1 National Food Research Institute, 2112, Kannon-dai, Tsukuba, Ibaraki 305-8642 and 2 Central Research Laboratories, Ajinomoto Co., Inc., 11, Suzuki-cho, Kawasaki-ku, Kawasaki, Kanagawa 210-8681, Japan
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Abstract |
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Keywords: codon usage/CUG codon/killer toxin/Pichia farinosa/Pichia sorbitophila
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Introduction |
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Kawaguchi et al. demonstrated that the CUG codon is translated as Ser in Candida cylindracea (Kawaguchi et al., 1989). To date, it has been shown by in vitro translation experiments that 77 species and seven varieties of Candida species used codon CUG as Ser, including Candida cacaoi, the anamorph of P.farinosa. Non-universal decoding is widely distributed not only in Candida species but also in hemiascomycetous yeasts (Sugita and Nakase, 1999
). By inferring the genetic code from the frequencies of Saccharomyces cerevisiae amino acids corresponding to each codon obtained by the Hemiascomycete random sequence tag project, it was pointed out that the CUG codon is used to specify Ser instead of Leu in Pichia sorbitophila, a synonym of P.farinosa (Tekaia et al., 2000
). However, there is no in vivo evidence that the CUG codon is translated as Ser in P.farinosa.
We have recently demonstrated that the expression of SMK1 under the control of a galactose-inducible promoter is lethal in wild-type cells of S. cerevisiae (Suzuki et al., 2000). We also showed that spf1 disruptant cells lacking a P-type ATPase Spf1p is highly resistant to both exogenous SMKT and endogenously expressed SMK1 products (Suzuki et al., 2000
). Heterologous expression with the CUG codon in S.cerevisiae, which uses the universal genetic code, would substitute the strongly hydrophobic Leu for polar Ser, which might perturb the three-dimensional structure of the protein or alter its activity or stability. On the other hand, CUG encoding Ser residues are found at non-essential surface sites in some cases (Cutfield et al., 2000
). It is therefore necessary to evaluate whether the lethal effect of the SMK1 product in S.cerevisiae is caused by substitutions of the authentic Ser residues specified by the CUG codons for Leu.
In this paper, we provide in vivo evidence that the CUG codon is translated as unmodified Ser in P. farinosa. The expression of authentic SMK1 product by mutating the CUG codons to universal Ser codons was still lethal in S.cerevisiae but the secretion of authentic SMK1 product was more effective. Our results suggest that CUG encoding Ser residues in the region may be involved in the stability of protoxin.
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Materials and methods |
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P. farinosa (NFRI 3621) (Suzuki and Nikkuni, 1989), Saccharomyces cerevisiae W3031A (MATa ade2-1 his3-4, 15 leu2-3, 112 trp1-1 ura3-1 can1-100) and CS701C (spf1::LEU2 in W303A-1A background) (Suzuki and Shimma, 1999
) were used. YPD and YPGal/MB selective media were as described previously (Suzuki et al., 2000
).
Purification of SMKT and protoxin
SMKT was purified as described previously (Suzuki and Nikkuni, 1994). SMKT concentrations were determined from the UV absorption at 280 nm with
280 = 2.8x104 M1 cm1. Protoxin gp26 was purified as described previously (Suzuki, 1999
).
Amino acid sequence analysis of lysylendopeptidase fragments of SMKT and protoxin was performed as described previously (Suzuki, 1999).
Mass spectrometry
The electrospray ionization (ESI) mass spectrum of the native SMKT solution containing 0.5 µM protein, 1.0% (w/v) acetic acid and 50.0% (w/v) methanol was acquired using a TSQ700 triple-stage quadrupole mass spectrometer equipped with an electrospray ion source (Finnigan, San Jose, CA). The measurement conditions of the ESI mass spectra were almost the same as described previously (Kashiwagi et al., 2000).
In order to identify residue 206, peptide mapping of the reduced, carboxymethylated and proteolytic digested ß subunit was carried out by liquid chromatographyelectrospray ionization ion trap mass spectrometrymass spectrometry (LCESI IT-MSMS). The Cys residues of SMKT were reduced by incubating 100 µg of SMKT in 100 µl of 0.5 M TrisHCl buffer (pH 8.1) containing 6 M guanidine, 2 mM ethylenediaminetetraacetic acid (EDTA) and 15 mM dithiothreitol (DTT) at 50°C for 3 h and then at room temperature for 10 h. Next, 10 µl of 0.5 M TrisHCl buffer (pH 8.1) containing 0.1 M iodoacetic acid was added to this solution. After 30 min, the reduced and S-carboxymethylated (RCM) ß subunit was isolated by reverse-phase liquid chromatography using a Vydac (San Francisco, CA) C4 capillary column packed with LC packing and lyophilized. The RCM-ß subunit was digested by lysylendopeptidase (Wako Pure Chemical Industries, Osaka, Japan), under the conditions of a 200:1 molar ratio of substrate to enzyme in 20 µl of 50 mM ammonium bicarbonate buffer (pH 9.0) at 35°C for 8 h. Digestion was stopped by the addition of 30 µl of 0.1% trifluoroacetic acid (TFA). Next, 10 µl of a 5-fold dilution of this solution was subjected to LCESI IT-MSMS. The LC solvents consisted of (A) 0.1% aqueous TFA and (B) acetonitrilewater (9:1) containing 0.095% TFA. The digested peptides of the RCM-ß subunit were isolated by 10 min isocratic elution with 98% solvent A, gradient elution from 98% to 2% A (1050 min) and 10 min isocratic elution with 2% solvent A. ESI IT-MSMS was performed on a Finnigan LCQ instrument equipped with a Finnigan electrospray ion source. The measurement conditions for LCESI IT-MSMS were almost the same as those described previously (Hirayama et al., 1998).
Construction of plasmids
Standard molecular manipulations were similar to those described by Sambrook et al. (Sambrook et al., 1989).
Three CTG codons in the ORF of SMK1 subcloned into pUC118 (pCS106) were serially changed to TCG or TTC codons by site-directed mutagenesis using a QuikChange mutagenesis kit (Stratagene, La Jolla, CA) according to the instructions provided by the manufacturer. Oligonucleotides 5'L87S CAAGAGATCCTCGGATTCTTTCTCTATTGTCAACC, 5'L137S GGCTACCACTTCACCTCTGATGGAAGTGGGCCCTG and 5'L206S TATATGATCAAGTTCTCGTT-GGCCGGTGGC and their complementary oligonucleotides were used to change Leu87, Leu137 and Leu206 in S.cerevisiae, respectively. The introduced mutations were confirmed by sequencing. The 1 kb SphI fragment containing the native SMK1 in pCS224 was substituted for that containing mutated SMK1, resulting in pCS262. The plasmids were transformed into yeast strains as described previously (Elble, 1992).
Reverse transcriptase polymerase chain reaction (RT-PCR)
Total RNA was prepared according of the method of Köhrer and Domdey (Köhrer and Domdey, 1991). After DNase I digestion, RT-PCR was performed as described previously (Suzuki, 1999
).
Other methods
Preparation of cell lysates, precipitation of secreted proteins by TCA, electrophoresis and immunoblotting were performed as described previously (Suzuki, 1999). Protein A purified rabbit antiserum against the
subunit, that against the ß subunit and horseradish peroxidase-linked anti-rabbit immunoglobulin (Bio-Rad Technologies, Richmond, CA) were used at dilutions of 1:5000, 1:1000 and 1:3000, respectively. For detection, the ECL Plus Western Blotting Detection Reagents (Amersham Pharmacia Biotech, Piscataway, NJ) were used.
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Results and discussion |
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The native SMKT was also analyzed by ESI-MS. Under the conditions described in Materials and methods, SMKT was completely dissociated into two subunits and the mass values of the and ß subunits were estimated as 6341.9 and 7847.0 by ESI-MS. The calculated molecular masses of the
subunits, ß subunit with Leu206 and ß subunit with Ser206 were 6342.17, 7872.54 and 7846.46, respectively. The observed molecular mass of the ß subunit indicates that the 206th residue should be Ser.
For further analysis of residue 206, the ß subunit was reduced, carboxymethylated and digested with lysylendopeptidase. The resultant peptide fragments were analyzed by LCESI IT-MSMS (Figure 1). Each peak was clearly identified as the expected peptide fragments. Peak 7 was identified as the C-terminal peptide including carboxymethylated Cys199 and Ser206. The product ion spectrum obtained by LCESI IT-MSMS measurement of peak 7 is shown in Figure 1C
. Fragmentation of the peptide residues 205222 indicated that residue 206 is unmodified Ser. Based on these data, we concluded that the CUG codon is read as Ser in P.farinosa.
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To examine the effects of two other Ser residues, all three CUG codons in SMK1 corresponding to Ser87, Ser137 and Ser206 were replaced by universal Ser codons. The modified SMK1 gene, SMK1L/S, was inserted under the control of a galactose-inducible promoter, pGal1. The resultant plasmid, pCS262, was transformed into the wild-type strain (W303-1A) of S.cerevisiae. When SMK1L/S was induced by galactose, the colonies of transformants showed a blue color in the presence of methylene blue employed to stain dead cells. As shown in Figure 2, the colonies of cells expressing SMK1L/S product turned blue, as was observed when unmodified SMK1 and SMK1L206S were expressed, suggesting that the side chains of residues Ser87, Ser137 and Ser206 do not affect the structure stability and/or the toxicity of the SMK1 product. When pCS224 or pCS262 was transformed into the spf1 disruptant cells (CS701C), which are highly resistant to exogenous SMKT, the transformant colonies did not show a blue color on YPGal/MB plates (Figure 2
). We have recently demonstrated that the spf1 disruptants acquire resistance to SMKT by trapping the toxin at the modified cell surface (Suzuki and Shimma, 1999
). Glycosylation is defective in spf1 disruptants, which may generate molecules with affinity to SMKT. However, the spf1 disruptants also acquired resistance to endogenous SMK1 products, suggesting that the intracellular target site of SMKT is also modified in the absence of Spf1p.
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The amount of the secreted SMK1L/S product from pCS262 was greater than that of the SMK1 product from pCS224. Especially the secretion of protoxin with authentic amino acid sequence was significantly increased. To determine whether the loss of the rare CUG codon increases the expression or Ser residues in the region are involved in the secretion processes, the transcription level was examined by RT-PCR. As shown in Figure 3C
, the presence or absence of CUG codon did not have much effect on the transcription level of SMK1 either in the wild-type or in spf1 disruptant cells. Therefore, the increased expression of protoxin with the residues of Ser87, Ser137 and Ser206 is not due to the elevated level of transcription but is probably due to the stable conformation by the authentic amino acid residues.
The SMK1L/S product accumulated in a significant amount in P100 of spf1 disruptants but was hardly detected in those of the wild-type cells. Recently, we have shown by subcellular fractionation experiments that the fractionation pattern of Spf1p was similar to that of an early Golgi protein, Och1p (Suzuki, 2001). Glycosylation is defective in spf1 disruptants. Loss of Spf1p may perturb the ion homeostasis in the secretory pathway, which may result in glycosylation defects and disturbance of the secretion process. Accumulation of the SMK1L/S product may be due to the partially perturbed secretory pathway.
Alternative codon usage in P.sorbitophila and C.cacaoi was predicted from the sequence information from the genome and from in vitro experiments, respectively. However, there was no discussion about each Ser residue encoded by CUG codon. So far, two genes in P.sorbitophila have been sequenced. In the case of Pichia TIM10, Ser83 is encoded by CUG codon and is conserved in S.cerevisiae and Candida albicans (Kayingo et al., 2000). In the case of PsLYS2, the gene encoding the
-aminoadipate reductase from P.sorbitophila, three CUG codons corresponding to Ser41, Ser1196 and Ser1322 were found in the ORF, although these residues were specified as Leu (Bleykasten-Grosshans et al., 2001
). The corresponding residues to Ser1196 and Ser1322 in C.albicans are also Ser. Because PsLYS2 is functional in S.cerevisiae, these residues are not critical for its function. There are 112 Ser residues in the PsLYS2 product including those encoded by CUG codon, suggesting that the CUG codon is a rare codon in P.sorbitophila. On the other hand, CUG is relatively abundant in the SMK1 gene, in which three out of 20 Ser residues (15%) are encoded by CUG codons. Since no sequence similar to SMK1 was found, the origin of the chromosomal killer gene is unknown. The abundance of CUG codon might be peculiar to the killer gene, which is irrelevant to the evolution of genome.
P.farinosa/P.sorbitophila is highly resistant to osmotic stress in general and particularly to salt stress up to 4 M NaCl. Previous studies showed that glycerol, the major solute in this yeast, is actively co-transported with protons to maintain osmotic balance (Lages and Lucas, 1995; Oliveira et al., 1996
). In addition to the high halotolerance, P.farinosa secretes proteins with relatively small sugar chains. gp26, the secreted protoxin of SMKT, has a mannose-containing sugar chain about 2 kDa in size (Suzuki, 1999
). Highly glycosylated sugar chains observed in S.cerevisiae were not added to the protoxin. These properties are potentially useful for heterologous expression of proteins, especially those derived from mammals. Because the CUG codon encodes Ser in most Candida species, the character of P.farinosa is promising for recombinant protein production derived from such species. The expression system of P.farinosa is currently being sought based on the need for further elucidation of the killer mechanism and potential use of this yeast as a host in functional expression of heterologous genes.
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Notes |
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Acknowledgments |
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References |
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Received November 16, 2001; revised December 6, 2001; accepted December 7, 2001.