Ribosomal -1 Frameshifting during Decoding of Bacillus subtilis cdd Occurs at the Sequence CGA AAG

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Journal of Bacteriology, May 1999, p. 2930-2937, Vol. 181, No. 9
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Ribosomal $-$ 1 Frameshifting during Decoding of Bacillus subtilis cdd Occurs at the Sequence CGA AAG

Nina Mejlhede,¹ John F. Atkins,² and Jan Neuhard¹^,^*

Center for Enzyme Research, Institute of Molecular Biology, University of Copenhagen, DK-1307 Copenhagen K, Denmark,¹ and Department of Human Genetics, University of Utah, Salt Lake City, Utah 84112-53302²

Received 16 November 1998/Accepted 11 February 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

During translation of the Bacillus subtilis cdd gene, encoding cytidine deaminase (CDA), a ribosomal $-$ 1 frameshift occursnear the stop codon, resulting in a CDA subunit extended by 13amino acids. The frequency of the frameshift is approximately16%, and it occurs both when the cdd gene is expressed from amulticopy plasmid in Escherichia coli and when it is expressedfrom the chromosomal copy in B. subtilis. As a result, heterotetramericforms of the enzyme are formed in vivo along with the dominanthomotetrameric species. The different forms have approximatelythe same specific activity. The cdd gene was cloned in pUC19 suchthat the lacZ' gene of the vector followed the cdd gene in the $-$ 1 reading frame immediately after the cdd stop codon. By usingsite-directed mutagenesis of the cdd-lacZ' fusion, it was shownthat frameshifting occurred at the sequence CGA AAG, 9 bp upstreamof the in-frame cdd stop codon, and that it was stimulated bya Shine-Dalgarno-like sequence located 14 bp upstream of the shiftsite. The possible function of this frameshift in gene expressionisdiscussed.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Some mRNAs contain signals that direct a high proportion of ribosomes to change reading frame at a specific shift site. These"programmed" events can occur at levels that are 1,000- to 10,000-foldabove the low background of error frameshifting. Their functioncan be either as a sensor for regulatory circuits, as in the decodingof the genes for Escherichia coli polypeptide chain release factor2 (prfB) or mammalian antizyme, or to give a set ratio of twodifferent products that have some identical sequences, as in thedecoding of E. coli dnaX or human immunodeficiency virus gag-pol.Quite a number of cases of programmed frameshifting are knownin the expression of viruses and in mobile chromosomal elementssuch as yeast Ty elements and IS elements of the IS3 family (forreviews, see references 5, 11 and 13). However, very fewcases are known for nonmobile chromosomal genes. In mammals antizymeis the only known case (26, 29), and in bacteria the listis restricted to prfB (8, 40) and dnaX, which encode twosubunits of DNA polymerase III (4, 12, 39).

Early studies showed that disruption of codon-anticodon pairing and re-pairing of the anticodon to an overlapping codon explainedmany cases of frameshifting in model systems, and the involvementof a single tRNA in such a process is the basis for $-$ 1 frameshiftingin potato virus M (14). However, studies on retroviruses showedthat for $-$ 1 frameshifting, tandem shifts of two tRNAs on a sequenceof the general form X XXY YYZ was very effective (15). In E.coli, a very slippery form of this heptanucleotide was found tobe A AAA AAG, which occurs at the shift sequence for dnaX (4,12, 39) and IS911 (32). The majority of these tandem shiftsites were found to require secondary mRNA structures such aspseudoknots or stem-loop structures downstream of the slipperyheptanucleotide to achieve maximal efficiency (5, 22, 38).

Frameshifting studies showed that the anti-Shine-Dalgarno (anti-SD) sequence close to the 3' end of 16S rRNA within translatingribosomes must be scanning mRNA for potential complementarity.An SD-like sequence 3 bases 5' of the shift site is importantfor the obligatory +1 frameshifting in decoding release factor2 and its spacing has to be precise (9, 40). An SD-like sequence10 bases 5' of the shift site is important for the $-$ 1 frameshiftingin dnaX, with flexibility between 9 and 15 nucleotides for thespacer length (21).

The Bacillus subtilis cdd gene, encoding the pyrimidine salvage enzyme cytidine deaminase (CDA), was cloned and sequencedby Song and Neuhard (37). The deduced amino acid sequence indicateda subunit size of 14.9 kDa, and preliminary studies suggestedthat the native enzyme was a homotetramer. In the present work,we observed that expression of the gene, both from a plasmid-bornecopy in E. coli and from the chromosome in B. subtilis, yieldedtwo types of subunits: the predicted 14.9-kDa subunit and smalleramounts of a 16-kDa subunit. As a result, measurable amounts ofheterotetrameric forms of the enzyme were detected. We showedthat the heterogeneity in subunit size is due to a $-$ 1 ribosomalframeshift occurring during translation of the 3' end of the codingsequence and identified a new type of shift site with an upstreamstimulatory SD-likesequence.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Bacterial strains and growth conditions. The E. coli strains used were JF611 (cdd pyrE argE his proA thr leu thi), obtained from Jim Friesen, and SØ5299, a cdd::Tn10derivative of JM83. Both strains are defective in CDA due to cddmutations. They were grown at 37°C in Luria broth (2) or ABminimal medium (6) supplemented with 0.2% glucose, 0.2% CasaminoAcids, and 1 µg of thiamine per ml. When required, ampicillinwas present at 100 µg per ml. B. subtilis 168 (trpC) was grownat 37°C in a modified Spizizen salts minimal medium supplementedwith 0.4% glucose, 0.2% glutamate, and 1 µg of thiamine per ml(36).

DNA techniques. DNA manipulations, transformations, and isolation of plasmid DNA were performed by standard procedures as described by Sambrooket al. (34). PCR products were purified with the Qiagen PCRpurification kit. Endonuclease digestion and ligation of DNA weredone as specified by the suppliers. DNA sequencing was performedby the chain-termination method (35) with double-stranded DNAsastemplates.

Plasmids. To achieve overproduction of B. subtilis CDA in E. coli, plasmid pSO143 was used (Fig. 1A) (37). It contains the B. subtiliscdd gene without its promoter but with its native ribosomal bindingsite on a 740-bp KpnI-EcoRI fragment in pUC19. Immediately downstreamof cdd, with a 20-nucleotide overlap, the fragment carries thefirst third of the bex gene (18). Expression of cdd occurs fromthe lac promoter on the vector. All other plasmids used in thepresent study were derived from pSO143 and varied only in theregion between the cdd stop codon and lacZ' of the vector. PlasmidpSO1000 was constructed by subcloning the cdd gene from pSO143on a 470-bp PstI-BsaBI fragment into PstI- and SmaI-digested pUC19(Fig. 1B). On pSO1000, lacZ' is in the 0 reading frame comparedto cdd. In unrelated structure-function studies of B. subtilisCDA, we used pSO1000 as a template for PCR-mediated site-directedmutagenesis of the coding region of cdd. One of the constructsobtained, pSO1001, was shown by DNA sequencing to have sufferedan unintended deletion of 1 bp (A) immediately 3' of the cdd stopcodon, in addition to the mutation introduced by PCR in the codingregion (TG $right-arrow$ CA, yielding a C53H mutation in CDA). As a resultof the deletion, lacZ' is fused in the $-$ 1 reading frame comparedto cdd on pSO1001 (Fig. 1B). Plasmid pSO1001 was opened at theunique EcoRI site in front of lacZ', digested by mung bean nucleaseto remove the 5' overhangs, and ligated to create pSO1002, whichcarries lacZ' in the +1 reading frame (Fig. 1B).

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FIG. 1. Structures of the plasmids used in this study. (A) pSO143. Thin lines, pUC19 DNA; solid bar, coding region of the B. subtilis cdd gene; open bar, leader region of the cdd gene; hatched bar, coding region of the 5' end of the B. subtilis bex gene. Restriction endonuclease sites: E, EcoRI; Bs, BsaBI; K, KpnI; P, PstI; S, SmaI. The nucleotide sequence in the frameshift region near the end of the cdd gene, as well as the deduced amino acids encoded by the three reading frames, are shown below the graph. Capital letters, C-terminal amino acids of the wild-type CDA subunit; bold capital letters, C-terminal amino acids of the extended subunit (S^ext); italicized capital letters, N-terminal amino acids of the Bex protein. (B) Nucleotide sequence of the region between the CDA stop codon and lacZ' in various plasmids. The CDA stop codon is overlined, and the EcoRI site is underlined. pUC19 sequences are in italics, and lacZ' sequences are in lowercase letters. Numbers in parentheses refer to the reading frame of lacZ' relative to cdd.

Plasmid pNMJ62 was used for quantitation of $-$ 1 frameshifting. It contains the entire cdd coding region inserted in pUC19 insuch a way that the $-$ 1 reading frame of cdd continues into lacZ'of the vector. It was constructed by PCR amplification of cddfrom pSO143 with, as the 5' primer, the 24-mer reverse sequencingprimer ( $-$ 48) of M13/pUC and, as the 3' primer, the wild-type primershown in Table 1. This latter primer was complementary to thelast 4 codons of cdd and had an EcoRI site introduced 1 bp afterthe stop codon. The resulting fragment was digested with PstIand EcoRI and inserted into the multiple-cloning site of pUC19.

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TABLE 1. 3' primers for PCR-mediated site-directed mutagenesis

Site-directed mutagenesis. Site-directed mutagenesis of the frameshift region upstream of the cdd stop codon was accomplished by PCR amplification ofthe entire cdd gene on pNMJ62 with, as the 5' primer, the 24-merreverse sequencing primer ( $-$ 48) of M13/pUC in all cases. The 3'primers were all complementary to the 3' end of the cdd gene exceptfor the desired mutation(s) and included the EcoRI site 1 bp downstreamof the stop codon (Table 1). The amplified fragments were digestedwith PstI and EcoRI and cloned into pUC19 digested with the sameenzymes. Thus, the vector-borne lacZ' followed the cdd stop codonin the $-$ 1 reading frame of cdd, as in pNMJ62. All plasmid constructswere confirmed by DNAsequencing.

Purification of recombinant CDA from E. coli. Cells from a 1-liter culture of E. coli JF611/pSO143 grown overnight at 37°C in Luria broth supplemented with ampicillin (100µg/ml) were harvested by centrifugation, washed with 0.9% NaCl,resuspended in 6 to 8 volumes of 50 mM Tris-HCl (pH 7.2) (bufferA), and disrupted by sonic oscillations at 4°C. All subsequentsteps were performed at 4°C. Cellular debris was removed by centrifugation,and streptomycin sulfate was added to the supernatant to a finalconcentration of 1%. Following centrifugation, the supernatantwas applied to a DEAE-cellulose (DE-52) column (2.5 by 24 cm)equilibrated with buffer A. The column was washed with 7 volumesof buffer A, and the enzyme was eluted with a linear gradientof NaCl in buffer A. The fractions containing CDA activity wereconcentrated by pressure filtration to 5 ml and treated at 68°Cfor 10 min. The supernatant after heat denaturation was subjectedto gel filtration on a Sephadex G-100 column (2.5 by 85 cm) equilibratedand eluted with buffer A. The active fractions were pooled andapplied to an ion-exchange column (Q5; Bio-Rad) equilibrated with20 mM Tris-HCl (pH 7.6) and connected to a Pharmacia fast proteinliquid chromatography (FPLC) apparatus. The column was washedwith 3 volumes of 20 mM Tris-HCl (pH 7.6), and the enzyme waseluted with a gradient of KCl in the same buffer. For the resultof a typical purification, see Table 2.

Purification of native CDA from B. subtilis. Cells from a 5-liter culture of B. subtilis 168 in early stationary phase were harvested by centrifugation, washed with cold0.9% NaCl, resuspended in 6 to 8 volumes of buffer A, and disruptedby sonication. The enzyme from the sonic extract was partiallypurified by the same procedure as described for the recombinantenzyme. The final preparation represented a 150-fold purificationover crude extract and yielded an enzyme which, according to sodiumdodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE),was approximately 30%pure.

Preparation of cell extracts and enzyme assays. Crude cellular extracts were prepared by sonic disruption of cells suspended in 0.1 M Tris-HCl (pH 7.6), followed by centrifugationto remove cellular debris. $beta$ -Galactosidase activity was determinedas described by Miller (28), and CDA activity was measured spectrophotometrically(7). Protein concentration was measured by the Lowry methodwith bovine serum albumin as thestandard.

SDS-PAGE. Protein samples or whole cells were incubated for 2 min at 100°C in 2× SDS loading buffer (100 mM Tris-HCl [pH 6.8], 20% glycerol,4% SDS, 0.2% bromophenol blue) and run on SDS-polyacrylamide gels(19). Polypeptides were identified on the gels by staining withCoomassie blueG250.

Preparation of antibodies and Western blotting. The antibodies were prepared by Michael Theisen, State Serum Institute, Copenhagen, Denmark. The antibodies were raised inrabbits with a homogenic preparation of homotetrameric CDA purifiedfrom E. coli JF611/pSO143. The antibody preparation (serum) wasstored at 4°C. Polypeptides separated by SDS-PAGE were transferredto a nitrocellulose membrane (Schleicher & Schüll, Dassel, Germany)in 48 mM Tris-39 mM glycine-1.3 mM SDS-20% methanol by using aSemi-dry electroblotter (JKA-Biotech) for 1 h at 50 mA. The membranewas incubated with phosphate-buffered saline (PBS) (8 mM Na₂HPO₄,20 mM KH₂PO₄, 130 mM NaCl) plus 0.5% Tween 20 for 10 min and subsequentlyincubated overnight with PBS containing 0.05% Tween 20, 0.37 MNaCl, and antibodies against CDA diluted 1:50. After incubationwith primary antibody, the membrane was washed twice in PBS containing0.05% Tween 20 and 0.37 M NaCl and incubated with swine anti-rabbitimmunoglobulin conjugated with horseradish peroxidase (Dako, Copenhagen,Denmark) for 1 h. The membrane was washed twice for 20 min eachin PBS containing 0.05% Tween 20 and 0.37 M NaCl and once for1 min in citrate-phosphate buffer (pH 5.0) (100 mM Na₂HPO₄, 50mM citric acid). Staining was carried out in 10 ml of 0.8% (wt/vol)dioctylsodium phosphosuccinate in ethanol (DONS solution)-0.33ml of tetramethylbenzidine (7% [wt/vol] in DONS solution)-40 mlof citrate-phosphate buffer (pH 5.0)-20 µl of 30% H₂O₂. Finally,the membrane was washed in 10 ml of DONS solution-40 ml of H₂O.

N-terminal amino acid determination. Heterotetrameric CDA purified from JF611/pSO143 was subjected to SDS-PAGE (13.5% polyacrylamide), and the bands correspondingto the two subunits were blotted to a polyvinylidene difluoridemembrane (Bio-Rad) by using a Semi-dry electroblotter (JKA-Biotech).The N-terminal amino acid sequence of the blotted polypeptideswas determined by automated Edman degradation on an Applied Biosystems477A gas-phase Sequenator by Arne Jensen, Department of ProteinChemistry, University of Copenhagen, Copenhagen,Denmark.

Mass spectrometry. Liquid chromatography-mass spectrometry analysis, using positive-ion electrospray ionization, of the homotetrameric (S₄) andthe heterotetrameric (S₃S^ext) forms of CDA was performed. Aliquots of the homotetramer (1,300pmol) and the heterotetramer (500 pmol) in 5 mM Tris buffer wereloaded onto a C₁₈ reversed-phase high-pressure liquid chromatographycolumn (Brownlee Aquapore RP-300; 7-µm pore size, 100 by 2.1 mm),which was used as a trapping device to desalt the protein productsfor subsequent electrospray ionization and mass analysis. Theproteins were washed (desalted) on the high-pressure liquid chromatographycolumn with 30% acetonitrile-0.2% acetic acid for 3 min and theneluted by increasing the acetonitrile to 70% over a period of2 min at a flow rate of 200 µl/min. About 33% of the eluent wasdirected to the electrospray interface of a Quattro II mass spectrometer(Micromass, Inc.). Mass spectra were acquired over the range of750 to 1,250 Da every 5 s with a spray voltage of 2.7 kV and asample cone voltage of 33 eV. Protein molecular mass spectra wereprocessed through deconvolution of multiply charged molecularions by using MaxEnt software (Micromass, Inc.) (see Fig. 6).Molecular mass assignments for the standard translation product(homotetramer, 14,854.6 Da) and the frameshift product (heterotetramer,16,355.9 Da) are within 0.003% mass error of the predictedmasses.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

CDA is expressed as two different subunits from one DNA sequence. Recombinant B. subtilis CDA was purified from E. coli JF611 harboring the B. subtilis cdd gene on the multicopy plasmid pSO143(Table 2). SDS-PAGE of the enzyme preparation following DEAE-cellulosechromatography, heat treatment, and gel filtration (Table 2,step 5) showed two bands corresponding to polypeptides with apparentmolecular masses of 14.5 and 16 kDa, respectively (Fig. 2, lane4). Automated Edman degradation of the two polypeptides showedthat both had the N-terminal amino acid sequence MNRQE, whichis identical to the sequence of the first five N-terminal aminoacids deduced from the nucleotide sequence. The coding regionof cdd consists of 408 nucleotides encoding a 136-amino-acid polypeptidewith a predicted molecular mass of 14,854 Da. This correspondedto the mass of the major polypeptide of the purified CDA. The16-kDa polypeptide was present in smaller amounts and presumablyrepresented a CDA subunit with an extended C terminus.

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TABLE 2. Purification of B. subtilis recombinant CDA^a

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FIG. 2. SDS-PAGE (16% polyacrylamide) of recombinant B. subtilis CDA. Lanes: 1, size markers; 2, crude cellular extract of JF611; 3, crude cellular extract of JF611/pSO143; 4, purified recombinant CDA from step 5 of the purification in Table 1. The polypeptide bands were visualized by staining with Coomassie brilliant blue G-250.

FPLC of the purified CDA preparation (Table 2, step 5) on a Q5 ion-exchange column resolved the enzyme in three peaks (Fig.3) of approximately the same specific CDA activity (data not shown).SDS-PAGE of the individual peak fractions (Fig. 3) showed thatCDA from peak 1 consisted of the 14.5-kDa subunit (S) only andhence represented the homotetrameric form (S₄). In contrast, CDAfrom peaks 2 and 3 contained both S and the extended subunit (S^ext). As judged from the relative intensities of the bands on thegel, peaks 2 and 3 represented heterotetrameric forms of the enzymewith the compositions S₃S^ext and S₂S^ext₂, respectively.

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FIG. 3. Chromatography of purified recombinant CDA from step 5 of Table 1 on a Q5 FPLC column. (Left) Elution profile. Full line, absorbance at 280 nm (A280) of individual fractions; dashed line, salt gradient percentage of 1 M KCl. (Right) SDS-PAGE (13.5% polyacrylamide) of individual peak fractions from the column. Lanes: 1, peak 1; 2, peak 2; 3, peak 3; 4, size markers.

To assess whether the production of S^ext was a result of overexpressing the B. subtilis cdd gene in E. coli, a preparation ofCDA, partially purified from B. subtilis 168, was subjected toSDS-PAGE and the electropherogram was immunoblotted with polyclonalantibodies raised against the purified recombinant enzyme. Asshown in Fig. 4, the immunoblot revealed two bands with aboutthe same mobilities and relative intensities as observed withthe recombinant enzyme produced in E. coli.

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FIG. 4. Immunoblot of an SDS-PAGE (13.5% polyacrylamide) electropherogram with antibodies raised against recombinant B. subtilis CDA. Lanes: 1, partially purified CDA from B. subtilis 168; 2, crude extract of JF611/pSO143.

The ribosome slips to the $-$ 1 frame in front of the cdd stop codon. The apparent molecular mass of S^ext (16 kDa) in conjunction with analysis of the DNA sequence of pSO143 suggested that a $-$ 1 frameshifthad occurred late in the cdd gene, resulting in a 13-amino-acidextension of the CDA subunit (Fig. 1A). To examine this further,lacZ' from pUC19 was fused to cdd in all three reading framesdownstream of the stop codon, yielding pSO1001, pSO1000, and pSO1002.A $-$ 1 frameshift occurring before the stop codon of cdd carriedby these plasmids would result in the synthesis of CDA subunitswith 93-, 19-, and 57-amino-acid extensions and molecular massesof 25.6, 17.0, and 20.9 kDa, respectively. E. coli cells harboringpSO1001, pSO1000, and pSO1002 were analyzed by SDS-PAGE and immunoblottingas described above. As shown in Fig. 5, the apparent sizes ofthe extended subunits were all in accordance with the values predictedas a result of a $-$ 1 frameshift occurring in front of the cdd stopcodon. Accordingly, the pSO1001 construct, which constituted thein-frame situation for lacZ' in the $-$ 1 reading frame of cdd, mediated $beta$ -galactosidase activity when transformed into SØ5299, a lac deletionstrain carrying $phi$ 80dlac $Delta$ (lacZ)M15.

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FIG. 5. Immunoblot of an SDS-PAGE (15% polyacrylamide) electropherogram with antibodies raised against recombinant B. subtilis CDA. Crude cellular extracts of the following strains were used: lane 1, JF611/pSO143; lane 2, SØ5299/pSO1001; lane 3, SØ5299/pSO1000; lane 4, SØ5299/pSO1002.

Identification of the slip site. Mass spectrometric analysis of purified homotetrameric (Fig. 3, peak 1) and heterotetrameric (peak 2) CDA established thatthe exact masses of the two subunits, S and S^ext, were 14,854.5 and 16,355.9 Da, respectively (Fig. 6). The 14,854.5-Davalue agreed exactly with a mass of 14,854 Da for S calculatedfrom the deduced amino acid sequence. Inspection of the nucleotidesequence revealed that a $-$ 1 frameshift at the penultimate cddcodon, i.e., AAG to AAA (Fig. 1), would give rise to a subunitwith a deduced molecular mass of 16,356 Da, in complete accordancewith the determined size of 16,355.9 Da. No other $-$ 1 frameshiftin the distal end of cdd would give rise to a subunit of thatsize.

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FIG. 6. Electrospray mass spectra of CDA. Top, homotetramer (S₄); bottom, heterotetramer (S₃S^ext). Measured molecular weights are shown.

Analysis of the slip site by site-directed mutagenesis. To examine the effect of the nucleotide sequence context on the $-$ 1 frameshift at the putative shift site, A-AAG, mutationswere introduced at each of the five last codons of the gene, includingthe termination codon. The mutations were made in pNMJ62, whichcontained lacZ' fused in the $-$ 1 frame of cdd immediately followingthe termination codon. With the exception of one insertion mutation(AAG $right-arrow$ AAAG) and the change of the stop codon to a sense codon(TAA $right-arrow$ TAC), the mutations did not change the amino acid sequencein the 0 reading frame. The resulting constructs were transformedinto SØ5299, and the level of $beta$ -galactosidase in the transformantswas used as a measure of frameshifting. Table 3 summarizes theresults obtained with the different mutants. As an indicator ofthe intracellular level of functional CDA transcript, the specificCDA activity was also determined in each strain (data not shown).Two of the mutants, i.e., Stop UAA $right-arrow$ Tyr UAC and AAG $right-arrow$ AAAG, producedno detectable CDA activity. Translation of these constructs inthe 0 frame produced CDA subunits with 51- and 86-amino-acid extensions,respectively, which presumably are incapable of forming activeenzymes. Correction of the $beta$ -galactosidase values for CDA activitydid not result in major changes in the measured frameshift levels,as shown by the numbers in parentheses in Table 3.

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TABLE 3. Mutational analysis of the shift region in the 3' terminus of cdd^a

Changing the UAA stop codon to the tyrosine codon UAC, the leucine codon CUU to CUG, or the 5' glutamic acid codon GAA toGAG had only a minor effect on the $beta$ -galactosidase level, resultingin a frameshift level of 155, 85, or 91%, respectively, comparedto that of the wild type. In contrast, mutations in the lysineand arginine codons that changed the sequence A-AAG had dramaticeffects. Thus, the frameshift level dropped to 6% when the lysinecodon AAG was changed to AAA, and modifications of the rare CGAcodon for arginine to the common CGC codon resulted in barelydetectable frameshift levels. Mutating the CGA codon to arginineAGA also resulted in very low levels of frameshifting, indicatingthat the minimal sequence requirement for efficient frameshiftingwas CGAAAG.

Stimulatory mRNA elements. An SD-like sequence, capable of forming five Watson-Crick base pairs with the 3' end of 16S rRNA, is located 14 nucleotides5' of the slip region CGA AAG. Since an SD sequence has been shownto stimulate $-$ 1 frameshifting in the E. coli dnaX gene (21),this region was mutated such that base pairing with the 16S rRNAwas weakened without changing the corresponding protein product.Modifying the sequence G GAG GA to C GAA GA reduced the frameshiftlevel to 9% (Table 3), indicating that this region on the mRNAis a 5' stimulatory element for theframeshift.

A number of frameshift events were found to be stimulated by secondary mRNA structures such as pseudoknots or stem-loop structureslocated 3' of the shift site. A computer search for stable downstreamsecondary mRNA structures did not identify any putative stimulatoryelement. Since dramatic changes in the sequence of the downstreammRNA, such as those present in pSO1000, pSO1001, and pSO1002,did not affect the level of frameshifting significantly (Fig.5), it was inferred that no shift-stimulating structure was locateddownstream of the shiftsite.

Frameshift level. As judged by SDS-PAGE, the number of S^ext subunits was roughly 10 to 20% of that of the number of S subunits (Fig. 2, 4, and5). To make a more accurate measurement of the wild-type frameshiftlevel, we inserted an additional A at the shift site in pNMJ62,i.e., AAG $right-arrow$ AAAG. In this mutant, lacZ' was in frame with the0 reading frame of cdd. As shown in Table 3, this mutant mediateda $beta$ -galactosidase level 6.3 times higher than that of the wild-typeconstruct, indicating that ribosome frameshift was about 16%.In the absence of the upstream SD-like sequence, frameshiftingwas reduced to about 1.5%.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Studies of B. subtilis CDA expression in E. coli have revealed a new frameshift site, CGA AAG, and probably a new type ofdisposition of the tRNAs involved. The intrinsic shiftiness ofthis shift site on its own is 1.5% (Table 3), compared to 2%seen with A AAA AAG (21), which rates it as a good shift site.Simultaneous slippage of tandem tRNAs, as has been observed onsequences of the general form X XXY YYZ, is not involved, as evidencedby the lack of re-pairing possibilities for the cognate CGA-decodingarginine tRNA, whose anticodon is 3'GCI5', where I is inosine.A and I are the only two purines that face each other in decoding.If they were to pair, it would require nonstandard geometry thatmay destabilize the codon-anticodon complex (10, 23). It seemsprobable that the I frequently occludes the A and triplet codingensues. However, occasionally the A may be available for pairingas the first base of the next codon, resulting in doublet translocationand $-$ 1 frameshifting (Fig. 7). A somewhat similar scenario waspreviously observed for decoding of the glycine GGA codon. Itwas shown that normal levels of tRNA-Gly2 with a single substitutionthat gave a CCC anticodon mediated both doublet and triplet decodingof GGA. Due to several differences elsewhere in the tRNA, it requiresoverexpression of E. coli tRNA-Gly1, which has the same anticodon,to mediate detectable doublet decoding (30). Previously, Lagerkvistand colleagues showed that C at position 32 of Mycoplasma mycoidestRNA-Gly was substantially responsible for its decoding all fourglycine GGN codons (20, 24). Replacement of the base at position32 of E. coli tRNA-Gly1 with C led to enhanced efficiency of doubletdecoding.

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FIG. 7. Model of $-$ 1 frameshifting in CDA. U*, 5-methylaminomethyl-2-thiouridine.

Pairing of the third base of the second codon, AAG, within the shift site to its cognate lysine-tRNA is also compromised.In E. coli, the lysine codons AAG and AAA are both decoded bya single tRNA with the anticodon 5'-mnm⁵s²UUU-3' containing 5-methylaminomethyl-2-thiouridine at the wobbleposition. The modification causes more efficient binding of thetRNA to AAA than to AAG in vitro (25, 42). In the presentcase, frameshifting involves dissociation from the AAG codon andre-pairing to the overlapping AAA codon, which includes the Awhich previously flirted with inosine (Fig. 7). The observationthat replacing AAG by AAA caused a strong reduction in frameshiftingindicates that binding of tRNA-Lys to AAA is favored over bindingto AAG in vivo. Interestingly, replacing the rare CGA codon withanother rare arginine codon, AGA, resulted in a very low levelof frameshifting, despite conservation of the shifty A AAG sequence.Most probably this is because the AGA codon is decoded by tRNA-Argwith the anticodon UCU, which forms three Watson-Crick base pairsin the codon-anticodon complex, thereby making A at the thirdposition unavailable for re-pairing with the tRNA-Lys in the $-$ 1frame.

The presence of an SD-like sequence 14 nucleotides upstream of the slip site resulted in an 11-fold stimulation of $-$ 1 frameshifting(Table 3). Previously, SD interactions by translating ribosomeswere found to stimulate $-$ 1 frameshifting in decoding of the dnaXgene of E. coli (41), and it was shown by Larsen et al. (21)that the optimal spacing between the SD sequence and the slipsite was 10 to 13 nucleotides, i.e., slightly shorter than inthe present situation. Mutations in regions of the 16S rRNA nearthe 3' end have been shown to promote stop codon readthrough andframeshifting during elongation, indicating that these regionsare in proximity to the site of codon-anticodon interaction inthe ribosome (31). It seems likely that when the spacing betweenthe SD sequence and the site of action is significantly largerthan the optimal spacing for translation initiation, the ribosomewill be strained and will tend to pull the peptidyl-tRNA towardthe $-$ 1frame.

The frameshift in the 3' end of the B. subtilis cdd gene occurs not only when the gene is expressed from a multicopy plasmidin E. coli but also in the native condition when the gene is expressedfrom the chromosome in B. subtilis. Thus, slippage is not dueto overexpression of an alien sequence with exotic codon usage.The tRNA anticodons of E. coli (17) and B. subtilis (18) arevery similar, and no tRNAs with perfectly matching anticodonsexist for the arginine CGA and the lysine AAG codons in eitherorganism. The 3' sequences of the 16S rRNA from the two bacteriaare similar and will presumably base pair equally well with theSD sequence upstream of the cdd stop codon (27). Therefore,it seems likely that the same mechanism is responsible for theframeshifting in bothorganisms.

The frameshift appears to be irrelevant to CDA expression since no significant difference in CDA activity of the homotetramericand the heterotetrameric forms of the enzyme was found. However,the 5' end of the bex gene overlaps the 3' end of cdd by 20 nucleotidesand the SD-like sequence discussed above is part of the ribosome-bindingsite for initiation of bex translation (Fig. 1A). The bex geneencodes, in the +1 reading frame relative to cdd, a polypeptideof 301 amino acids. The deduced amino acid sequence of Bex has39% identity to the gene product of the E. coli era gene, whichencodes a membrane-bound G-protein essential for cell growth (1).The function of bex is unknown, but it has been shown to complementan era mutation in E. coli (33). The frameshift event may beexpected to cause a translating ribosome to pause in the SD region,thereby preventing initiation of bex translation. Accordingly,any physiological condition that affects frameshifting at thissite would be expected to influence bex expression. In that context,it should be recalled that B. subtilis is a differentiating eubacteriumand that developmental changes as well as changes in the growthconditions strongly influence the modification of tRNA in thisorganism (3). A search of the current databases revealed thatof the nine putative prokaryotic CDA genes recovered, only theB. subtilis cdd gene displayed the shifty CGA AAG motif at the3' end of the gene and only B. subtilis showed the overlappingorganization of cdd and bex (era). Furthermore, the search revealedin Archaeoglobus fulgidus, where the gene for 16S rRNA has thesequence CCTCCT at its 3' end, a GGAGG at nucleotide 7169 (16)followed 11 nucleotides 3' by CGA AAG. There is a potential initiationcodon in the preshift open reading frame followed by 61 codonsbefore the CGA AAG and then 101 codons in the $-$ 1 frame beforea stop codon. While in this case there is no indication that thisis even a real gene, an extensive search for the utilization ofCGA AAG-programmed frameshifting in gene expression seemsmerited.

	ACKNOWLEDGMENTS

We thank Frode Engbæk for facilitating the collaboration and Chad Nelson for mass spectrometry work. The help of Barry Mooreand Lisbeth Stauning is gratefullyacknowledged.

This work was funded by the Danish National Research Foundation to J.N. J.F.A. is funded by NIH grant GM48152 and was supportedby the Howard Hughes Medical Institute for part of thiswork.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biological Chemistry, Sølvgade 83, DK-1307 Copenhagen K, Denmark. Phone:(45) 35 32 20 02. Fax: (45) 35 32 20 40. E-mail: neuhard{at}mermaid.molbio.ku.dk.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Ahnn, J., P. E. March, H. E. Takiff, and M. Inouye. 1986. A GTP-binding protein of Escherichia coli has homology to yeast RAS proteins. Proc. Natl. Acad. Sci. USA 83:8849-8853[Abstract/Free Full Text].

2. Bertani, G. 1951. Studies of lysogenesis. I. The mode of phage liberation by lysogenic Escherichia coli. J. Bacteriol. 62:293-300[Free Full Text].

3. Björk, G. R., J. U. Ericson, C. E. Gustafsson, T. G. Hagervall, Y. H. Jönsson, and P. M. Wikström. 1987. Transfer RNA modification. Annu. Rev. Biochem. 56:263-287[Medline].

4. Blinkova, A. L., and J. R. Walker. 1990. Programmed ribosomal frameshifting generates the Escherichia coli DNA polymerase III $gamma$ subunit from within the $tau$ subunit reading frame. Nucleic Acids Res. 18:1725-1729[Abstract/Free Full Text].

5. Chandler, M., and O. Fayet. 1993. Translational frameshifting in the control of transposition in bacteria. Mol. Microbiol. 7:497-503[Medline].

6. Clark, D. J., and O. Maaløe. 1967. DNA replication and the cell division cycle in Escherichia coli. J. Mol. Biol. 2:99-112.

7. Cohen, R. M., and R. Wolfenden. 1971. Cytidine deaminase from Escherichia coli. Purification, properties, and inhibition by the potential transition state analog 3,4,5,6-tetrahydrouridine. J. Biol. Chem. 246:7561-7565[Abstract/Free Full Text].

8. Craigen, W. J., and C. T. Caskey. 1986. Expression of peptide chain release factor 2 requires high-efficiency frameshift. Nature 322:273-275[Medline].

9. Curran, J., and M. Yarus. 1988. Use of the tRNA suppressors to probe regulation of Escherichia coli release factor 2. J. Mol. Biol. 203:75-83[Medline].

10. Curran, J. F. 1995. Decoding with the A:I wobble pair is inefficient. Nucleic Acids Res. 23:683-688[Abstract/Free Full Text].

11. Farabaugh, P. J. 1996. Programmed translational frameshifting. Microbiol. Rev. 60:103-134[Free Full Text].

12. Flower, A. M., and C. S. McHenry. 1990. The gamma subunit of DNA polymerase III holoenzyme of Escherichia coli is produced by ribosomal frameshifting. Proc. Natl. Acad. Sci. USA 87:3713-3717[Abstract/Free Full Text].

13. Gesteland, R. F., and J. F. Atkins. 1996. Recoding: dynamic reprogramming of translation. Annu. Rev. Biochem. 65:741-768[Medline].

14. Gramstat, A., D. Prüfer, and W. Rohde. 1994. The nucleic acid-binding zinc finger protein of potato virus M is translated by internal initiation as well as by ribosomal frameshifting involving a shifty stop codon and a novel mechanism of P-site slippage. Nucleic Acids Res. 22:3911-3917[Abstract/Free Full Text].

15. Jacks, T., H. D. Madhani, F. R. Masiarz, and H. E. Varmus. 1988. Signals for ribosomal frameshifting in the Rous sarcoma virus gag-pol region. Cell 55:447-458[Medline].

16. Klenk, H.-P., R. A. Clayton, J.-F. Tomb, O. White, K. E. Nelson, et al. 1997. The complete genome sequence of the hyperthermophilic, sulphate-reducing archaeon Archaeoglobus fulgidus. Nature 390:364-370[Medline].

17. Komine, Y., T. Adachi, H. Inokuchi, and H. Ozeki. 1990. Genomic organization and physical mapping of the transfer RNA genes in Escherichia coli K12. J. Mol. Biol. 212:579-598[Medline].

18. Kunst, F., N. Ogasawara, I. Moszer, A. M. Albertini, G. Alloni, V. Azevedo, et al. 1997. The complete genome sequence of the gram-positive bacterium Bacillus subtilis. Nature 390:249-256[Medline].

19. Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 277:680-685.

20. Lagerkvist, U. 1978. "Two out of three": an alternative method for codon reading. Proc. Natl. Acad. Sci. USA 75:1759-1762[Abstract/Free Full Text].

21. Larsen, B., N. M. Wills, R. F. Gesteland, and J. F. Atkins. 1994. rRNA-mRNA base pairing stimulates a programmed $-$ 1 ribosomal frameshift. J. Bacteriol. 176:6842-6851[Abstract/Free Full Text].

22. Larsen, B., R. F. Gesteland, and J. F. Atkins. 1997. Structural probing and mutagenic analysis of the stem-loop required for Escherichia coli dnaX ribosomal frameshifting: programmed efficiency of 50%. J. Mol. Biol. 271:47-60[Medline].

23. Lim, V., and C. Venclovas. 1992. Codon-anticodon pairing. A model for interacting codon-anticodon duplexes located at the ribosomal A- and P-sites. FEBS Lett. 313:133-137[Medline].

24. Lustig, F., T. Borén, C. Claesson, C. Simonsen, M. Barciszewska, and U. Lagerkvist. 1993. The nucleotide in position 32 of the tRNA anticodon loop determines ability of anticodon UCC to discriminate among glycine codons. Proc. Natl. Acad. Sci. USA 90:3343-3347[Abstract/Free Full Text].

25. Lustig, F., P. Elias, T. Axberg, T. Samuelsson, I. Tittawella, and U. Lagerkvist. 1981. Codon reading and translational error. Reading of the glutamine and lysine codons during protein synthesis in vitro. J. Biol. Chem. 256:2635-2643[Abstract/Free Full Text].

26. Matsufuji, S., T. Matsufuji, Y. Miyazaki, Y. Murakami, J. F. Atkins, R. F. Gesteland, and S. Hayashi. 1995. Autoregulatory frameshifting in decoding mammalian ornithine decarboxylase antizyme. Cell 80:51-60[Medline].

27. McLaughlin, J. R., C. L. Murray, and J. C. Rabinowitz. 1981. Unique features in the ribosome binding site sequence of the gram-positive Staphylococcus aureus $beta$ -lactamase gene. J. Biol. Chem. 256:11283-11291[Abstract/Free Full Text].

28. Miller, J. 1972. Experiments in molecular genetics. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

29. Nilsson, J., S. Koskiniemi, K. Persson, B. Grahn, and I. Holm. 1997. Polyamines regulate both transcription and translation of the gene encoding ornithine decarboxylase antizyme in mouse. Eur. J. Biochem. 250:223-231[Medline].

30. O'Connor, M. 1998. tRNA imbalance promotes $-$ 1 frameshifting via near-cognate decoding. J. Mol. Biol. 279:727-736[Medline].

31. O'Connor, M., C. L. Thomas, R. A. Zimmermann, and A. E. Dahlberg. 1997. Decoding fidelity at the ribosomal A and P sites: influence of mutations in three different regions of the decoding domain in 16S rRNA. Nucleic Acids Res. 25:1185-1193[Abstract/Free Full Text].

32. Polard, P., M. F. Prère, M. Chandler, and O. Fayet. 1991. Programmed translational frameshifting and initiation at an AUU codon in gene expression of bacterial insertion sequence IS911. J. Mol. Biol. 222:465-477[Medline].

33. Powell, B. December 1994. Accession no. U18532. [Online.] http://www.embl-heidelberg.de/srs5/. [6 April 1999, last date accessed.]

34. Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

35. Sanger, J., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain-terminating inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].

36. Saxild, H. H., and P. Nygaard. 1987. Genetic and physiological characterization of Bacillus subtilis mutants resistant to purine analogs. J. Bacteriol. 169:2977-2983[Abstract/Free Full Text].

37. Song, B. H., and J. Neuhard. 1989. Chromosomal location, cloning and nucleotide sequence of the Bacillus subtilis cdd gene encoding cytidine/deoxycytidine deaminase. Mol. Gen. Genet. 216:462-468[Medline].

38. Tsuchihashi, Z. 1991. Translational frameshifting in the Escherichia coli dnaX gene in vitro. Nucleic Acids Res. 19:2457-2462[Abstract/Free Full Text].

39. Tsuchihashi, Z., and A. Kornberg. 1990. Translational frameshifting generates the gamma subunit of DNA polymerase III holoenzyme. Proc. Natl. Acad. Sci. USA 87:2516-2520[Abstract/Free Full Text].

40. Weiss, R. B., D. M. Dunn, J. F. Atkins, and R. F. Gesteland. 1987. Slippery runs, shifty stops, backward steps, and forward hops: $-$ 2, $-$ 1, +1, +2, +5, and +6 ribosomal frameshifting. Cold Spring Harbor Symp. Quant. Biol. 52:687-693[Abstract/Free Full Text].

41. Weiss, R. B., D. M. Dunn, A. E. Dahlberg, J. F. Atkins, and R. F. Gesteland. 1988. Reading frame switch caused by base-pair formation between the 3' end of 16S rRNA and the mRNA during elongation of protein synthesis in Escherichia coli. EMBO J. 7:1503-1507[Medline].

42. Yokoyama, S., T. Watanabe, K. Murao, H. Ishikura, Z. Yamaizumi, S. Nishimura, and T. Miyazawa. 1985. Molecular mechanism of codon recognition by tRNA species with modified uridine in the first position of the anticodon. Proc. Natl. Acad. Sci. USA 82:4905-4909[Abstract/Free Full Text].

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1.	Ahnn, J., P. E. March, H. E. Takiff, and M. Inouye. 1986. A GTP-binding protein of Escherichia coli has homology to yeast RAS proteins. Proc. Natl. Acad. Sci. USA 83:8849-8853[Abstract/Free Full Text].
2.	Bertani, G. 1951. Studies of lysogenesis. I. The mode of phage liberation by lysogenic Escherichia coli. J. Bacteriol. 62:293-300[Free Full Text].
3.	Björk, G. R., J. U. Ericson, C. E. Gustafsson, T. G. Hagervall, Y. H. Jönsson, and P. M. Wikström. 1987. Transfer RNA modification. Annu. Rev. Biochem. 56:263-287[Medline].
4.	Blinkova, A. L., and J. R. Walker. 1990. Programmed ribosomal frameshifting generates the Escherichia coli DNA polymerase III $gamma$ subunit from within the $tau$ subunit reading frame. Nucleic Acids Res. 18:1725-1729[Abstract/Free Full Text].
5.	Chandler, M., and O. Fayet. 1993. Translational frameshifting in the control of transposition in bacteria. Mol. Microbiol. 7:497-503[Medline].
6.	Clark, D. J., and O. Maaløe. 1967. DNA replication and the cell division cycle in Escherichia coli. J. Mol. Biol. 2:99-112.
7.	Cohen, R. M., and R. Wolfenden. 1971. Cytidine deaminase from Escherichia coli. Purification, properties, and inhibition by the potential transition state analog 3,4,5,6-tetrahydrouridine. J. Biol. Chem. 246:7561-7565[Abstract/Free Full Text].
8.	Craigen, W. J., and C. T. Caskey. 1986. Expression of peptide chain release factor 2 requires high-efficiency frameshift. Nature 322:273-275[Medline].
9.	Curran, J., and M. Yarus. 1988. Use of the tRNA suppressors to probe regulation of Escherichia coli release factor 2. J. Mol. Biol. 203:75-83[Medline].
10.	Curran, J. F. 1995. Decoding with the A:I wobble pair is inefficient. Nucleic Acids Res. 23:683-688[Abstract/Free Full Text].
11.	Farabaugh, P. J. 1996. Programmed translational frameshifting. Microbiol. Rev. 60:103-134[Free Full Text].
12.	Flower, A. M., and C. S. McHenry. 1990. The gamma subunit of DNA polymerase III holoenzyme of Escherichia coli is produced by ribosomal frameshifting. Proc. Natl. Acad. Sci. USA 87:3713-3717[Abstract/Free Full Text].
13.	Gesteland, R. F., and J. F. Atkins. 1996. Recoding: dynamic reprogramming of translation. Annu. Rev. Biochem. 65:741-768[Medline].
14.	Gramstat, A., D. Prüfer, and W. Rohde. 1994. The nucleic acid-binding zinc finger protein of potato virus M is translated by internal initiation as well as by ribosomal frameshifting involving a shifty stop codon and a novel mechanism of P-site slippage. Nucleic Acids Res. 22:3911-3917[Abstract/Free Full Text].
15.	Jacks, T., H. D. Madhani, F. R. Masiarz, and H. E. Varmus. 1988. Signals for ribosomal frameshifting in the Rous sarcoma virus gag-pol region. Cell 55:447-458[Medline].
16.	Klenk, H.-P., R. A. Clayton, J.-F. Tomb, O. White, K. E. Nelson, et al. 1997. The complete genome sequence of the hyperthermophilic, sulphate-reducing archaeon Archaeoglobus fulgidus. Nature 390:364-370[Medline].
17.	Komine, Y., T. Adachi, H. Inokuchi, and H. Ozeki. 1990. Genomic organization and physical mapping of the transfer RNA genes in Escherichia coli K12. J. Mol. Biol. 212:579-598[Medline].
18.	Kunst, F., N. Ogasawara, I. Moszer, A. M. Albertini, G. Alloni, V. Azevedo, et al. 1997. The complete genome sequence of the gram-positive bacterium Bacillus subtilis. Nature 390:249-256[Medline].
19.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 277:680-685.
20.	Lagerkvist, U. 1978. "Two out of three": an alternative method for codon reading. Proc. Natl. Acad. Sci. USA 75:1759-1762[Abstract/Free Full Text].
21.	Larsen, B., N. M. Wills, R. F. Gesteland, and J. F. Atkins. 1994. rRNA-mRNA base pairing stimulates a programmed $-$ 1 ribosomal frameshift. J. Bacteriol. 176:6842-6851[Abstract/Free Full Text].
22.	Larsen, B., R. F. Gesteland, and J. F. Atkins. 1997. Structural probing and mutagenic analysis of the stem-loop required for Escherichia coli dnaX ribosomal frameshifting: programmed efficiency of 50%. J. Mol. Biol. 271:47-60[Medline].
23.	Lim, V., and C. Venclovas. 1992. Codon-anticodon pairing. A model for interacting codon-anticodon duplexes located at the ribosomal A- and P-sites. FEBS Lett. 313:133-137[Medline].
24.	Lustig, F., T. Borén, C. Claesson, C. Simonsen, M. Barciszewska, and U. Lagerkvist. 1993. The nucleotide in position 32 of the tRNA anticodon loop determines ability of anticodon UCC to discriminate among glycine codons. Proc. Natl. Acad. Sci. USA 90:3343-3347[Abstract/Free Full Text].
25.	Lustig, F., P. Elias, T. Axberg, T. Samuelsson, I. Tittawella, and U. Lagerkvist. 1981. Codon reading and translational error. Reading of the glutamine and lysine codons during protein synthesis in vitro. J. Biol. Chem. 256:2635-2643[Abstract/Free Full Text].
26.	Matsufuji, S., T. Matsufuji, Y. Miyazaki, Y. Murakami, J. F. Atkins, R. F. Gesteland, and S. Hayashi. 1995. Autoregulatory frameshifting in decoding mammalian ornithine decarboxylase antizyme. Cell 80:51-60[Medline].
27.	McLaughlin, J. R., C. L. Murray, and J. C. Rabinowitz. 1981. Unique features in the ribosome binding site sequence of the gram-positive Staphylococcus aureus $beta$ -lactamase gene. J. Biol. Chem. 256:11283-11291[Abstract/Free Full Text].
28.	Miller, J. 1972. Experiments in molecular genetics. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
29.	Nilsson, J., S. Koskiniemi, K. Persson, B. Grahn, and I. Holm. 1997. Polyamines regulate both transcription and translation of the gene encoding ornithine decarboxylase antizyme in mouse. Eur. J. Biochem. 250:223-231[Medline].
30.	O'Connor, M. 1998. tRNA imbalance promotes $-$ 1 frameshifting via near-cognate decoding. J. Mol. Biol. 279:727-736[Medline].
31.	O'Connor, M., C. L. Thomas, R. A. Zimmermann, and A. E. Dahlberg. 1997. Decoding fidelity at the ribosomal A and P sites: influence of mutations in three different regions of the decoding domain in 16S rRNA. Nucleic Acids Res. 25:1185-1193[Abstract/Free Full Text].
32.	Polard, P., M. F. Prère, M. Chandler, and O. Fayet. 1991. Programmed translational frameshifting and initiation at an AUU codon in gene expression of bacterial insertion sequence IS911. J. Mol. Biol. 222:465-477[Medline].
33.	Powell, B. December 1994. Accession no. U18532. [Online.] http://www.embl-heidelberg.de/srs5/. [6 April 1999, last date accessed.]
34.	Sambrook, J., E. F. Fritsch, and T. Maniatis. 1989. Molecular cloning: a laboratory manual, 2nd ed. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
35.	Sanger, J., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain-terminating inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].
36.	Saxild, H. H., and P. Nygaard. 1987. Genetic and physiological characterization of Bacillus subtilis mutants resistant to purine analogs. J. Bacteriol. 169:2977-2983[Abstract/Free Full Text].
37.	Song, B. H., and J. Neuhard. 1989. Chromosomal location, cloning and nucleotide sequence of the Bacillus subtilis cdd gene encoding cytidine/deoxycytidine deaminase. Mol. Gen. Genet. 216:462-468[Medline].
38.	Tsuchihashi, Z. 1991. Translational frameshifting in the Escherichia coli dnaX gene in vitro. Nucleic Acids Res. 19:2457-2462[Abstract/Free Full Text].
39.	Tsuchihashi, Z., and A. Kornberg. 1990. Translational frameshifting generates the gamma subunit of DNA polymerase III holoenzyme. Proc. Natl. Acad. Sci. USA 87:2516-2520[Abstract/Free Full Text].
40.	Weiss, R. B., D. M. Dunn, J. F. Atkins, and R. F. Gesteland. 1987. Slippery runs, shifty stops, backward steps, and forward hops: $-$ 2, $-$ 1, +1, +2, +5, and +6 ribosomal frameshifting. Cold Spring Harbor Symp. Quant. Biol. 52:687-693[Abstract/Free Full Text].
41.	Weiss, R. B., D. M. Dunn, A. E. Dahlberg, J. F. Atkins, and R. F. Gesteland. 1988. Reading frame switch caused by base-pair formation between the 3' end of 16S rRNA and the mRNA during elongation of protein synthesis in Escherichia coli. EMBO J. 7:1503-1507[Medline].
42.	Yokoyama, S., T. Watanabe, K. Murao, H. Ishikura, Z. Yamaizumi, S. Nishimura, and T. Miyazawa. 1985. Molecular mechanism of codon recognition by tRNA species with modified uridine in the first position of the anticodon. Proc. Natl. Acad. Sci. USA 82:4905-4909[Abstract/Free Full Text].

Ribosomal 1 Frameshifting during Decoding of Bacillus subtilis cdd Occurs at the Sequence CGA AAG

Ribosomal $-$ 1 Frameshifting during Decoding of Bacillus subtilis cdd Occurs at the Sequence CGA AAG