.	----« ----
glnU	D10122	93 (82b)	Alters thestructure of	Induces reduced level of charged	----« ----
----« ----	C3737	13	----« ----	----« ----	----« ----
glnS	D10122	1	Alters the structure of GlnRS	––« ––	----« ----
proL	D10122	85b	Alters the structure of or delete	Induces deficiencyof Pro-	Alt A in Fig. 1
----« ----	C3737	21 (3b)	----« ----	----« ----	----« ----
----« ----	C10106	57	----« ----	----« ----	----« ----
----« ----	D10110	9	----« ----	----« ----	----« ----
----« ----	D10111	38b	----« ----	----« ----	----« ----
	C10109	43			----« ----
proM	D10111	1		Induces a structural alteration of	Alt B in Fig. 1
proK	D10110	2		Induces structural alterations in	Alt A and B in Fig. 1
trmD	C3737	2	Alters the tRNA(m1G37) methyltransferase	Results in m1G37 deficiency in e.g. all three proline tRNAs	Alt B in Fig. 1
----« ----	D10110	1	----« ----	----« ----	----« ----
----« ----	D10111	16 (13b)	----« ----	----« ----	----« ----
rpsI	D10122	2	Ribosomal protein S9	Results in C-terminal truncated version of ribosomal protein S9	Changed P-site environment (See Fig. 6.)
		Total no. of mutants : 467

a)The various his-alleles used were: hisD3737 (CCC-CAA), hisC10106 (CCC-AUG), hisC10109 (CCC-UGG), hisD10110 (CCC-UAU), hisD10111 (CCC-AAG), or hisD10122 (CCC-CAA).

b)These mutations were not sequenced but localized by transduction to a transposon closely linked to the indicated gene. The linkage between the transposon and the mutation was consistent with the mutation being in the indicated gene.

2. Alterations of the Primary Sequence of (106 mutants) or an Alteration of the Gln-tRNA Synthetase (One Mutant) Induce Low Concentration of Charged Gln-, which causes Slow Entry into the A-site and thereby Allowing a +1 Frameshift in the P-site

A glutamine codon is present in two of the six frameshift sites used (Table 2). We therefore expected mutations influencing the activity of and indeed this was the case.

We obtained 93 mutants as extragenic suppressors in the glnU gene to the hisD10122 mutation based on their linkage to a transposon close to the structural gene (glnU) for . Of these 11 were verified by determination of the glnU sequence. We also obtained 13 mutants as extragenic suppressors to hisC3737, which were sequenced and further analyzed (Table 4, Fig. 2). Three of these mutants displayed a temperature sensitive phenotype (glnU1529-30, 1538), nine (glnU1526-28; 1531-33;1535-37) were cold sensitive, and one mutant (glnU1537) had a reduced growth which was similar at all three temperatures tested (Table 4). According to our model (Fig. 1), we suspected that alterations of or a defect of Glu-tRNA synthetase should reduce the level of charged Gln-. Transfer RNA was prepared from wild type and from the various mutants under conditions which preserve the aminoacylation of tRNA [62]. Although there was no difference in the relative level of glutaminyl-tRNA in the mutants compared to tRNA from the wild type (Fig. 2), a reduced level of relative to tRNAArg was observed in the mutants. We conclude that the alterations in all glnU mutants did not affect the charging of , but made the tRNA more unstable resulting in a lower concentration of the Gln- than in the wild type mediating +1 frameshifting consistent with our model.

Table 4

Growth and suppressor ability of mutants with structural changes in .

Mutants(allele number)	No. of indep.glnU mut.	Mutations	Efficiency of suppressiona)(E+glu/E+glu+His)	TYSb) 30 °C(2 days)	TYSb) 37 °C(1 day)	TYSb) 42.5 °C(1 day)	Growth Phenotypec)
1537	1	T1C	0.2	0.8	0.7	0.8	Similar reduction at all temp.
1529, 1530	2	G4T	0.1	0.9	1.1	0.7	Ts
1538	1	G5C	0.6	0.8	0.7	0.5	Ts
1526-1528	3	G52A	0.7-1.1	0.3r	0.4	0.6	Cs
1533, 1535-1537	4	G53A	0.3	0.6	0.6	0.9	Cs
1531-1532	2	G53T	0.3	0.6	0.7	0.9	Cs
WT			0	1.0	1.0	1.0

a)Figures represent the relative colony size of the mutant on minimal glucose plates without histidine after 3 days of incubation at 37°C to the colony size on plates with histidine at the same temperature. Thus, this measurement is an estimation of suppression efficiency corrected for the general growth reduction of the mutant. Ts, temperature sensitive growth phenotype and Cs, cold sensitive growth phenotype.

b)Figures represent colony size relative to the size of wild type control on rich plates (TYS) at indicated temperatures and time of incubation. The colony size of the wild type was 3.2, 2.2, and 2.7 mm at 30, 37 and 42,5°C, respectively.

c) Cs, Cold sensitive; Ts, temperature sensitive.

Figure 2

Sequence and aminoacylation levels in vivo of various mutant :s.

The positions of charged (ch) Gln or Arg-tRNA and uncharged (unch) Gln-tRNA are indicated and their migration pattern was obtained from control experiments. The position of uncharged Arg-tRNA is between Gln-ch and Arg-ch as shown by a control experiment. Since Arg-tRNA was 100% charged the uncharged Arg-tRNA is not indicated in the figure. Sequence of wild type glnU and various mutants (base alteration shown in red). s4U, 4-thiouridine, #, 2′-O-methylguanosine (Gm), D, dihydrouridine, J, 2′-O-methyluridine (Um), N, 5.-carboxymethylaminomethyl-2-thiouridine (cmnm5s2U), m2A, 2-methyladenosine, P, pseudouridine (Ψ), T, 5-methyluridine (m5U).

Two mutants, glnU1538 (G5C) and glnU1531 (G53T) were chosen to determine the frameshift event at the site of the hisC3737 mutation. For that purpose the plasmid pUST290 was constructed (Fig. 3). The frameshift sequence was inserted between the genes encoding glutathione-S-transferase (GST) and maltose-binding protein (MBP, encoded by the malE gene) with six histidine residues (6×His) at the carboxy terminus in the gst-malE fusion gene. malE is in the +1 frame relative to gst, explaining why the complete GST-MBP-6×His fusion protein is only synthesized when a +1 frameshift occurs. If +1 frameshifting does not occur, translation terminates at the UAA stop codon present downstream of the gst gene and only GST is produced (Fig. 3). The complete fusion protein was purified from strains containing plasmid pUST290 and glnU1531 or glnU1538 mutations using the GST and 6×His affinity tags. To liberate the slippage junction fused to the MBP-6×His, the frameshift product was treated with PreScission Protease. This protease cuts the protein at the specific protease site between the GST moiety and the rest of the peptide. The N-terminus of the slippage junction fused to MBP-6×His was sequenced. From both mutants the first 15 amino acids of the peptide were determined as GPLGILNP-KANNSQL, where P (proline) was the last amino acid inserted in 0 frame suggesting that the frameshifting tRNA at the frameshift site CCC-CAA-UGA in hisC3737 was a wild type pro-tRNA and not the altered.

Figure 3

Amino acid sequence of the frameshift product encoded from plasmids pUST290, pUST292, pUST310, and pUST311.

The frameshift window, within which the frameshift must occur, is bordered by the stop codon UAA (italics and underlined) in +1 frame and the stop codon UGA UAA in the zero frame (Indicated by a * below the DNA sequence). P or F (in red) denote the last amino acid decoded in the zero frame found in the frameshift product.

In order to analyze the influence the P-site tRNA exerts on the frameshifting event we also constructed a plasmid pUST292 with UUU (Phe) instead of the CCC (Pro) codon (Fig. 3). The sequence of this frameshift peptide revealed that it was the wild type in the P-site that caused the frameshifting event (Fig. 3). Thus, in both cases low concentration of the Gln- caused the wild type peptidyl-tRNA (Pro or Phe) to slip forward one nucleotide and thereby moving the ribosome into the zero frame. Since both wild type Pro- and Phe-peptidyl tRNA, which interact with two different codons in the P-site were induced to slip by a ribosomal pause, the identity of the last amino acid in the peptiyl-tRNA and the anticodon-codon interaction in the P-site is not critical. Thus, the frameshift phenotype of these mutants was consistent with our model (Fig. 1, alt. C).

Reduced charging capacity may also occur if the Gln-tRNA synthetase (GlnS) is defective. Indeed we obtained a GlnS mutant with an alteration (N70S) changing the environment where the CCA-end of binds to GlnS during the glutaminylation reaction [63]. Since this is an essential gene it was not surprising that we only obtained one mutant.

3. Deficiency of the Wobble Nucleoside cmnm5s2U in causes a +1 Frameshift in the P-site (72 Independently Isolated Mutants)

The first step in the synthesis of the side chain present at position 5 of wobble nucleoside (c)mnm5s2U34, which is present in tRNAs specific for Gln, Lys and Glu, is catalyzed by a heterodimer of MnmG (earlier denoted GidA) and MnmE proteins [64] (Fig. 4). This reaction generates the cmnm5-side chain in the presence of glycine or nm5-side chain in the presence of ammonia. The MnmC1 activity of MnmC (MnmC enzyme contains two activities, C1 and C2 [65]) converts the cmnm5-group to an nm5-group which in turn is converted to the mnm5-side chain by the MnmC2 methyltransferase activity. The cmnm5-side chain is present in a subset of whereas and chains contain only the mnm5-side chain. Therefore, the synthesis of the mnm5-side chain depends on four enzymatic activities and any alterations of these proteins encoded by the mnmE, mnmG and mnmC genes might change the extent of modification of the wobble nucleoside (c)mnm5s2U34 and thereby inducing inefficient decoding.

Figure 4

Schematic picture of the synthesis of (c)mnm5s2U34, mnm5ges2U34, and se2(c)mnm5U.

(“ge” is a geranylgroup abbreviated “ge”; GPP is geranylpyrophosphate). The sulfur relay from Cys to the s2-group of the nucleoside is shown in red and the different enzymes involved in the synthesis of these thiolated derivatives are shown in green denoted as protein with their genetic symbols starting with a capital letter. A geranylgroup from GPP is transferred to cmnm5s2U of by YbbB to generate the hypermodified ges2cmnm5U34 [69] and to mnm5s2U of Lys- and Glu-tRNA to generate ges2 mnm5U [77]. YbbB is also responsible for the exchange of s2 by Se forming mnm5Se2U if selenium phosphate is available [89].

The first step in the synthesis of the s2-group, also present in mnm5s2U, is catalyzed by the cysteine desulfurase IscS, whose activity is required for the synthesis of all thiolated nucleosides in bacteria [66], [67]. The IscS delivers persulfide sulfur from Cys to TusA, which in turn transfers the sulfur to tRNA in a sulfur relay system consisting of the TusBCDE complex and finally delivers the sulfur to the tRNA by MnmA [68]. Thus, the formation of the s2-group depends on seven proteins (IscS-TusA-TusECDE-MnmA) and alterations in any of these proteins should reduce the formation of the s2-group of (c)mnm5s2U34. Deficiency of the s2-group should negatively influence the coding capacity of the three tRNAs having (c)mnm5s2U34 as wobble nucleoside.

Of the 467 extragenic +1 frameshift suppressor mutants isolated 72 abolished, or reduced, the synthesis of (c)mnm5s2U34. This large fraction of this kind of mutants depends on the fact that 10 genes are the targets for mutations reducing the synthesis of the (c)mnm5s2U34. Several of these mutants were analyzed for the level of (c)mnm5s2U in their tRNA. Both the frameshifting phenotype and the reduced level of (c)mnm5s2U in the tRNA were returned to that of the wild type by introducing a complementing plasmid (Table 5). According to our model, reduced activity of Gln- due to deficiency of the modified nucleoside should induce a shift in frame by the peptidyl-Pro-tRNA and indeed this is the case [16]. Moreover, the entry of , which also contains the wobble nucleoside mnm5s2U, to its cognate codon AAG in the A-site should also be reduced. We therefore determined the sequence of the frameshift peptide using plasmids pUST310 (CCC-CAA(Gln)) or pUST311(CCC-AAG(Lys)) which should monitor the slippage of peptidyl-Pro-tRNA upon slow entry of and , respectively (Fig. 3). The amino acid sequences of the frameshift peptide for two different mnmA mutants (lacking the s2-group) and one mnmE mutant (lacking the mnm5-sidechain) were all consistent with a frameshift error occurring at the sequence CCC-CAA or CCC-AAG by peptidyl-Pro-tRNA (Table 5). Thus, we conclude that the frameshifting phenotype of these 72 mutants lacking (c)mnm5s2U34 is consistent with our proposed model (Fig. 1, alt. C).

Table 5

Analysis of some typical mutations in genes inducing suppression of frameshift mutations.

Locus	Site used atselection	Alteration	mnm5s2U(% of wt)	Suppression		Complementation		P-site	Peptide (c)
				Growth withoutHis (a)	Rel b-gal(b)	FS	Rel β-gal
mnmA3	D10122	G24D	<3	Yes	4.4	Yes	90	Yesh	p310(P)
mnmA2	D10111	F35S	<3	Yes	2.39	Yes	nd	Yesh	p311(P)
iscS56	C3737	S184I	38	Yes	nd	Yes	102	Yesi
tusDCB (B27)	D10122	Q31stop	3	Yes	3.95	Yes	95	Yesi
tusCD(CD33)	D10111	deletion	nd	Yes	nd	nd	nd
tusE30	D10122	K128stop	<3	Yes	4.24	Yes	73	Yesi
tusA32	D10122	C19Y	3	Yes	nd	Yes	104	Yesi
mnmE13	D10122	Codon 247-271 deleted	5	Yes	1.44	Yes	88	Yesh	p310 (P)
mnmG1 (gidA)	D10122	58 nt deletion from A402	5	Yes	1.5	Yes	100	Yesj
mnmG2	D10111	G340stop	<3	Yes	1.87	Yes	111	Yesj
hisT	D10122	deletion	Not rel	yes	Nd.	Nd.	nd	Yesk
proL2240	D10122	A G added in AC	Not rel	Yes	2.66	Not rel	Not rel	Yese
proL2231	C3737	G2A		Yes	nd	“	“	Yese
proL2241	D10111	G10A		Yes	nd	“	“	Yese
proK2236	D10110	G added in AC		Yes	nd	“	“	Yesd
proM2219	D10111	G31A		Yes	1.78	“	“	Yesd	p290(P)f
trmD39	D10111	D150G	16 (m1G)	Yes	1.91	Yes	95 (m1G)	Yese	p310(P); p311(F), p311 (P)
glnU1538	C3737	G5C	Not rel	Yes	nd	Not rel	Not rel	Yes	p290(P); p292 (F)
glnS1544	D10122	N70S	Not rel	Yes	nd	Yes	Not rel.	nd	nd
rpsI2	D10122	20 aa shorter	Not rel	Yes	2.86f	Yes	Not rel.	Yesf	p290(P)f; p292 (F)f; p310 (Pro)f
rpsI3	D10122	33 aa shorter	Not rel	Yes	3.86f	Yes	Not rel.	Yesf	p290(P)f; p292 (F)f; p310 (Pro)f
ybbB181		G67R	Reduced/newmodification	Yes	nd	No, ybbB181 is dominant		Yesg	p290 (P)g

a)Monitored as the ability to suppress the his-allele the mutant was selected to suppress. Growth of mutants on a plate lacking His following and incubation at 37°C for 4–6 days. The parental strain, which has no suppressor mutation but the indicated his-allele, did not grow on plates without His.

b)The suppression was monitored as the ability to suppress the CCC-CAA-UAG sequence placed in front of the lacZ gene (See M–M).

c)Plasmids (See figure 4) used to determine the amino acid sequence at the frameshifting site and the last amino acid in the zero frame is indicated in parenthesis.

d)P-site according to Qian et al 1998 [34].

e)P-site according to [35].

f)According to [36].

g)According to [69].

h)According to [16].

i)P-site since these mutants also lack the s2-group of mnm5s2U similar to the mnmA mutants.

j)P-site since mnmG mutants like mnmE mutants lack the mnm5-side chain of mnm5s2U.

k)According to [71].

pUST136: contains the metT operon in which glnU is present. It also contains the gene miaB. See Esberg et al 1999 [85].

pCBS4 (glnS) contains the glnS wild type allele.

4. Geranylation of (c)mnm5s2U34 Results in a Decreased Charging of (c)mnm5s2U34 Containing tRNAs and thereby Inducing a +1 Frameshift Phenotype (One Mutant)

One mutant was found to have an altered YbbB protein (G67R). The mutation is dominant and it induces the ability of the altered YbbB protein to add a geranyl-group (a C10H17-fragment abbreviated “ge”) to the sulfur of the wobble nucleoside cmnm5s2U34 of tRNAs specific for Gln [69], [70]. This generates the presence of mnm5ges2U34 in a fraction of which in turn reduces the level of glutaminylated . Apparently, only certain amino acid substitutions induce this activity explaining that we only found one mutant among the 467+1 frameshift mutants isolated. Interestingly, the alteration of YbbB found here (ybbB181,G67R) is an amino acid substitution at the same position of YbbB as a mutant (denoted ybbB204,G67E) isolated in 1966 and earlier characterized by us [69]. In the case of this alteration results in a decreased level of charged [69] nicely explaining its ability to induce +1 frameshifting. A reduced level of charged induces a pause and allows the peptidyl-Pro- to shift frame. The resulting frameshift peptide is consistent with this interpretation [69]. Thus, the frameshifting phenotype of the YbbB (G67R) mutant was found to be consistent with the proposed model (Fig. 1, alt C).

5. Deficiency of Ψ38 of Induces +1 Frameshifts (10 Independent Mutants)

Pseudouridine (Ψ) is present in the anticodon loop and stem in positions 38, 39, and 40 in several tRNA species. The has Ψ in position 38 and , which reads the CCC codon, has Ψ40. Whereas deficiency of Ψ in position 38 reduces the rate of A-site selection of all :s which all have Ψ38, deficiency of Ψ40 of does not [71] (Reviewed in [72]). Such reduced rate of A-site selection results in a frameshift in the P-site [71]. Therefore, Ψ38 deficient enters the A-site slowly resulting in a ribosomal pause and thereby allowing the (most likely the ) in the P-site to shift frame according to our model. We characterized 10 hisT mutants and found that their frameshifting phenotype is consistent with our model (Fig. 1, alt. C).

6. Alterations in the Activity of the Three tRNAPro :s Induce +1 Frameshifts (253 proL, 1 proM and 2 proK Mutants)

The four proline codons are read by proL (), proM () and proK () and their coding capacities are shown in Figure 5. The proM reads all four proline codons and is the only tRNAPro that read CCA [73]. Accordingly, the proM tRNA is essential for viability and no frameshift suppressor mutant has earlier been isolated as having an altered proM tRNA. The proL has anticodon GGG and reads the codons CCC and CCU and the proK with its anticodon CGG reads only CCG. The classical dominant +1 frameshift suppressors are derivatives of proL (sufB2) and of proK (sufA6). Both these frameshift suppressors have an extra base inserted in the anticodon loop [34], [74]. We isolated 253+1 frameshift suppressor mutants, which were in some way defective in the synthesis or activity of proL (Table 5). This large amount of proL mutants was expected, since the proL gene, is not essential for viability and deletion of this gene induces +1 frameshifting [75]. Table 6 shows that deletions, duplications, base substitutions and promoter mutations were obtained. Only three mutants (two in proK and one in proM) were obtained that affected the other two tRNAPro:s. Since the proM is essential we did not expect many mutants defective in this gene especially as no +1 frameshift mutant has earlier been characterized (See Discussion). However, the proK is not essential [73] and we expected an equally large amount of mutations in this gene as in proL. However, this was not the case and moreover, the two independently isolated proK mutants have an insertion of a G in the anticodon similar to the classical sufA6 tRNAPro [34]. A deletion of the proK gene does not induce +1 frameshifts of either the hisD10122 nor the hisC3737 mutations ([76] and unpublished results). The small number of proK mutants suggests that only specific alterations of the proK gene induce frameshifting and this aspect is discussed below (See Discussion).

Figure 5

Modified nucleosides in positions 32, 34, 37, and 38–40 and the coding capacities of the corresponding tRNAs.

In the proline coding box there are three tRNAs reading the four proline codons and they are encoded by proK, proL, and proM (One copy of each gene is present in Salmonella). proM tRNA has cmo5U34 as wobble base and decode all four proline codons [73]. A circle corresponds to a codon read by a tRNA and the line between circles denotes that the same tRNA read those codons. Note also that the proM tRNA is essential, since it is the only tRNA reading the CCA codon. The proL tRNA having G34 as wobble nucleoside reads U and C ending codons and proK tRNA, which has C34 as wobble nucleoside, should read only CCG codon. The Gln codons CAA/G are read by two tRNAs having mnm5s2U34 and C34 as their wobble nucleoside. The C34 containing tRNA reads only CAG whereas the mnm5s2U containing tRNA (glnU tRNA) decodes both CAA and CAG although less efficient CAG (Unfilled circle). Note that the latter tRNA (glnU tRNA) is essential, since it is the only tRNA reading the CAA codon. In the Lys and Glu codon boxes one tRNA having mnm5s2U as wobble nucleoside reads AAA (Lys)/GAA (Gln) and less efficient AAG (Lys)/GAG (Glu) (Unfilled circle).

Table 6

+1 frameshift suppressor mutants lacking or with defects in the proL .

His-alleles used for selection		C3737	C10106	D10110	C10109	D10122	D10111
Mutations	Alterations in tRNA regions	ccc- caa	ccc- aug	ccc-uau	ccc-ugg	ccc- caa	ccc-aag
Not sequenceda)	N/D	3				85	38	126
proL::Tn10	N/R	11						11
proL::EZ	N/R		44		5			49
G2A	AA-stem	1						1
G2A, G-2A	”	1						1
G7A	”	1						1
G72A	”	1						1
G53A	TΨ-loop	1						1
G10A	D-stem	1			8			9
C11U	D-stem		1					1
G15A	D-loop				1			1
G19U	D-loop			2				2
G20A	D-loop				1			1
dupl G42-C48	AC-stem		2					2
dupl G36-C42 (U39-G44)	AC-loop and and stem		1					1
del G40-G46(G45-G51)	AC-stem		1					1
del U40	AC-stem			1				1
G67U	AA-stem			1				1
delG36-C42	AC-stem			4				4
delG39-G45	AC-stem				4			4
G29A	AC-stem				1			1
dupl G44-G50	AC-stem				1			1
G36A	AC				1			1
extra G in the anticodon	AC	1		1				2
del G in anticodon	AC		1					1
del G35-C41	AC-loop		7		20			27
promoter mutation −35					1			1
								0
Total		21	57	9	43	85	38	253

a)These mutations were not sequenced but located by transduction with a transposon closely linked to the indicated gene. The linkage between the transposon and the mutation was consistent with it being in the proL gene.

The 256 characterized mutations altering a proline tRNA induce +1 frameshift errors. For proL mutants it has been shown earlier that the frameshift occurs in the P-site [35] and this is the case also for mutants in proK [34] and in proM [36]. Thus, the frameshifting phenotypes of all these 256 mutants defective in any of the three tRNAPro are all consistent with the frameshifting model [Fig. 1, Alt. A (proL and proK) and B (proK and proM)].

7. m1G37 Deficiency Induces +1 Frameshift in the P-site (19 Mutants)

The trmD gene codes for the enzyme (tRNA(m1G37)methyltransferase, which synthesizes m1G37 in all proline tRNAs, all leucine tRNAs reading the CNN codons, and the arginine tRNA reading codon CGG. We obtained 19 trmD mutants of which 6 were sequenced and tested for the level of m1G in their tRNAs. As expected, very low levels of m1G were present in their tRNA (Table 6). Lack of m1G37 was the first modification deficiency shown to induce frameshift errors [18] and such deficiency induces frameshift errors in the P-site [35] consistent with our model (Fig. 1, alt. B).

8. Physical Alterations in the Ribosomal P-site Induce +1 Frameshifts (Two Mutants)

Alterations of the ribosomal P-site might also induce +1 frameshifts if the ribosomal grip of the peptidyl-tRNA is weakened. The C-terminal end of ribosomal protein S9 penetrates the ribosome like a tentacle and the two last amino acids make a contact with the 5′ phosphate of nucleotide 32 (R130) and the 5′-phosphates of positions 33 and 34 (K129) of peptidyl-tRNA (Fig. 6; [6]). Thus, ribosomal protein S9 might be an important feature of the ribosomal grip of the peptidyl-tRNA in order to maintain the reading frame. Indeed, two of the 467 independently isolated +1 frameshift mutants (rpsI2 and 3) had a 20 amino acids or a 33 amino acids, respectively, truncated C-terminal of ribosomal protein S9. Analysis of these mutants as well as two mutants isolated by direct substitution of amino acid R130 and K129 revealed that the frameshift occurred in the P-site as shown both by peptide sequencing of the frameshift product and by reduced frameshift by overexpression of the aa-tRNA predicted to read the A-site codon [36]. The unexpected isolation of these two +1 frameshift mutants having a defective ribosomal protein S9 among all our 467 independently isolated +1 frameshift suppressor mutants strongly support the fundamental importance of the ribosomal P-site in maintaining the reading frame.

Figure 6

The anticodon loop of the peptidyl-tRNA and the extreme C-terminal end of ribosomal protein S9.

The anticodon of the peptidyl-tRNA is labeled blue, the C-terminal Arg130 of S9 is in purple and Lys129 is in orange. The arrow points to the 5′ phosphate of the wobble nucleotide pC34. The dashed line indicates a possible H-bond between the phosphate of pC34 and the amino group of Lys129 [6]. The figure is adopted from [36] with permission.

Discussion

Maintaining the reading frame is a vital feature of translation in all organisms. Here we extensively test a model for how +1 frameshift errors may occur (Fig. 1). A key feature of the model is the critical role of interactions between constituents of the ribosomal P-site and the peptidyl-tRNA in maintaining the reading frame. If a ternary complex consisting of aa-tRNA, EF-Tu and GTP, is slow reading the codon in the A-site, the probability of destructions of interactions between the peptidyl-tRNA and some key components of the ribosomal P-site increases and a frameshift error may occur by the peptidyl-tRNA. We have characterized many (467) independently isolated mutants able to suppress a +1 frameshift mutation; i.e mutants with defects in maintaining the reading frame. Analyses of the frameshifting phenotype of all these mutants can be explained by our model. The mutants were defective in 16 different loci of which 15 in various ways reduced the activity of a tRNA and thereby changed either the rate with which the ternary complex enters the A-site or its interaction as part of the peptidyl-tRNA with some P-site component(s). The model also predicts that some alterations of the P-site environment might mediate a slippage of wild type peptidyl-tRNA. Indeed, we obtained two such +1 frameshifting mutants which possessed an altered ribosomal protein S9, whose C-terminal reaches into the P-site and interacts with the anticodon of the peptidyl-tRNA (Fig. 6). The fact that we obtained these S9 mutants as able to suppress +1 frameshift mutations is a strong support for the pivotal role of the P-site in maintaining the reading frame.

At certain frameshifting sites (Table 2) the glutamine codon CAA was present. This codon is read by encoded by the glnU gene, which is found in only one copy in Salmonella. It is thus essential for viability. Using such sites to select for frameshift suppressor mutants, we expected to find only mutants with a reduced level, charging, or stability of this tRNA, but no deletion of its only structural gene glnU. This was indeed the case and we obtained 106 mutants of which we sequenced 23 and analyzed 12 in detail (Fig. 2; Table 3 and 4). Using the two frameshift mutations hisC3737 and hisD10122, both having the frameshift site CCC-CAA, these kinds of mutants were frequent, suggesting that deficiency of a fully active results in efficient frameshifting, explaining the ease with which we obtained them. The 12 mutants analyzed in detail were either temperature or cold sensitive. All of them charged the efficiently, but the level of Gln- was decreased due to instability of the tRNA (Fig. 2). According to our model a reduced availability of Gln- should induce a shift in frame by tRNAPro in the P-site. Indeed this was shown by sequencing the frameshift product and the expected amino acid was consistent with the tRNAPro in the P-site having shifted frame (Fig. 3, plasmid pUST290). Moreover, to show that a lower level of could also induce another peptidyl-tRNA to shift frame, we determined the frameshift product of a UUU-CAA site (Fig. 3, plasmid pUST292). Such an analysis showed that the tRNAPhe shifted frame. Thus, we conclude that the frameshift phenotype of all these glnU mutants is consistent with our model (Fig. 1). The is charged by Gln-tRNA synthetase (GlnRS), which is encoded by the glnS gene. Defective GlnRS results in reduced charging of but we expected to find only a few mutations in this gene since it is essential explaining why we find only one such mutant.

The and have as wobble nucleoside (c)mnm5s2U34, the complex synthesis of which is shown in Figure 4. Neither the s2- nor the (c)mnm5-group are essential for growth although deficiency of any of them severely reduces the growth. We have earlier shown that lack of this wobble modification induces +1 frameshifting [16]. Since synthesis of this modification requires as many as 10 genes, we expected many mutants defective in the synthesis of (c)mnm5s2U as was the case. The 72 independently isolated mutants were obtained using either the hisD10122/C3737 (CCC-CAA) or the hisD10111 (CCC-AAG) frameshift mutations. Deficiency of the s2-group or the mnm5-group induces frameshifting irrespectively of which gene involved in their synthesis is affected. This shows that it is the undermodified tRNA that is responsible for the frameshift phenotype and not lack of any of the biosynthetic proteins involved in the synthesis of these modifications. Determination of the frameshift products encoded both at a CCC-CAA and CCC-AAG site, showed that it was the P-site tRNAPro that slipped into the +1 frame (Fig. 3; pUST310 and pUST311; Table 6). Thus, these 72 independently isolated mutants defective in the synthesis of mnm5s2U induce a +1 frameshift by peptidyl-tRNA slippage caused by slow entry of the mnm5s2U34 deficient tRNA specific for Gln or Lys consistent with the model presented in Figure 1 (Alt. C).

We also obtained one mutant with an amino acid alteration at position 67 of the YbbB protein and such alteration increases the activity of the YbbB protein to transfer a geranyl (“ge”) group to the s2-group of cmnm5s2U in generating a ges2cmnm5U hypermodified [69], [70]. This hypermodification decreases the glutaminylation of the geranylated [69], [77]. As the sequence of the trans-frame encoded peptide revealed, it induces +1 frameshifting in the P-site [69]. Such alteration of the YbbB protein also mediates geranylation of the Glu- and Lys-tRNA, which contain the mnm5s2U as wobble nucleoside [77]. Unlike the hypermodified Gln-tRNA, the hypermodified tRNALys and tRNAGlu are aminoacylated to the same level as the respective wild type tRNA and still a +1 frameshift occurs at a +1 frameshift mutation containing lysine codons [77]. Since the frameshift peptide was not established it is not known which tRNA makes the frameshift error. However, a ternary complex having a tRNA with such a large hydrophobic compound as part of the wobble nucleoside is not likely to be efficiently accepted, if at all, in the A-site. This causes a ribosomal pause and induces the peptidyl-tRNA to make a +1 frameshift error. Thus, the +1 frameshifting induced by geranylated Lys-tRNA may be consistent with our model (Fig. 1 alt C).

The proL gene is not essential for viability and deletion of this gene also mediates +1 frameshift suppression [36], [75]. Therefore, we expected to obtain many mutations in the proL gene, as we indeed did (Table 3). Since we obtained deletions, duplications, promoter mutations as well as various base substitutions in this gene, it appears that any alteration that reduces the activity of mediated +1 frameshifting (Table 5) consistent with the observation that a deletion of the proL gene induces +1 frameshifting. Note, that one of the proL mutations had an extra G in the anticodon and thus was identical to the classical sufB2 mutation obtained in 1970 [46], [74]. Genetically it is possible to remove the cmo5U modification, which is only present in the proM among the tRNAPro:s. Such manipulation reduces, by almost 100%, the proL mediated +1 frameshift suppression, demonstrating that it is the wild type proM that makes the frameshift error and not the altered proL [34]. Although is able to read the CCC codon [73], its interaction with the near-cognate codon CCC in the P-site may not be optimal thus inducing a +1 slippage upon a ribosomal pause. Since the frameshifting event occurs in the P-site [35], the many mutants obtained with defects in the proL gene is consistent with our model (Fig. 1, alt A).

The proM is essential for growth and no alterations of this tRNA have been described earlier. We therefore did not expect many mutants with altered proM . The one we obtained (G31A) disrupted the last base-pair of the anticodon stem creating a 9 member anticodon loop. Using localized mutagenesis we have isolated additional 108 mutants all with point mutations in the proM gene [36]. Among these 109 mutants, none had an extra base in the anticodon as the classical +1 frameshift derivatives of proL (sufB2) and proK (sufA6) have. The G31A mutation was found in 32% of these proM mutants most likely because it is the strongest frameshift suppressor among the 108 proM mutants characterized. Interestingly, most of the alterations in the proM are in close proximity to components in the ribosomal P-site further supporting the pivotal role of the P-site in reading frame maintenance [36]. Accordingly, the frameshift error induced by these altered proM : s occurs in the P-site as determined by amino acid sequence of the frameshift product and from overexpression of the tRNA reading the A-site codon [36]. Clearly, our extensive selection of +1 frameshift suppressor mutants identified novel alterations in the tRNAPro family and identified, for the first time, an alteration of the proM that mediates a frameshift error with a mechanism consistent with our model (Fig. 1, alt. B).

In Salmonella is encoded by a single gene, proK, and with its C34 as wobble nucleoside it should only read CCG (Fig. 5). Although a mutant with a proK deletion is viable and grows as wild type such a strain does not suppress the hisC3737 or the hisD10122 mutations (unpublished observation). Apparently only specific changes of the proK induce +1 frameshift suppression consistent with a proK mutation (sufA6) being dominant [78]. We therefore did not expect many +1 frameshift suppressor mutants with alterations in this tRNA. Indeed, this was the case, since only two independently isolated mutants (proK2236 and proK2237) with an altered proK were obtained. Interestingly, both of them had the same alteration as the classical sufA6 mutant; i.e an extra G in the anticodon loop. The sufA6 tRNA, and therefore the two altered proK :s characterized here, have a normal sized anticodon bordered by m1G37 and U33 and the insertion of the extra G is 3′ to the m1G37 [34]. Such altered proK tRNA induces frameshifting in the P-site according to our model [34]. The three-nucleotide size of the anticodon of these proK mutants and their induction of +1 slippage in the P-site are not consistent with the quadruplet translocation model. Such proK mutants have three tRNAPro:s (wild type proL and proM in conjunction with the altered proK ) any of which may cause the +1 frameshift error and thereby suppress the +1 frameshift mutation. Of these, the proL is the cognate tRNA reading the CCC codon and we therefore find it unlikely that this tRNA makes the frameshift error in the P-site, since its structural interaction with the P-site environment and potential anticodon-codon interaction, is normal. Thus, either the wild type proM or the altered proK causes the frameshift error. Removing the cmo5U modification genetically reduces the frameshift suppression by about 50% suggesting that this part of the frameshifting is due to wild type proM , since it is the only tRNAPro containing this modified nucleoside [34] (Fig. 1, alt A). As the sufA6 (a derivative of proK) mediated frameshifting occurs in the P-site [34], it is apparently a mixed population of peptidyl-Pro-tRNAPro (wild type proM and mutant proK (sufA6, proK2236, or proK2237) tRNAs) that slips into the +1 frame in the P-site. The proM is less abundant in the cell compared to proL and proK tRNAs (68% of proL and 95% of proK at growth rate of 2.5 doublings [79]). In the proK mediated frameshifting, proM must therefore compete efficiently with the wild type proL in reading the CCC codon, since 50% frameshifting is caused by the proM [34]. The residual 50% of frameshifting occurring in the P-site must therefore be caused by the altered proK (Fig. 1, alt B). The distance between the two strands of the tRNA and mRNA in the anticodon-codon interaction is too large for two pyrimidines (C34 of proK and C(III) in the codon) to interact. Consequently it is not likely that proK makes a pairing with the third nucleoside (CIII) of the CCC codon. We therefore propose that the altered proK with its extra G in the anticodon loop, but still having a normal sized anticodon bordered between m1G37 and U33 [34], is able to make 2 out of 3 interaction with the CCC codon in the A-site. After a three nucleotide interaction, its fitting in the P-site is not optimal making it prone to shift frame. Since the proL is present in the cell at about the same concentration as the altered proK such a 2 out of 3 interaction can compete with a cognate interaction by the wild type proL to read the CCC codon consistent with the altered proK being dominant. The fact that we found two proK mutants with the same alteration as the classical sufA6+1 frameshift mutant is consistent with our model since the frameshift event occurs in the P-site [34].

As pointed out above, deletion of proK is viable but does not suppress the hisC3737 (CCC-CAA) or hisD10122 (CCC-CAA). However, in the presence of the proK mutant tRNA with an extra G in the anticodon loop, 50% of the suppressor activity is due to the wild type proM (Fig. 1, alt A). From this result one would expect that a deletion of proK should allow proM mediated frameshifting. Why is this not occurring? Apparently the proM is able to read the CCC codon in the presence of mutant proK tRNA but not when the wild type proK is absent. The reason may be that in a cell having proM and proL tRNAs, like in a mutant with proK deleted, the only tRNA reading the CCG codon is proM . This may result in too low a concentration of the proM to compete with the proL in reading the CCC codon explaining that a deletion of the proK gene does not induce a frameshift by the proM .

From above we conclude that the ability to decode the four proline codons depends not only on the decoding capacities as revealed by the anticodon-codon interaction but also on the availability of the different Pro-tRNAs to decode the various proline codons in the cell at various conditions. Clearly, the analysis of the +1 frameshift phenotypes of the proK, proL, and proM mutants have revealed an intricate competition between the three Pro-tRNAPro:s to read the CCC codon and thereby induce +1 frameshifting in the P-site at the various frameshift mutations used.

All three tRNAPro have m1G37 next to and 3′ of the anticodon. Lack of m1G37 results in a tRNAPro having three consecutive G:s in the anticodon loop. When it was discovered that lack of m1G induces +1 frameshifts [18], it was suggested that such m1G deficient tRNAPro therefore had the possibility of making a four base interaction in the A-site and by a quadruplet translocation move the tRNA to the P-site. However, the m1G deficient tRNA slips forward one nucleotide in the P-site [35] which is not consistent with the quadruplet translocation model but is consistent with the model presented here (Fig. 1). The rate with which the three tRNAPro:s enter the A-site is reduced, by 50–90%, due to the lack of m1G [71]. Of the three tRNAPro:s, the proL is the least affected (50%) by m1G deficiency. It is the cognate tRNA for the CCC codon and its concentration in the cell is larger than that of proM , which also reads CCC. Therefore we suggest that it is mainly the m1G deficient cognate proL which makes a slippage in the P-site due to the lack of m1G although we cannot exclude that also the m1G deficient proM makes such an error. The m1G37 may interact in the P-site with some constituents of rRNA/r-protein(s), and lack of it in proL or in proM , may disrupt such a stabilizing interaction of the peptidyl-tRNA. Lack of the ms2-group or of the ms2io6-groups of the ms2io6A37, which is, like m1G37, present in position 37 but in tRNAPhe and tRNATyr, also induces +1 slippage in the P-site [16]. Crystal studies of tRNAPhe show that the ms2i6A37 is part of a network of interactions with the first base of the P-site codon, third base of the E-site codon and anchors the tRNA in the P-site with A790 and U789 of the 16S rRNA [80]. Thus, these structural data support a pivotal role of the P-site environment to maintain the reading frame and more specifically point to some fundamental interactions between position 37 of the peptidyl-tRNA and 16S rRNA. Interestingly, lack of two other modified nucleosides (t6A37 and yW37) present in position 37 of the tRNA also mediate increased frameshifting [21]–[23]. Apparently, the modification in position 37 of several tRNAs is important to maintain the reading frame. In summary, the fact that m1G deficiency induces frameshift errors in the P-site further supports the model in Figure 1 and the structural data presented for another modified nucleoside present in the same position as m1G, strengthen the importance of the P-site environment in reading frames maintenance and the role of modification in position 37 of tRNA in this process.

If the ribosomal P-site is important for reading frame maintenance, one would expect that a nonessential alteration in this part of the ribosome would also induce +1 frameshifting. Of course we did not expect many mutants defective in this part of the ribosome since many of such alterations would be lethal due to the important function of the P-site in translation. Still, we obtained two mutants among the 467+1 frameshift mutants both of which lacked several amino acids of the C-terminal end of ribosomal protein S9. The S9 protein is part of the common core shared by bacteria and eukaryotes and is one of the 34 conserved ribosomal proteins (15 in the small subunit and 19 in the large subunit) [81]. The C-terminal part of the S9 protein penetrates like a tentacle into the P-site of the ribosome and the two last amino acids of the protein make contacts with the 5′-phosphate of nucleotide 32 (R130) and the 5′-phosphates of positions 33 and 34 (K129) of peptidyl-tRNA [6] (Fig. 6). The existence of these mutants prompted us to change the two most C-terminal amino acids of S9 protein and monitor the ability to induce +1 frameshifts [36]. Indeed all these rpsI (S9) mutants induce +1 frameshifts. The isolation and characterization of these mutants defective in ribosomal protein S9 is a strong support that the frameshift event occurs in the P-site and makes the ribosomal grip of the peptidyl-tRNA one of the important features to maintain the reading frame.

Conclusion

All our results support the frameshifting model presented in Figure 1 and demonstrate the pivotal role of the ribosomal grip of the peptidyl-tRNA. Moreover, the results demonstrate an intricate competition between the three Pro-tRNAs to read the four codons in the Pro-box and highlight the importance of the modified nucleosides in positions 37 (next to and 3′ of the anticodon), 34, and 38 in maintaining the reading frame.