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Antimicrobial Agents and Chemotherapy, May 2002, p. 1550-1552, Vol. 46, No. 5
0066-4804/02/$04.00+0     DOI: 10.1128/AAC.46.5.1550-1552.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

New Mg²⁺-Dependent Oxytetracycline Resistance Determinant Tet 34 in Vibrio Isolates from Marine Fish Intestinal Contents

Lisa Nonaka and Satoru Suzuki^*

Center for Marine Environmental Studies (CMES), Ehime University, Matsuyama 790-8577, Japan

Received 19 July 2001/ Returned for modification 4 October 2001/ Accepted 24 January 2002

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A new oxytetracycline (OTC) resistance (Otc^r) determinant, Tet 34, was cloned from chromosomal DNA of Vibrio sp. no. 6 isolated from intestinal contents of cultured yellowtail (Seriola quinqueradiata). The transformant, containing cloned Tet 34, could grow in broth containing 25 µg of drug per ml with 10 mM MgCl₂. Tet 34 encoded an open reading frame (ORF) 154 amino acids long. The amino acid sequence of the ORF was homologous to sequences of several bacterial xanthine-guanine phosphoribosyltransferases (XPRTs), which act in purine nucleotide salvage synthesis. Mg²⁺ binding site residues and the active site were highly conserved in XPRT and the ORF of Tet 34. The results suggest that Tet 34 encodes a new Mg²⁺-dependent Otc^r mechanism.

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Oxytetracycline (OTC) has widely been used in aquaculture, and there are many reports on the occurrence of OTC-resistant (Otc^r) fish-pathogenic bacteria (3, 5, 9, 16, 17). The Otc^r bacteria were found not only among the pathogenic bacteria, but also in aquacultural environments (7, 13, 16). In our previous study, a high prevalence of Otc^r bacteria appeared in intestinal contents and rearing water of yellowtail (Seriola quinqueradiata) (14). The frequency of Otc^r reached 56 to 91% of the total viable bacteria. Several Tet determinants (Tet A to G) were reported from fish-pathogenic bacteria or the marine environment (1, 2, 5, 16). As a first step toward a better understanding of the dynamics of the Otc^r determinant in aquatic environments, we cloned the Otc^r determinant from Vibrio sp. isolated from intestinal contents of cultured yellowtail.

Otc^r strains of Vibrio spp. were isolated from cultured yellowtail obtained during 1999 in Japan (14). We isolated 288 Otc^r isolates from intestinal contents and seawater at that time. We checked the Otc^r strains used for cloning. These strains were not PCR positive for one of the known tet genes, tet(G) (3). Only a small number of tet genes among marine bacteria have been reported, which reminds us to be able to find unknown factors. We had performed cloning with 10 strains of them and got a new determinant successfully from Vibrio sp. no. 6. The MIC of OTC for this strain was 500 µg/ml.

Since it is known that the efflux system of tetracycline resistance is sometimes dependent on various divalent cations, we assessed whether Vibrio sp. no. 6 requires MgCl₂ for the Otc^r. Cell growth was determined in broth containing 100 µg of OTC per ml with or without MgCl₂ at concentrations of 10, 1, and 0.1 mM at 25°C. The broth used contained 5 g of polypeptone (Wako, Osaka, Japan); 1 g each of yeast extract (Difco, Detroit, Mich.), proteose peptone (Difco), beef extract (Wako); and 20 g of NaCl per liter of distilled water. Growth of Vibrio sp. no. 6 was sensitive to OTC when MgCl₂ was absent, whereas addition of MgCl₂ allowed growth in a dose-dependent manner in the presence of OTC (data not shown). In the presence of 10 mM MgCl_2, the growth of Vibrio sp. no. 6 was almost the same as the growth in broth without OTC. This indicates that the Otc^r of Vibrio sp. no. 6 is dependent on MgCl₂.

The Otc^r determinant was cloned from chromosomal DNA, because Vibrio sp. no. 6 seemed not to possess a plasmid (data not shown). However, it is possible that there exists a low-copy-number plasmid that could not be detected by agarose gel electrophoresis and/or a megaplasmid, which might be removed with the chromosome during extraction. The chromosomal DNA was extracted from the bacteria as follows. The bacterial pellet was suspended in extraction solution (0.15 M NaCl, 0.1 M EDTA, 0.5 mg of RNase A per ml, and 0.5% sodium dodecyl sulfate [SDS]) and incubated at 65°C for 5 min. This solution was mixed with phenol saturated with 10 mM Tris-HCl (pH 8.0) plus 1 mM EDTA (TE) and centrifuged (17,000 x g) for 3 min. The DNA in the supernatant was extracted two times with TE-saturated phenol-chloroform-iso-amyl alcohol (25:24:1 [vol/vol/vol]) and with chloroform. Precipitated DNA with ethanol was resuspended in 50 µl of TE and stored at -20°C. After the chromosomal DNA and vector pUC119 (TaKaRa, Kyoto, Japan) were digested by restriction endonucleases PstI (TaKaRa) and EcoRI (TaKaRa), they were ligated with a DNA ligation kit, version 2 (TaKaRa). Escherichia coli JM109 was transformed and spread on Luria-Bertani (LB) medium containing 50 µg of ampicillin per ml, 10 µg of OTC per ml, 40 µg of 5-bromo-4-chloro-3-indolyl-ß-D-galactopyranoside (X-Gal) per ml, and 0.1 mM isopropyl-ß-D-thiogalactopyranoside (IPTG). After three passages of candidate colonies, we obtained a viable transformant. This transformant possessed a 919-bp inserted fragment, and the recombinant plasmid was designated pOV. Growth of transformants (pOV/JM109) with the cloned fragment was examined with or without MgCl₂. The results are shown in Fig. 1. pOV/JM109 grew in the LB broth with 25 µg of OTC per ml (Fig. 1A), but not in the broth without MgCl₂ (Fig. 1B)_. The same growth profiles were observed in the case of cultures containing 12.5 µg of tetracycline per ml (data not shown). This suggests that pOV/JM109 is also a tetracycline resistance determinant acting in the same manner as OTC and that the resistance ability of the transformed E. coli is dependent on MgCl₂ as well as Vibrio sp. no. 6. Furthermore, we have retransformed pOV to different host E. coli DH5 cells. The transformants (pOV/DH5) showed resistance in the presence of 10 mM MgCl₂, the same as in JM109 (data not shown). On the other hand, the transformant pUC119/DH5 could not grow on the plate with OTC, regardless of the presence and absence of MgCl₂. This suggests that Tet 34 can be expressed in both strains JM109 and DH5.

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FIG. 1. Growth of E. coli JM109 transformed with pOV (, •) or pUC119 (, ). LB broth contained 25 µg of OTC and 50 µg of ampicillin per ml. Panel A shows results with 10 mM MgCl2, and panel B shows results without MgCl2. Open symbols, without OTC; solid symbols, with OTC. O.D., optical density.

To confirm that the cloned fragment originated from the chromosomal DNA of Vibrio sp. no. 6, Southern hybridization was performed. The cloned fragment was labeled with a DIG-Chem-Link labeling and detection set (Roche Diagnostics, Mannheim, Germany) in accordance with the manufacturer's directions. Ten micrograms of DNA was digested with PstI and EcoRI and employed for Southern transfer. After denaturation and neutralization were performed, DNA was fixed with UV light (254 nm) by irradiation for 1 min. Fifty nanograms of digoxigenin (DIG)-labeled DNA probe was added to the blotted filter and hybridized at 65°C overnight. The membrane was washed three times with wash solution (40 mM NaH₂PO₄, 0.1% SDS [pH 7.2]). The DIG-labeled DNA was reacted with nitroblue tetrazolium chloride-9-bromo-4-chloro-3-indoyl phosphate toluidine salt (NBT/BCIP), with the enzymatic reaction followed by an anti-DIG antibody-conjugated alkaline phosphatase (Roche Diagnostics). Tet 34 probes hybridized to Vibrio sp. no. 6, but not to E. coli JM109 chromosome (data not shown). This result confirms that Tet 34 is coded on the chromosome DNA of Vibrio sp. no. 6.

Tet 34 was sequenced by using an ABI PRISM BigDye Terminator cycle sequencing FS Ready Reaction kit (PE Biosystems, Tokyo, Japan) with an ABI PRISM 310 DNA sequencer (PE Biosystems, Tokyo, Japan) in the Center for Gene Research, Ehime University. An open reading frame (ORF) of 465 bp (154 amino acids) was found on this fragment, which existed between 306 and 770 bp. Sequence analysis was performed with the homology search program FASTA. However, the DNA sequence of the determinant did not show homology with any Tet determinants, as described above. This determinant was named Tet 34 according to the recommendation proposed in reference 11. The deduced amino acid sequence of the ORF showed 79.8% homology with xanthine-guanine phosphoribosyltransferase (XPRT) of Vibrio cholerae (8) and 68 and 66% homology with XPRTs of E. coli (15) and Salmonella enterica serovar Typhimurium (12), respectively. The alignment with the known XPRTs is shown in Fig. 2.

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FIG. 2. Alignment of the amino acid sequence of the ORF on Tet 34 with five XPRTs obtained from the database. The PRib-PP motif is boxed, and the conserved amino acid residues related to activity of XRPT are in boldface. Asterisks denote the consensus amino acid residues. See references 6 (noted by no. 1) and 19 (noted by no. 2) for review.

From our studies, we propose another mechanism to explain Otc^r by Tet 34. XPRT is an enzyme that acts in purine nucleotide salvage synthesis. This enzyme catalyzes the transfer of the phosphoribosyl moiety from 5-phospho--D-ribosyl-1-pyrophosphate (PRib-PP) to the 6-oxo-guanine and -xanthine (20). GMP and XMP are formed by this reaction, and then these nucleotides are converted to triphosphate forms. The fact that Tet 34 has homology to XPRT suggests it has a similar function. It is known that the Mg²⁺ ion interacts with the Asp-89 in the PRib-PP binding site motif of XRPT (20). Asp-89 was found conserved in the ORF on Tet 34 (Fig. 2). The fact that Vibrio sp. no. 6 requires MgCl₂ for Otc^r might relate to the Mg²⁺-binding property of the PRib-PP-like protein coded in Tet 34. The PRib-PP binding site motif in Tet 34 consists of the residues 85-IVEDLVDSG-96 (Fig. 2). In Tet 34, the region of the motif revealed high similarity to the PRib-PP binding site of the previously reported phosphoribosyltransferase (PRT) (20). XRPT comprises three subunits (A, B, and C). The active residues Pro-25, Ser-26, Trp-29, and Arg-53 are present in subunit A; Arg-37 and Asp-89 are present in subunit B; and Arg-152 is present in subunit C (20). The Pro-25, Trp-29, Arg-37, Arg-53, and Asp-89 residues were highly conserved in the sequence of the Tet 34 determinant. The PRib-PP binding site sequence forms part of the active site, and its relative position is completely conserved among several PRT structures by structural analysis (20). These findings suggest that the Tet 34 determinant possesses a similar function to PRTs, including XRPT.

Tetracycline inhibits bacterial growth by inhibiting protein synthesis in ribosomes (4, 18). The inhibition of protein synthesis is caused by disruption of codon-anticodon interactions. Elongation factor Tu (EF-Tu) (10) is a protein that plays a crucial role in the polypeptide elongation step of protein biosynthesis. This factor is required for the correct binding of the aminoacyl-tRNA to the ribosomal acceptor site and is a key factor in maintaining translational fidelity. During protein synthesis, the EF-Tu·GTP complex binds strongly to aminoacyl-tRNA, thereby preventing spontaneous hydrolysis of the aminoacyl-tRNA ester bond. When the EF-Tu · GTP · tRNA complex interacts with the ribosome, the GTP is hydrolyzed, and then EF-Tu·GDP is released from the ribosome (10). The GDP is thereafter recycled to the GTP (10). The similarity of protein sequence between Tet 34 and XPRT, which catalyzes formation of GMP, XMP, and IMP from guanine, xanthine, and hypoxanthine, respectively, suggests that the Tet 34 product supplies the purine nucleotides needed for the translational step described above. Consequently, an excess supply of GTP may have some effect on accelerating the binding of aminoacyl-tRNA and EF-Tu·GTP, which attenuates inhibition by OTC.

In conclusion, we cloned a new Tet determinant and determined that the possible function of the determinant is activation of Mg²⁺-dependent purine nucleotide synthesis, which finally protects protein synthesis.

Nucleotide sequence accession number. The sequence of the Tet 34 determinant has been submitted to the DDBJ database under accession no. AB061440.

 
We thank S. Nakano for useful suggestions and D. E. Taylor, University of Alberta, for critical review of the manuscript.

This work was partly supported by a grant-in-aid from MEXT. Genetic experiments were performed in the Center for Gene Research, Ehime University.

 
* Corresponding author. Mailing address: Center for Marine Environmental Studies, Ehime University, Matsuyama 790-8577, Japan. Phone: 81-89-927-8552. Fax: 81-89-927-8552. E-mail: ssuzuki{at}agr.ehime-u.ac.jp.

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Antimicrobial Agents and Chemotherapy, May 2002, p. 1550-1552, Vol. 46, No. 5
0066-4804/02/$04.00+0     DOI: 10.1128/AAC.46.5.1550-1552.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

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