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Journal of Bacteriology, January 2004, p. 8-14, Vol. 186, No. 1
0021-9193/04/$08.00+0     DOI: 10.1128/JB.186.1.8-14.2004
Copyright © 2004, American Society for Microbiology. All Rights Reserved.

Cysteinyl-tRNA^Cys Formation in Methanocaldococcus jannaschii: the Mechanism Is Still Unknown

Benfang Ruan,^1, Hiroaki Nakano,^1, Masashi Tanaka,² Jonathan A. Mills,^3, Joseph A. DeVito,^3, Bokkee Min,¹ K. Brooks Low,⁴ John R. Battista,² and Dieter Söll^1,5*

Departments of Molecular Biophysics and Biochemistry,¹ Chemistry,⁵ Therapeutic Radiology, Yale University, New Haven, Connecticut 06520-8114,⁴ Department of Biological Sciences, Louisiana State University, Baton Rouge, Louisiana 70803,² DuPont Pharmaceuticals Company, Wilmington, Delaware 19801³

Received 31 July 2003/ Accepted 2 October 2003

	ABSTRACT

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Most organisms form Cys-tRNA^Cys, an essential component for protein synthesis, through the action of cysteinyl-tRNA synthetase (CysRS). However, the genomes of Methanocaldococcus jannaschii, Methanothermobacter thermautotrophicus, and Methanopyrus kandleri do not contain a recognizable cysS gene encoding CysRS. It was reported that M. jannaschii prolyl-tRNA synthetase (C. Stathopoulos, T. Li, R. Longman, U. C. Vothknecht, H. D. Becker, M. Ibba, and D. Söll, Science 287:479-482, 2000; R. S. Lipman, K. R. Sowers, and Y. M. Hou, Biochemistry 39:7792-7798, 2000) or the M. jannaschii MJ1477 protein (C. Fabrega, M. A. Farrow, B. Mukhopadhyay, V. de Crécy-Lagard, A. R. Ortiz, and P. Schimmel, Nature 411:110-114, 2001) provides the "missing" CysRS activity for in vivo Cys-tRNA^Cys formation. These conclusions were supported by complementation of temperature-sensitive Escherichia coli cysS(Ts) strain UQ818 with archaeal proS genes (encoding prolyl-tRNA synthetase) or with the Deinococcus radiodurans DR0705 gene, the ortholog of the MJ1477 gene. Here we show that E. coli UQ818 harbors a mutation (V27E) in CysRS; the largest differences compared to the wild-type enzyme are a fourfold increase in the K_m for cysteine and a ninefold reduction in the k_cat for ATP. While transformants of E. coli UQ818 with archaeal and bacterial cysS genes grew at a nonpermissive temperature, growth was also supported by elevated intracellular cysteine levels, e.g., by transformation with an E. coli cysE allele (encoding serine acetyltransferase) or by the addition of cysteine to the culture medium. An E. coli cysS deletion strain permitted a stringent complementation test; growth could be supported only by archaeal or bacterial cysS genes and not by archaeal proS genes or the D. radiodurans DR0705 gene. Construction of a D. radiodurans DR0705 deletion strain showed this gene to be dispensable. However, attempts to delete D. radiodurans cysS failed, suggesting that this is an essential Deinococcus gene. These results imply that it is not established that proS or MJ1477 gene products catalyze Cys-tRNA^Cys synthesis in M. jannaschii. Thus, the mechanism of Cys-tRNA^Cys formation in M. jannaschii still remains to be discovered.

	INTRODUCTION

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Cysteinyl-tRNA synthetase (CysRS), a highly conserved essential enzyme, is a key component in protein biosynthesis. It is the smallest monomeric class I aminoacyl-tRNA synthetase (14, 20). A recent determination of the crystal structure of Escherichia coli CysRS (30) revealed that a zinc ion positioned at the active site is responsible for the precise binding of the substrate cysteine. This metal ion coordinates with the side chains of Cys28, Cys209, His234, and Glu238 (30). CysRS is well conserved in all three domains of life; phylogenetic studies suggest a transfer of cysS from bacteria to some archaea (24). Based on the knowledge of a large number of complete organism genomes, it is clear that only three methanogenic archaea, Methanocaldococcus jannaschii (8), Methanothermobacter thermautotrophicus (33), and Methanopyrus kandleri (32), do not contain an open reading frame (ORF) resembling that for CysRS.

How is Cys-tRNA^Cys formed in these methanogenic archaea? One apparent answer came from reports that archaeal prolyl-tRNA synthetases (ProRSs) could form Cys-tRNA^Cys in addition to Pro-tRNA^Pro (26, 35). Apart from biochemical data, the conclusion was based on the persuasive in vivo result (35) that the M. jannaschii, M. thermautotrophicus, and Methanococcus maripaludis proS genes could restore the growth, albeit weakly, of temperature-sensitive E. coli cysS(Ts) strain UQ818 (5) at a nonpermissive temperature. Poor growth of the transformed strains was attributed to slow translation in E. coli of the large number of AGA codons present in the archaeal proS genes (35). A different route to archaeal Cys-tRNA^Cys formation was proposed on the basis of the existence of an unusual aminoacyl-tRNA synthetase that lacks the typical features of class I and class II synthetases and is encoded by the M. jannaschii MJ1477 ORF (15). The heterologously expressed MJ1477 protein was shown to cysteinylate in vitro both M. jannaschii total tRNA and purified E. coli tRNA^Cys, but the MJ1477 gene could not rescue the growth of E. coli cysS(Ts) strain UQ818 (15). Instead, DR0705, the Deinococcus radiodurans ortholog of MJ1477, was shown to complement strain UQ818. While these data suggested that MJ1477 provides Cys-tRNA^Cys in M. jannaschii, MJ1477 orthologs are not present in the genomes of M. thermautotrophicus (33) or the viable cysS deletion strain (36) of M. maripaludis (J. Leigh, unpublished data).

In both of the above-mentioned studies (15, 35), the conclusions were based on the weak complementation of E. coli strain UQ818 by the archaeal proS genes or the D. radiodurans DR0705 gene. E. coli UQ818 has a thermolabile CysRS; cell extracts display little CysRS activity at 33°C (5). Strain UQ818 does not grow at the nonpermissive temperature of 41°C but does grow after complementation with cysS genes from E. coli (14, 20) or from M. maripaludis or Methanosarcina barkeri (24). A characterization of the cysS mutation in strain UQ818 has not been reported.

Although the finding that archaeal ProRSs form Cys-tRNA^Cys has been reported repeatedly (9, 26, 27, 34, 35), a biochemical reexamination of the amino acid recognition of ProRS enzymes showed that cysteine charging in vitro is a property of ProRS enzymes from all domains (1); however, the reaction product is the misacylated Cys-tRNA^Pro species (2). Therefore, we wanted to further examine the in vivo complementation of E. coli cysS(Ts) strain UQ818 and to analyze the complementation of an E. coli cysS deletion strain (cysS). In addition, we attempted to evaluate the physiological significance of DR0705 by using a gene deletion in D. radiodurans (3).

	MATERIALS AND METHODS

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General. [³⁵S]Cysteine (1,075 Ci/mmol) was purchased from Perkin-Elmer Life Sciences (Boston, Mass.). [¹⁴C]Serine (155 mCi/mmol) was obtained from Amersham Pharmacia Biotech (Little Chalfont, United Kingdom). E. coli total tRNA was obtained from Sigma (St. Louis, Mo.), and the TOPO-TA cloning kit was obtained from Invitrogen (Carlsbad, Calif.). Oligonucleotide synthesis and DNA sequencing were performed at the Keck Foundation Research Biotechnology Resource Laboratory at Yale University (New Haven, Conn.). Protein concentrations were determined by the method of Bradford (6) with bovine serum albumin as a standard.

Plasmids, strains, and culture medium. Table 1 lists the plasmids and strains used in this study. Primers were designed to PCR amplify each ORF and introduce the desired restriction sites. The forward primers contained a restriction site and 20 nucleotides identical to the start sequence of the 5' end; the reverse primers contained a restriction site and 20 nucleotides complementary to the sequence of the 3' end. Standard PCR procedures were used to generate the coding sequences of the M. jannaschii proS, M. maripaludis proS and cysS, D. radiodurans DR0705 and cysS, and E. coli cysE and cysS genes from their corresponding genomic DNAs. The amplified coding sequences were cloned into the pCR2.1-TOPO vector. After verification of the DNA sequences, the genes were subcloned into the desired vector. For in vivo complementation, the genes were subcloned into the pCYB1 vector between the NdeI and BamHI sites under the control of an isopropyl-ß-D-thiogalactopyranoside (IPTG)-inducible tac promoter. An E. coli cysE mutant allele, cysEM256I (10), was generated by PCR mutagenesis of the cysE gene (created above) with primers that contained the corresponding mutation.

The M. jannaschii tRNA^Cys gene behind the lpp promoter was subcloned from pTech-Mj-tRNA^Cys (35) into pACYC184 by using restriction enzymes AvaI and BstZ171. This procedure removed the cat gene from pACYC184. The resulting plasmid, pACYC-Tc-Mj-tRNA^Cys, confers tetracycline resistance.

The following antibiotics at the concentrations indicated were used in Luria-Bertani (LB) medium (31): ampicillin (100 µg/ml), chloramphenicol (34 µg/ml), kanamycin (20 µg/ml), and tetracycline (20 µg/ml). The final concentrations of arabinose and isopropyl-ß-D-thiogalactopyranoside (IPTG) in the culture medium were 0.02% and 1 mM, respectively.

Cloning of E. coli cysS genes and purification of CysRS enzymes. Genomic DNA of E. coli strain W3110 or UQ818 was used. PCR primers were designed to amplify the cysS ORF, and the resulting DNA fragment was cloned into the pET15b vector at the NdeI and BamHI sites for expression of proteins as N-terminal His₆-tagged proteins. These pET15b-cysS clones were transformed into E. coli BL21(DE3) cells, and the transformants were grown in 500 ml of LB-ampicillin medium to a cell density (A₆₀₀) of 0.4. At this point, cysS expression was induced with 1 mM IPTG treatment for 2 h. Cells were harvested and lysed, and wild-type and mutant His₆-CysRS proteins were purified from cell extracts by Ni-nitrilotriacetic acid-agarose chromatography as described in the Qiagen (Valencia, Calif.) protein purification manual. Both proteins were judged to be >95% pure by sodium dodecyl sulfate-polyacrylamide gel electrophoresis after Coomassie brilliant blue staining. Active-site titration showed that the CysRS and CysRSV27E (CysRS with a V27E mutation) preparations contained 100 and 52% active enzymes, respectively. These values were used to determine enzyme concentrations for the calculation of k_cat. The enzymes were stored in 10% glycerol in 50 mM HEPES-KOH (pH 7.0)-50 mM KCl-15 mM MgCl2-5 mM dithiothreitol at -20°C.

Assay for CysRS activity. Cys-tRNA formation was measured as acid-precipitable radioactivity as described previously (1). The standard reaction mixture contained 50 mM HEPES-KOH (pH 7.0), 50 mM KCl, 15 mM MgCl₂, 5 mM dithiothreitol, 10 mM ATP, 0.2 mM [³⁵S]cysteine, and 10 mg of unfractionated E. coli tRNA/ml (unless specified otherwise) in a final volume of 0.1 ml. The final enzyme concentrations were 0.37 nM for CysRS and 1.6 nM for CysRSV27E. Initial velocities were measured at 30°C. The substrate concentrations ranged from 0.01 to 20 times the K_m values, and the experiments were done in triplicate.

Active-site titration of CysRS enzymes. CysRS preparations were incubated at 30°C in 100 mM Tris-HCl (pH 7.5)-10 mM KCl-10 mM MgCl₂-4 mM ATP (pH 7)-200 µM [³⁵S]cysteine (650 cpm/pmol)-5 mM dithiothreitol-1 U of inorganic pyrophosphatase in a total volume of 0.1 ml. Aliquots (25 µl) were used at various times for active-site titration as described previously (1).

Growth of E. coli UQ818 at nonpermissive temperatures under various conditions. A cysteine gradient plate (12) was used to show the growth of UQ818 at nonpermissive temperatures in the presence of cysteine. UQ818 cells were grown overnight in LB medium. A 10^-4 dilution of the overnight culture (0.1 ml) was spread on a plate (1% Bacto Tryptone, 0.5% sodium chloride, 1.5% agar). After the plate was dried, an aliquot (0.15 ml) of cysteine (0.4 M) was placed in a central well, and the plate was incubated for 2 days at 41°C.

In order to evaluate the growth restored by cysEM256I, UQ818 was transformed with pCYB1, pCYB-ECcysS, pCYB-cysEM256I, or pCYB-MMcysS. The transformants were cultured overnight in LB-ampicillin medium, and the liquid cultures (one loop) were streaked on LB-ampicillin agar plates containing 1 mM IPTG. The plates were grown at 30 or 41°C for 2 days.

In order to compare the growth restored by various genes, we measured at 42°C the growth curves for W3110 cells and UQ818 cells transformed with pCYB-ECcysS, pCYB-MMcysS, pCYB-DR0705, pCYB-MMproS, pCYB-MJproS, pCYB-ECcysEM256I, or pCYB1. UQ818 transformants with archaeal proS genes also contained an M. jannaschii tRNA^Cys gene (35). Each strain from an overnight culture was inoculated into LB medium with antibiotics and IPTG in triplicate and grown at 42°C for 8 h. Aliquots (1 ml) were taken every 0.5 h to measure the A₆₀₀.

Construction of an E. coli cysS chromosomal deletion strain. An E. coli chromosomal deletion strain was constructed by using the generalized recombination system of bacteriophage (39). The cysS gene was expressed from an arabinose regulon on pBADbrcysS, while the chromosomal cysS copy in E. coli strain EC723 was replaced with a lox-kan cassette (18). The details of strain construction were adapted from the method of Yu et al. (39). The genomic DNA of E. coli strain EC400 served as the template for PCR amplification of the lox²-kan cassette (11), and the resulting cassette was flanked with 50-bp sequences identical to those found in the upstream and downstream regions of the cysS gene. The deletion cassette was transformed into heat-shocked (15 min) E. coli strain EC723 containing a rescue plasmid, pBADbrcysS. Transformants were selected on kanamycin plates, and strains containing a cysS chromosomal deletion were screened by PCR and nucleotide sequencing.

Plasmid exchange experiments with the E. coli cysS chromosomal deletion strain. The cysS chromosomal deletion strain was further transformed with pACYC-Tc-Mj-tRNA^Cys, which provides M. jannaschii tRNA^Cys for M. jannaschii cysS to function in E. coli (35). The resulting strain was transformed by electroporation (31) with pCYB derivative plasmids (50 ng) containing cysS or other genes at 30°C to prevent lysis of the host (39). Transformants were cultured in LB medium containing kanamycin and tetracycline for 60 min, and then a series of dilutions of the transformants were spread on LB agar plates containing kanamycin, tetracycline, ampicillin, L-arabinose, and IPTG. Cells were grown at 30°C for 1 day, and the numbers of ampicillin-resistant colonies were counted. Colonies then were replicated to LB agar plates containing either chloramphenicol (34 µg/ml) or ampicillin (50 µg/ml) and also containing kanamycin, tetracycline, L-arabinose, and IPTG. After 24 h of incubation, the growth of the replicants was checked.

Construction of plasmids for use in deleting DR0705 and cysS (DR1670) from the D. radiodurans R1 genome. The plasmid used for DR0705 deletion, pTNK301 (carrying the DR0705 deletion cassette) (Fig. 1B), was generated in a three-step process by splicing by overlap extension (13, 19). The Tn903 neomycin phosphotransferase gene (npt) was fused to a 120-bp sequence upstream of the initiation codon of the D. radiodurans R1 katA gene (PkatA in Fig. 1) (16). The primers shown in Fig. 1B were used for PCR to amplify the 806-bp sequence immediately downstream of the DR0705 termination codon and the 971-bp sequence upstream of the DR0705 initiation codon and for PCR to splice both fragments to the PkatA-npt cassette. The resulting cassette was cloned into pGEM-T to give pTNK301 for DR0705 deletion.

View larger version (26K): [in this window] [in a new window]   FIG. 1. Scheme of cassette constructs for Deinococcus gene deletions. (A) DR0705 in the D. radiodurans R1 chromosome. (B) DR0705 deletion cassette. (C) DR1670 deletion cassette. Primers indicated above or below the cassette were used for PCR. Sections of the diagrams are labeled as follows: A upstream, 971 bp immediately upstream of the initiation codon of DR0705; A downstream, 806 bp immediately downstream of the termination codon of DR0705; B upstream, 886 bp immediately upstream of the initiation codon of DR1670; B downstream, 957 bp immediately downstream of the termination codon of DR1670.

Deletion of DR0705 from D. radiodurans R1. DR0705 was disrupted by targeted mutagenesis as described previously (13). The DR0705 deletion cassette (Fig. 1B) was transformed into an exponential-phase D. radiodurans R1 culture, and the recombinants were selected on tryptone-glucose-yeast extract (TGY) plates containing kanamycin (10 µg/ml). Since D. radiodurans is multigenomic, individual colonies had to be screened to determine whether they were homozygous for the disruption. Genomic DNAs of the individual recombinants were extracted and subjected to PCR analysis for the existence of wild-type DR0705 or the deletion cassette. Briefly, putative deletion mutants were subjected to PCR amplification for wild-type DR0705 with primers AFW4 and ARV4 (Fig. 1A). No PCR product should be obtained if DR0705 has been deleted. To verify the disruption, genomic DNAs from D. radiodurans R1 and the DR0705 deletion strain were PCR amplified to obtain DNA fragments of the deletion region with primers AFW2 and ARV3 (Fig. 1A and B), and the amplified DNA fragments (2.7 kb) were further subjected to HindIII and XhoI digestions. The npt gene-containing fragments should be cut in half, because the npt gene, but not DR0705, contains single restriction sites for HindIII and XhoI.

Deletion of cysS from D. radiodurans R1. The cysS (DR1670) deletion cassette (Fig. 1C) was transformed into exponential-phase D. radiodurans R1 cells by the CaCl₂ method (13). The culture was spread on TGY plates containing chloramphenicol (3 µg/ml) and incubated at 30°C. Recombinants were observed on these plates within 6 days. Candidates were purified in three rounds of single-colony isolation. Then, chloramphenicol-resistant colonies were PCR screened for the loss of cysS by using genomic DNA isolated from each candidate.

	RESULTS

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The mutant CysRS in strain UQ818 is defective in cysteine binding. E. coli strain UQ818 was isolated as a spontaneous temperature-sensitive mutant and lacks CysRS activity in vitro at 42°C (5). In order to characterize the CysRS in this strain, we cloned and sequenced the cysS(Ts) gene. We found a single nucleotide change (TA at position 80) leading to a VE change at position 27 of the CysRS protein. Sequence alignment of 76 canonical CysRS proteins showed that valine is the most abundant amino acid at position 27 (in 51 out of 76 proteins), the other amino acids being leucine, threonine, cysteine, alanine, tyrosine, asparagine, and glycine.

To understand the effect of the V27E mutation on cysteinylation, the N-terminal His₆-tagged CysRS and CysRSV27E enzymes were overexpressed and purified on an Ni-nitrilotriacetic acid matrix. Aminoacylation kinetics were determined at 30°C, a temperature at which the CysRSV27E enzyme retains activity. The results (Table 2) indicated a significant difference in the K_m values for cysteine (7.2 and 28.2 µM, respectively). The K_m values for the other substrates, tRNA and ATP, did not differ significantly for the mutant and wild-type enzymes. However, the k_cat values for both substrates were about four- to ninefold lower in the mutant, with a ninefold decrease in the value for ATP. Kinetic constants for other CysRS enzymes were determined earlier by ATP-PP_i exchange (23, 29); thus, they are not strictly comparable to our aminoacylation data. However, our values are in the range of values reported for CysRS enzymes from E. coli (0.4 µM for tRNA^Cys), mammals (0.8 µM for tRNA^Cys, 800 µM for ATP, and 11 µM for cysteine), and yeasts (0.54 µM for tRNA^Cys, 80 µM for ATP, and 8 µM for cysteine). The V27E mutation does not affect the discrimination of the enzyme for serine, which was not charged by either wild-type or mutant CysRS (data not shown).

View larger version (139K): [in this window] [in a new window]   FIG. 2. Growth of E. coli cysS(Ts) strain UQ818 at 41°C on a cysteine gradient plate. The highest cysteine concentration is in the well (see Materials and Methods).

View larger version (85K): [in this window] [in a new window]   FIG. 3. Complementation of E. coli cysS(Ts) strain UQ818 with pCYB1, pCYB-ECcysS, pCYB-cysEM256I, or pCYB-MMcysS. LB agar containing ampicillin and IPTG was used for growth at 41°C (see Materials and Methods).

Only canonical cysS genes restore CysRS function to an E. coli cysS deletion strain. Because complementation of the cysS(Ts) gene in strain UQ818 is fraught with pitfalls, we constructed an E. coli cysS chromosomal deletion strain in order to perform an unambiguous test. Survival of a cysS deletion strain can be maintained with a rescue plasmid carrying E. coli cysS. This chloramphenicol-resistant plasmid, pBADbrcysS, can be replaced by transformation and selection for an incompatible plasmid carrying a functional cysS gene. We have constructed such incompatible plasmids (pCYB derivatives) that are ampicillin resistant. The pCYB plasmids contain various ORFs in order to test their ability to complement the E. coli cysS deletion strain. Upon transformation of the deletion strain, cells carrying only a pCYB plasmid (pBADbrcysS being lost due to plasmid incompatibility) would be chloramphenicol sensitive. Cells still containing both plasmids would be ampicillin and chloramphenicol resistant. Therefore, the CysRS activity encoded by genes cloned into pCYB can be assessed by their ability to replace the pBADbrcysS rescue plasmid in the E. coli cysS deletion strain.

pCYB transformants of the cysS strain were selected on ampicillin and then screened for chloramphenicol sensitivity to assess the efficiency of plasmid exchange. When pCYB plasmids containing cysS genes from E. coli or M. maripaludis were tested, transformation efficiencies were increased and the efficiency of plasmid exchange was high (Table 3). Even though the same amount of plasmid DNA (50 ng) was used for transformation of the same batch of competent E. coli cysS cells, the number of transformants was greatly reduced in the cysS strain when pCYB plasmids without functional cysS genes were introduced (Table 3). Presumably, selection against the pBADbrcysS rescue plasmid did not allow enough cysS to be expressed for functional complementation of the cysS chromosomal deletion. When the transformants were tested for chloramphenicol resistance, >90% of the proS or DR0705 transformants retained the pBADbrcysS rescue plasmid (Table 3); this result indicates that proS or DR0705 does not provide cysS function. Thus, proS and DR0705 do not encode a CysRS that is functional in E. coli.

View this table: [in this window] [in a new window]   TABLE 3. Plasmid exchange in the E. coli cysS straina

View larger version (73K): [in this window] [in a new window]   FIG. 4. Replacement of the D. radiodurans DR0705 gene with the PkatA-npt cassette. Lanes 1 and 10, DNA size markers; lanes 2, 4, 6, and 8, DNA from D. radiodurans R1; lanes 3, 5, 7, and 9, DNA from DR0705 deletion strain TNK201. Lanes: 2 and 3, PCR products of primers AFW4 and ARV4; 4 and 5, PCR products of primers AFW2 and ARV3; 6 and 7, HindIII digestion of DNA in lanes 4 and 5, respectively; 8 and 9, XhoI digestion of DNA in lanes 4 and 5, respectively. DR0705 has no restriction sites for HindIII and XhoI, while the npt gene is cut once by both enzymes.

	DISCUSSION

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The work presented here examined the earlier interpretation (9, 26, 27, 34, 35) of the data on Cys-tRNA^Cys formation in archaea. In vitro evidence has clearly shown that the ProRS enzymes from all three domains of life can charge cysteine to tRNA (1, 2). Even though the ProRS enzymes lack the amino acid landscape of the extremely conserved cysteine binding pocket of the canonical CysRS enzymes (30), the crystal structure of M. thermautotrophicus ProRS showed efficient binding of cysteine to the active site of the enzyme (22). However, the specificity for cognate tRNA prevails, and ProRS generates misacylated Cys-tRNA^Pro, which is not edited by the enzyme (1, 2, 4, 27).

Thus, we looked for an explanation for the successful in vivo rescue of the temperature-sensitive cysS phenotype by complementation with archaeal proS genes (9, 35). It had already been reported (7, 38) that rescue of a temperature-sensitive aminoacyl-tRNA synthetase phenotype can occur through factors other than the wild-type gene product. For instance, partial suppression of a temperature-sensitive E. coli valyl-tRNA synthetase strain by ribosomal protein mutations was reported (7, 38). Such mutations or metabolic changes slow down the growth rate suitably so that the mutant synthetase at the nonpermissive temperature is able to provide sufficient aminoacyl-tRNA for adequate protein synthesis and cell survival. Stabilization of the mutant CysRS in strain UQ818 through increased cysteine levels or through interactions with other proteins may yield the same result. Therefore, the inability of archaeal proS genes to restore viability to the E. coli cysS strain indicates that archaeal proS genes do not generate Cys-tRNA^Cys, at least in E. coli. While all of the published data combined do not rule out the possibility that ProRS synthesizes some correctly charged Cys-tRNA, the conclusion (9, 35) that ProRS can form Cys-tRNA^Cys in vivo is not established. Therefore, we assume that archaeal ProRS does not supply Cys-tRNA^Cys in M. jannaschii. Whether this enzyme can provide this function with the help of an additional protein(s) is an open question (25).

The above findings may also explain the observation that the D. radiodurans DR0705 gene rescued the temperature-sensitive phenotype of strain UQ818 (15), even though this gene did not restore the growth of the E. coli cysS strain. The fact that the DR0705 gene can be deleted from D. radiodurans without any effect on growth shows that its gene product is not required for the viability of the organism. However, attempts to delete the canonical cysS gene did not result in a viable strain, suggesting that CysRS is indeed a required enzyme in D. radiodurans. Unfortunately, genetic methods to establish unambiguously the essentiality of a gene do not yet exist for D. radiodurans.

Although the product of M. jannaschii MJ1477 ORF cysteinylates the homologous tRNA with cysteine in vitro (15), the nature of this protein as CysRS has been questioned by extensive computational analyses that instead predict a secreted polygalactosaminidase or a related polysaccharide hydrolase (21, 28). Moreover, no MJ1477 orthologs are present in the completed genome sequences of the methanogens M. thermautotrophicus (33) and M. maripaludis (Leigh, unpublished); the former organism contains no canonical cysS gene, while a viable cysS deletion strain of M. maripaludis exists (36). Therefore, MJ1477 cannot explain the lack of cysS in M. thermautotrophicus. Given the results of the different lines of experimentation, it cannot be convincingly deduced that the MJ1477 and DR0705 proteins function as CysRS enzymes.

All of these data compel us to conclude that the mechanism of Cys-tRNA^Cys formation in M. jannaschii is still unknown.

	ACKNOWLEDGMENTS

 
We are indebted to Sotiria Palioura, Veronica Liu, and Anjana Agarwal for help with some experiments.

This work was supported by grants from the National Institute of General Medical Sciences (to D.S.), the Department of Energy (to J.R.B. and D.S.), and the National Aeronautics and Space Administration (to D.S.).

	FOOTNOTES

 
* Corresponding author. Mailing address: Department of Molecular Biophysics and Biochemistry, Yale University, P.O. Box 208114, 266 Whitney Ave., New Haven, CT 06520-8114. Phone: (203) 432-6200. Fax: (203) 432-6202. E-mail: soll{at}trna.chem.yale.edu.

B.R. and H.N. contributed equally to the work described in this report.

Present address: Symyx Technologies, Santa Clara, CA 95051.

Present address: Rib-X Pharmaceuticals, Inc., New Haven, CT 06511.

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Top Abstract Introduction Materials and Methods Results Discussion References

 

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