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Antimicrobial Agents and Chemotherapy, December 2008, p. 4518-4521, Vol. 52, No. 12
0066-4804/08/$08.00+0     doi:10.1128/AAC.00640-08
Copyright © 2008, American Society for Microbiology. All Rights Reserved.

Tet 42, a Novel Tetracycline Resistance Determinant Isolated from Deep Terrestrial Subsurface Bacteria {triangledown}

Mindy G. Brown,* Elizabeth H. Mitchell, and David L. Balkwill

Department of Biomedical Sciences, Florida State University College of Medicine, Tallahassee, Florida

Received 15 May 2008/ Returned for modification 24 July 2008/ Accepted 12 September 2008


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ABSTRACT
 
Tet 42, a novel tetracycline resistance determinant from deep subsurface bacteria, was characterized and found to have a 30% sequence similarity to TetA(Z). The protein is a putative efflux pump that shares characteristics with previously characterized pumps, including a divergently transcribed TetR repressor, a conserved GxxSDRxGRR motif, and transmembrane domains.


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TEXT
 
Tetracycline is a broad-spectrum antibiotic that binds to the 30S ribosomal subunit and inhibits translation by preventing the binding of tRNA. Tetracycline has been used clinically for more than 50 years, but the emergence of resistance has rendered it increasingly less useful. Tetracycline resistance was first characterized in the mid-1950s (3). Since then, more than 40 classes of resistance genes have been described, most of which confer resistance through active efflux (http://faculty.washington.edu/marilynr/tetweb4.pdf). Tetracycline resistance genes have been identified in bacteria from many environments (7, 14, 17), but little is known about resistance genes in terrestrial subsurface environments.

In the 1990s, sediments were extracted from 170 to 210 m below land surface at the U.S. Department of Energy Hanford Site (HS) in Washington State. Bacteria isolated from these sediments (6, 8) were later screened for resistance, and resistance to several antibiotics, including tetracycline, was reported (2). This study focused on the HS subsurface, because it has been isolated from surface influence for approximately 3 million years (23). The bacteria in these sediments have never been exposed to manmade antibiotics or to resistance genes that other bacteria have acquired through selective pressure from exposure to antibiotics. The aim of this study was to determine the genetic basis of tetracycline resistance in bacteria from this isolated environment.

The bacteria investigated in this study initially were found to be tetracycline resistant by plating on selective media containing 16 µg/ml tetracycline (2). MICs (Table 1) were then determined using a standard serial broth microdilution method (4).


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  		TABLE 1. Bacterial strains examined in this studya

Total DNA was extracted from strains G880, G887, G896, and G994 by using the 500G Genomic Tip kit (Qiagen, Valencia, CA). For strains G938, G983, and G985, cells were disrupted with the FastPrep-24 instrument (MP Biomedicals, Solon, OH) before extraction of DNA by a slight modification of the Genomic Tip protocol.

Chromosomal DNA was partially digested with various blunt-end restriction enzymes (New England Biolabs Inc., Ipswich, MA), and digests yielding fragments of 4 to 10 kbp were purified and concentrated by ethanol precipitation. Purified DNA digests were ligated into the pEZSeq vector (Lucigen Corporation, Middleton, WI) and transformed into electrocompetent cells (10G Elite; Lucigen) as described in the pEZSeq manual. The recovered cells were plated (100 µl/plate) onto yeast-tryptone agar plates with 16 µg/ml tetracycline. Resistant transformants were replated onto media containing tetracycline in order to determine the highest MIC for the resistance gene by using the standard agar dilution method (4). The MIC of the vector, without an insert, was determined by plating on media with 8 and 16 µg/ml tetracycline.

Clone plasmid DNA was screened using a double digest and run on a 1% agarose gel to identify clones containing an insert. DNA was sequenced as described in the supplementary methods to the article by Margulies et al. (12), with slight modifications as specified by 454 Life Sciences Corporation (Branford, CT).

Sequences were initially evaluated for homology to known tetracycline resistance determinants through a BLAST search. Sequence alignments and relatedness to homologous proteins were determined with the GCG SeqLab (version 11.1.3; Accelrys Software Inc., San Diego, CA) and PAUP (version 4.0 beta; D. Swofford, Sinauer Associates, Sunderland, MA) programs, respectively. Locations of conserved motifs were analyzed with the SMART website (9, 19).

DNA and protein sequence analysis. All seven strains possessed the same nucleotide base sequence for the resistance determinant described below. This sequence included two divergently transcribed open reading frames (ORFs) with low similarity to known proteins. The first and shorter ORF (612 nucleotides) was similar to the tetA repressor tetR. The second ORF (1,287 nucleotides) had a low similarity to previously characterized tetracycline efflux pumps. There is a 71-bp region between the two ORFs.

The larger ORF predicted a 429-amino-acid sequence most similar to TetA(Z) (21), with 30% homology (Fig. 1). The predicted amino acid sequence is <80% similar to any previously described tetracycline resistance determinant and was given the name TetA(42) according to current naming standards (11).


Figure 1
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  		FIG. 1. Amino acid sequence comparison for TetA(42) and the two most closely related sequences, TetA(Z) and TetA(30). White letters on a black background indicate amino acids that are identical in two of the three sequences. GenBank accession numbers for TetA(Z) and TetA(30) are AAD25063 and AAD09860, respectively.

Ten transmembrane domains, located at amino acids 19 to 41, 51 to 73, 85 to 107, 112 to 131, 143 to 165, 169 to 191, 228 to 250, 260 to 282, 291 to 313, and 378 to 400, were predicted for TetA(42). In contrast, previously reported efflux pumps contain 12 or 14 transmembrane domains (16). TetA(42) also contains the GxxSDRxGRR motif common to all tetracycline pumps (18). This region in TetA(42) (GrlSDRfGRR) is identical to that in TetA(Z) (Fig. 1).

The TetR(42) sequence comprises 204 amino acids and has a 41% amino acid similarity to the TetR transcriptional regulator from Streptomyces ambofaciens (1).

The intergenic region between tetA and tetR contains two TetR binding operators and promoters for both genes (16, 18). The putative operators (CGACAGTCTATCG and GACTACACTTTCG) are not perfect palindromic sequences and differ by 7 bases (Fig. 2). Similar variations have been seen in other determinants (22). The second operator, while not very similar to the first sequence, matches the second half of the first operator except for 1 base. The putative promoters are also shown in Fig. 2.


Figure 2
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  		FIG. 2. DNA sequence of the 71-bp tetA(42)-tetR(42) intergenic region. Putative TetR(42) binding operators are in boldface and overlined. Each asterisk indicates the center of the inverted repeat for an operator. The –35 and –10 potential promoter sequences are indicated.

A phylogenetic analysis of the protein sequences of TetA(42) and representatives of each class of previously reported efflux pumps (Fig. 3) clearly distinguished TetA(42) from the other proteins by placement on a separate deep branch of the tree. The most closely related proteins were TetA(Z) and TetA(30).


Figure 3
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  		FIG. 3. Phylogenetic tree based on distance matrix analysis of amino acid sequences for Tet 42 and representative tetracycline resistance determinants that have been reported previously. GenBank accession numbers are given to the right of each resistance determinant. Scale bar, 10 substitutions per 100 amino acids.

The MICs for the subsurface strains ranged from 16 to 32 µg/ml (Table 1). Resistant transformants with the Tet 42 determinant showed an increase in the MIC from 4 to 32 µg/ml compared to the wild type (Table 1). The GenBank accession number for the DNA sequence of this class A determinant is EU523697.

Concluding remarks. The current study presents another tetracycline resistance determinant, Tet 42, that most likely confers resistance through active efflux. This determinant shares certain distinctive characteristics with previously reported tetracycline efflux pumps but has a low sequence similarity to the most closely related determinants. The bacteria investigated in this study were recovered from sediments that have been isolated from surface influence for approximately 3 million years (23), and as a result, they have never been exposed to commercial antibiotics or to bacterial genes that evolved in response to exposure to these antibiotics. It is not surprising, then, that the subsurface strains possess a novel resistance determinant.

The Tet 42 sequences were identical in all seven strains, which were isolated from several different sediment depths and included both gram-negative and gram-positive genera (Table 1). This finding raises interesting questions as to whether horizontal gene transfer (HGT) has occurred in the HS sediments. Smets et al. (20) demonstrated HGT in laboratory microcosms of subsurface sediment, and Martinez et al. (13) found evidence for HGT of lead resistance in subsurface soils. It is also interesting that these bacteria possess antibiotic resistance when they have been isolated from exposure to manmade antibiotics, unless antibiotics are being produced in the subsurface. Alternatively, they could possess an efflux pump to rid the cell of heavy metals or other toxins. The new resistance determinant presented here should help to further understanding of how TetA and TetR function, as well as providing useful information on antibiotic resistance in nature and the evolution of resistance genes. The discovery of a novel resistance gene in subsurface bacteria supports the suggestion that a pool of uncharacterized resistance mechanisms exists in environments that have not yet been examined in this regard (10, 15, 17).


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ACKNOWLEDGMENTS
 
Part of this research was funded by a Leaders Educated to Make a Difference (LEAD) grant to M.G.B. from the Student Council on Research and Creativity (SCRC) at Florida State University.

We thank Laura McMurry of the Center for Adaptation Genetics and Drug Resistance, Tufts University School of Medicine, for assistance in providing a name for the novel determinant. We also thank William Farmerie, Regina Shaw, Savita Shanker, and Ernesto Almira of the Advanced DNA Sequencing Technology Group at the University of Florida Interdisciplinary Center for Biotechnology Research for assistance with 454 DNA sequencing and assembly of sequences.


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FOOTNOTES
 
* Corresponding author. Mailing address: Department of Biomedical Sciences, Florida State University College of Medicine, 1115 West Call Street, Tallahassee, FL 32306-4300. Phone: (850) 645-2933. Fax: (850) 644-5781. E-mail: mindy.brown{at}med.fsu.edu Back

{triangledown} Published ahead of print on 22 September 2008. Back


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Antimicrobial Agents and Chemotherapy, December 2008, p. 4518-4521, Vol. 52, No. 12
0066-4804/08/$08.00+0     doi:10.1128/AAC.00640-08
Copyright © 2008, American Society for Microbiology. All Rights Reserved.




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