Antimicrobial resistance markers of Class 1 and Class 2 integron-bearing Escherichia coli from irrigation water and sediments. (Research).Municipal and agricultural pollution affects the Rio Grande, a river that separates the United States from Mexico. Three hundred and twenty-two Escherichia coil isolates were examined for multiple antibiotic resistance phenotypes and the prevalence of class 1 and class 2 integron sequences. Thirty-two (10%) of the isolates were resistant to multiple antibiotics. Four (13%) of these isolates contained class 1-specific integron sequences; one isolate contained class 2 integron-specific sequences. Sequencing showed that the class 1 integron-bearing strain contained two distinct gene cassettes, sat-1 and aadA. Although three of the four class 1 integron-bearing strains harbored the aadA sequence, none of the strains was phenotypically resistant to streptomycin streptomycin (strĕp'tōmī`sĭn), antibiotic produced by soil bacteria of the genus Streptomyces and active against both gram-positive and gram-negative bacteria (see Gram's stain), including species resistant to other . These results suggest that integron-bearing E. coil strains can be present in contaminated irrigation irrigation, in agriculture, artificial watering of the land. Although used chiefly in regions with annual rainfall of less than 20 in. (51 cm), it is also used in wetter areas to grow certain crops, e.g., rice. canals and that these isolates may not express these resistance markers. ********** Integron gene sequences contribute to the spread of antimicrobial resistance alleles by lateral gene transfer of gene cassettes in a variety of enteric bacteria, including Campylobacter Campylobacter Genus of gram-negative spiral-shaped bacteria infecting mammals. Many species, especially C. fetus, cause miscarriage in sheep and cattle. C. jejuni is a common cause of food poisoning. Sources include meats (particularly chicken) and unpasteurized milk. spp., Escherichia coli, and Salmonella enterica serotype Typhimurium (1-4). The gastrointestinal environment is suspected of serving as a reservoir for integron-bearing strains; when antimicrobial exposure occurs, gene transfer events--which spread cassettes between commensal commensal /com·men·sal/ (kom-men´sil) 1. living on or within another organism, and deriving benefit without harming or benefiting the host. 2. a parasite that causes no harm to the host. organisms that are expelled into the environment (2)--would also occur. The Rio Grande, the river separating the United States from Mexico along the Texas-Mexico region, serves as a source for irrigation water in Texas and Mexico. Previous studies in our laboratory and others have shown that the transboundary region is subject to extensive microbial microbial pertaining to or emanating from a microbe. microbial digestion the breakdown of organic material, especially feedstuffs, by microbial organisms. and chemical contamination. This contamination has been associated with agricultural, municipal, and industrial wastes originating from both sides of the border (5,6). Leaking septic tanks and wastewater effluent discharges result in fecal contamination levels as high as 2,000 CFU/mL of fecal coliforms (7,8). Because of the strategic importance of the Rio Grande for U.S. agriculture and the potential transmission of antimicrobial resistance determinants by means of food crops, we investigated the prevalence and characteristics of class 1 and class 2 integron-bearing E. coli strains. These strains were previously isolated from a study investigating fecal contaminants in irrigation water and associated sediments at specific locations along the river (9). Methods Three hundred and twenty-two E. coli isolates were previously isolated from irrigation water and associated sediments at the El Paso, Presidio, and Weslaco regions of the river (9). After being confirmed as E. coli by MUG (4-methyl umbelliferyl-[beta]-D-glucoronide)-based fluorescence, these isolates were screened for antimicrobial susceptibility by using the agar dilution method (10,11). The isolates were tested against ampicillin ampicillin (ăm'pĭsĭl`ĭn), a penicillin-type antibiotic that is effective against both gram-negative microorganisms and gram-positive microorganisms such as Escherichia coli. , tetracycline tetracycline (tĕ'trəsī`klēn), any of a group of antibiotics produced by bacteria of the genus Streptomyces. They are effective against a wide range of Gram positive and Gram negative bacteria, interfering with protein , ceftriaxone ceftriaxone /cef·tri·ax·one/ (cef?tri-ak´son) a semisynthetic, ß–resistant, third-generation cephalosporin effective against a wide range of gram-positive and gram-negative bacteria, used as the sodium salt. , cephalothin cephalothin a first generation cephalosporin antibiotic. Sensitive organisms include many penicillin-resistant staphylococci. cephalothin Cefalotin® Infectious disease A parenteral semisynthetic derivative of cephalosporin C, and 3 , gentamicin gentamicin /gen·ta·mi·cin/ (jen?tah-mi´sin) an aminoglycoside antibiotic complex isolated from bacteria of the genus Micromonospora, , kanamycin kanamycin /kan·a·my·cin/ (kan?ah-mi´sin) an aminoglycoside antibiotic derived from Streptomyces kanamyceticus, effective against aerobic gram-negative bacilli and some gram-positive bacteria, including mycobacteria; used as the , streptomycin, chloramphenicol chloramphenicol (klōr'ămfĕn`əkŏl'), antibiotic effective against a wide range of gram-negative and gram-positive bacteria (see Gram's stain). It was originally isolated from a species of Streptomyces bacteria. , ciprofloxacin ciprofloxacin /cip·ro·flox·a·cin/ (sip?ro-flok´sah-sin) a synthetic antibacterial effective against many gram-positive and gram-negative bacteria; used as the hydrochloride salt. cip·ro·flox·a·cin n. , and trimethoprim/sulfamethoxazole. The antibiotics were tested at concentrations established by the National Antimicrobial Resistance System (12). Isolates that were multidrug resistant (resistant to two or more antimicrobial agents) were grown overnight in 5 mL of Mueller-Hinton broth (Accumedia, Baltimore, MD) with the appropriate concentration of antimicrobial compound. A 1-mL aliquot aliquot (al-ee-kwoh) adj. a definite fractional share, usually applied when dividing and distributing a dead person's estate or trust assets. (See: share) of the culture was centrifuged at 10,000 rpm for 2 min. The cell pellet was resuspended in 500 [micro]L of sterile water and boiled for 10 min. The resulting DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. suspension was used as template DNA in polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is (PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) ) amplification for the class 1 and class 2 integrase gene and variable regions using the primer sequences shown in the Table (13-15). The PCR reactions used 10 [micro]L of template DNA, 5 [micro]M of primers, 25 mM MgCl, 10 mM deoxynucleotide triphosphate triphosphate /tri·phos·phate/ (tri-fos´fat) a salt containing three phosphate radicals. tri·phos·phate n. A salt or ester containing three phosphate groups. , and 23 ng bovine serum albumin. Nuclease-free water (Ambion, Austin, TX) was added to achieve a volume of 50 [micro]L. A "hot start" method was used, and 1.25 U of Taq DNA polymerase (Sigma, St. Louis, MO) was added after initial template denaturation denaturation, term used to describe the loss of native, higher-order structure of protein molecules in solution. Most globular proteins exhibit complicated three-dimensional folding described as secondary, tertiary, and quarternary structures. . The PCR cycle was as follows: initial denaturation for 12 min at 94[degrees]C, hot start pause at 80[degrees]C followed by 35 cycles of denaturation at 94[degrees]C for 1 min, primer annealing annealing (ənēl`ĭng), process in which glass, metals, and other materials are treated to render them less brittle and more workable. at 60[degrees]C for 1 min, and extension at 72[degrees]C for 5 min at first cycle. An additional 5 s was progressively added to each cycle to reach a final of 7 min, 55 s. PCR products were analyzed on 1% agarose gel. Amplification products were extracted from the gels with the QIAGEN QIAquick gel extraction kit (Valencia, CA). The amplified products were sequenced at a commercial facility (MWG MWG Men with Guts (sports apparel company) MWG Match-Winning Goal (soccer) mWG Microworld of Gems (e-commerce business) MWG Measurements Working Group MWG Model Working Group Biotech Inc., High Point, NC) with the class 1 and class 2 integron variable region primers (integ and hep) (Table). Contiguous sequences were created from single sequence reads by using the CAP3 sequence assembly program (16). Contiguous sequences were analyzed by using the GenBank database of the National Center for Biotechnology Information The National Center for Biotechnology Information (NCBI) is part of the United States National Library of Medicine (NLM), a branch of the National Institutes of Health. The NCBI is located in Bethesda, Maryland and was founded in 1988. and the BLASTX search engine (17). Putative gene relationships and sequence data were analyzed by using a multiple sequence alignment A multiple sequence alignment (MSA) is a sequence alignment of three or more biological sequences, generally protein, DNA, or RNA. In general, the input set of query sequences are assumed to have an evolutionary relationship by which they share a lineage and are descended from a created by using Clustal W version 1.82 (18). Results Of the 322 E. coli isolates from sediment and irrigation water samples analyzed for antimicrobial resistance, 104 (32%) isolates showed resistance to at least one of the antimicrobial compounds (Figure 1). Approximately 10% (32/322) of all the isolates showed a multidrug resistance phenotype. Eighteen percent of the isolates were resistant to cephalothin; however, only 5 (2%) of 322 were resistant to ceftriaxone, which also belongs to the cephalosporin cephalosporin (sĕf'əlōspôr`ĭn), any of a group of more than 20 antibiotics derived from species of fungi of the genus Cephalosporium and closely related chemically to penicillin. Cephalosporins, e.g. family. Resistance to ampicillin was prevalent in approximately 35 (11%) of the isolates. Resistance to tetracycline (9%), kanamycin (2%), gentamicin (0.3%), and streptomycin (4%) was also observed. Resistance to the fluoroquinolone fluoroquinolone /flu·o·ro·quin·o·lone/ (-kwin´o-lon) any of a subgroup of fluorine-substituted quinolones, having a broader spectrum of activity than nalidixic acid. fluor·o·quin·o·lone n. ciprofloxacin was seen in one isolate. Three (<1%) of the 322 isolates were resistant to sulfonamide sulfonamide /sul·fon·amide/ (sul-fon´ah-mid) a compound containing the sbondSO2NH2 group. The sulfonamides, or sulfa drugs, are derivatives of sulfanilamide, competitively inhibit folic acid synthesis in microorganisms, and formerly were sulfamethoxazole sulfamethoxazole /sul·fa·meth·ox·a·zole/ (-meth-ok´sah-zol) a sulfonamideantibacterial and antiprotozoal, particularly used in acute urinary tract infections. sul·fa·me·thox·a·zole n. . On the basis of analysis of variance, antimicrobial resistance and the sampling location were correlated. Isolates from the El Paso sampling region had significantly higher (p<0.05) antimicrobial resistance as compared with the Presidio and Weslaco sampling regions (data not shown). [FIGURE 1 OMITTED] The 32 isolates identified as multiple antimicrobial resistant were assayed by PCR amplification for class 1 and class 2 integrase genes. Four isolates (approximately 13%) had the class 1 integrase gene intI1 (Figure 2A), and one isolate had the class 2 integrase gene intI2 (Figure 2B). Isolates identified as having the class 1 or class 2 integrase genes were further characterized through PCR amplification of the class 1 and class 2 variable regions. Of the four amplified class 1 integron variable regions, three isolates (isolate 16, isolate 19, and isolate 21) were approximately 1 kb in size, but the fourth isolate (isolate I-6) harbored a 2-kb fragment (Figure 3A). The 1-kb amplification products were observed in isolates from the El Paso area. Nucleotide sequencing showed that all of the 1-kb sequences contained a conserved configuration of a 780-bp gene cassette identified as the aadA gene (Figure 4). The 2-kb amplification product was seen in an isolate from the Presidio sampling region. Nucleotide sequencing showed that the variable region contained a 498-bp gene cassette, identified as the dhfrXII gene, which encodes trimethoprim trimethoprim /tri·meth·o·prim/ (-meth´o-prim) an antibacterial closely related to pyrimethamine; almost always used in combination with a sulfonamide, primarily for the treatment of urinary tract infections. resistance. The gene cassette did not exhibit perfect homology with the dhfrXIl gene (Figure 4). Within the identified 498-bp gene cassette, a 323-bp stretch showed 97% sequence homology; in addition, 59-bp and 56-bp fragments showed 88% and 89% homology, respectively. "Islands" of sequence within the variable region showed no sequence homology to any known genes. [FIGURES 2-4 OMITTED] When the 32 multiply antimicrobial-resistant isolates were screened for class 2 integrons, only 1 isolate was positive (Figure 2B). This particular isolate (isolate 29) was obtained in the Presidio region and had a 2,600-bp variable region (Figure 3B). Nucleotide sequencing identified two distinct gene cassettes, namely, the sat-1 and aadA genes, which code for streptothricin strep·to·thri·cin n. Any of a group of antibiotics produced by an actinomycete (Streptomyces lavendulae) and active against both gram-positive and gram-negative bacteria and some fungi. acetyl acetyl /ac·e·tyl/ (as´e-til) (as´e-tel?) (ah-se´til) the monovalent radical CH3COsbond, a combining form of acetic acid. a·ce·tyl n. transferase transferase /trans·fer·ase/ (trans´fer-as) a class of enzymes that transfer a chemical group from one compound to another. trans·fer·ase n. , and aminoglycosede adenyltransferase, respectively (Figure 5). [FIGURE 5 OMITTED] Discussion Antimicrobial resistance in human pathogens has become a major public health issue. Resistant organisms have been isolated from a number of natural and manmade environments (6,19,20). In natural environments, resistant organisms can be indigenous or introduced through natural or anthropogenic an·thro·po·gen·ic adj. 1. Of or relating to anthropogenesis. 2. Caused by humans: anthropogenic degradation of the environment. causes (21,22). Integron gene sequences have been identified as a primary source of resistance genes and are suspected to serve as reservoirs of antimicrobial resistance genes within microbial populations (1,2,23,24). Previous studies along the Texas-Mexico border have shown that fecal contamination of the Rio Grande does occur (7,25). The isolation of 322 E. coli isolates from irrigation water and associated sediments further confirms that fecal wastes are affecting this body of water. Previous studies have reported that municipal and animal wastes regularly harbor multidrug-resistant E. coli strains (6,26,27). In this study, 18% of the isolates were resistant to cephalothin. These results are similar to those from a recent survey of U.S. rivers, which found cefotaxime (a third-generation, cephalosporin-resistant, gram-negative bacterium) to range from 16% to 96% across 22 rivers (19). The higher frequency of isolation of resistant strains from the El Paso region compared with the other, less urbanized sampling locations is not surprising since the effluent from a number of wastewater treatment plants enters the river at that region (W. McElroy, unpub. data; 28). Previous studies with sludge and septic tank wastes showed relatively high levels of antimicrobial resistance in E. coli (6). The precise sources of the E. coli isolates used in this study could not be identified because of technical limitations in source tracking (29). Class 1 and class 2 integron gene sequences were found within these E. coli isolates. Together, they accounted for 5 (16%) of 32 multidrug-resistant isolates characterized in this study. This prevalence was higher than that reported by Rosser et al. (30), who showed that 3.6% of gram-negative bacteria in an estuarine es·tu·a·rine adj. 1. Of, relating to, or found in an estuary. 2. Geology Formed or deposited in an estuary. Adj. 1. estuarine - of or relating to or found in estuaries estuarial environment contained the class 1 integron. Three of the four class 1 integron-bearing E. coli in this study contained the nucleotide sequence of the spectinomycin-streptomycin resistance gene aadA1 (31). Resistance to streptomycin was not observed in these isolates, but resistance to the closely related kanamycin was seen. These results are similar to those reported by Zhao et al. (3), who identified that the aadA gene transferred to a strain of Hafnia alvei but did not report resistance to streptomycin or spectinomycin spectinomycin /spec·ti·no·my·cin/ (spek?ti-no-mi´sin) an antibiotic derived from Streptomyces spectabilis, used as the hydrochloride salt in the treatment of gonorrhea. . These researchers attributed their findings to the inefficient expression of the inserted gene cassette by the integron promoter. Previous studies have also shown that the antimicrobial resistance phenotype can be modulated once these strains are exposed to specific environmental conditions (32). The aadA gene cassette is not novel in class 1 integrons. Earlier work by Zhao et al. (3) and Bass et al. (24) has shown that the aadA gene is highly conserved among Shiga toxin-producing and avian clinical E. coli isolates, respectively. The only class 2 integron-bearing strain isolated in this study also contained the aadA gene in addition to the sat-1 gene, which codes for resistance to kanamycin, a finding in agreement with the phenotypic expression. The sat-1 gene, which codes for the streptothricin acetyl transferase, was not detected in any other E. coli isolate. The presence of the sat-1 gene cassette, in combination with the aadA gene, suggests that this class 2 integron is likely a derivative of the class 2 integron found on transposon transposon /trans·po·son/ (trans-po´zon) a small mobile genetic (DNA) element that moves around the genome or to other genomes within the same cell, usually by copying itself to a second site but sometimes by splicing itself out of its Tn7 (33,34). The aadA gene was conserved among the class 1 and class 2 integrons, which suggests a possible selective mechanism for this cassette in enteric bacteria from natural waters. The 2-kb integron-specific variable region-containing strain, which was isolated from the Presidio area, harbored the dihydrofolate reductase gene (dhfrXII) instead of the aadA gene (35). Overall, these results suggest that the irrigation canals and sediments associated with the Rio Grande are contaminated by bacteria of fecal origin that contain antimicrobial resistance genes. Of 322 E. coli isolates, 32 (approximately 10%) were resistant to multiple antimicrobial drugs. Five of these 32 E. coli isolates harbored class 1 and class 2 integron sequences. This study did not investigate the possibility that other integron-bearing nonfecal bacteria were present. The occurrence of integron-bearing E. coli in irrigation water is important since these organisms are known fecal contaminants, and the potential for lateral gene transfer exists. The results also indicate that integron bearing strains may not always express the antimicrobial phenotype; thus, phenotype-based isolation of resistant organisms can underestimate the levels of resistant organisms. Studies are needed to identify whether integronmediated antimicrobial resistance transfer does indeed occur within the irrigation canal sediments and on vegetable surfaces, when they are irrigated with contaminated irrigation water.
Table. Oligonucleotide primer sequences used for amplification of
class 1 and class 2 integrase and variable regions
Primer Primer sequence Target
Integ-1 5'-GGCATCCAAGCAAG-3' 5'-Class 1 integron
variable region
Integ-2 5'-AAGCAGACTTGACCTGA-3' 3'-Class 1 integron
variable region
hep51 5'-GATGCCATCGCAAGTACGAG-3' 5'-Class 2 integron
variable region
hep74 5'-CGGGATCCCGGACGGCATGCACGATTTGTA-3' 3'-Class 2 integron
variable region
intI1.F 5'-GGGTCAAGGATCTGGATTTCG-3' 5'-intI1 gene
intI1.R 5'-ACATGGGTGTAAATCATCGTC-3' 3'-intI1 gene
intI2.F 5'-CACGGATATGCGACAAAAAGGT-3' 5'-intI2 gene
intI2.R 5'-GTAGCAAACGAGTGACGAAATG-3' 5'-intI2 gene
Primer Reference
Integ-1 Levesque et al. 1995 (13)
Integ-2 Levesque et al. 1995 (13)
hep51 White et al. 2001 (14)
hep74 White et al. 2001 (14)
intI1.F Mazel et al. 2000 (15)
intI1.R Mazel et.al. 2000 (15)
intI2.F Mazel et al. 2000 (15)
intI2.R Mazel et al. 2000 (15)
Acknowledgments We thank Anne Summers and Cynthia Liebert for providing the integron-positive strains and James Zhu for helpful discussions concerning the sequencing data. This work was supported by funds from the State of Texas ATP ATP: see adenosine triphosphate. ATP in full adenosine triphosphate Organic compound, substrate in many enzyme-catalyzed reactions (see catalysis) in the cells of animals, plants, and microorganisms. project 00517-0361-1999, the U.S. Department of Agriculture (USDA USDA, n.pr See United States Department of Agriculture. )/CSREES-IFAFS grant 00-52102-9637, the USDA CSREES CSREES Cooperative State Research, Education, and Extension Service (USDA) grant 2001-34461-10405 and Hatch grant H8708. References (1.) Ochman H, Lawrence JG, Groisman EA. Lateral gene transfer and the nature of bacterial innovation. Nature 2000;405:299-304. (2.) Lucey B, Crowley D, Moloney P, Cryan B, Daly M, O'Halloran F, et al. Integronlike structures in Campylobacter spp. of human and animal origin. Emerg Infect Dis 2000;6:50-5. (3.) Zhao S, White DG, Ge B, Ayers S, Friedman S, English L, et al. Identification and characterization of integron-mediated antibiotic resistance among Shiga toxin-producing Escherichia coli isolates. Appl Environ Microbiol 2001;67:1558-64. (4.) Briggs CE, Fratamico PM. Molecular characterization of an antibiotic resistance gene cluster of Salmonella typhimurium DT104. Antimicrob Agents Chemother 1999;43:846-9. (5.) Mroz RC Jr, Pillai SD. Bacterial populations in the groundwater on the US-Mexico border in El Paso County, Texas El Paso County is the westernmost county in the U.S. state of Texas. According to the 2005 U.S. Census population estimates, the county had a population of 721,598. Its county seat is El Paso6. El Paso is Spanish for "the Pass. . South Med J 1994;87:214-7. (6.) Pillai SD, Widmer KW, Maciorowski KG, Ricke SC. Antibiotic resistance profiles of Escherichia coli isolated from rural and urban environments. J Environ Sci Health 1997;32:1665-75. (7.) International Boundary and Water Commission The International Boundary and Water Commission (Spanish: Comisión Internacional de Límites y Aguas) is an international body created in 1889 by the United States and Mexico to administer the many boundary and water-rights treaties and agreements between the two nations. . Water Bulletin #63: Flow of the Rio Grande and related data. El Paso (TX): The Commission; 1993. p. 132. (8.) Scandura JE, Sobsey MD. Viral and bacterial contamination of groundwater from on-site sewage treatment systems. Water Sci Technol 1997;35:141-6. (9.) Rayburn EL, Sternes KL, Weidenfeld RP, Pillai SD. Microbial pathogens in irrigation canals and associated sediments. In: Proceedings of the 101st General Meeting of the American Society for Microbiology The American Society for Microbiology (ASM) is a scientific organization, based in the United States although with over 43,000 members throughout the world. It is the largest single life science professional organization and its members include those whose interests encompass basic . 2001. Orlando (FL): American Society for Microbiology; 2001. (10.) Food and Drug Administration. Bacteriological bac·te·ri·ol·o·gy n. The study of bacteria, especially in relation to medicine and agriculture. bac·te analytical manual online. 8th ed. 2001. Available from: URL URL in full Uniform Resource Locator Address of a resource on the Internet. The resource can be any type of file stored on a server, such as a Web page, a text file, a graphics file, or an application program. : http://www.cfsan.fda.gov/~ebam/bam-toc.html (11.) National Committee for Clinical Laboratory Studies. Methods for dilution antimicrobial susceptibility tests for bacteria that grow aerobically. Vol. 10. Villanova (PA): The Committee; 1999. p. 33. (12.) Centers for Disease Control and Prevention/Food and Drug Administration; U.S. Department of Agriculture. National Antibiotic Resistance Monitoring System. Atlanta: The Centers; 1999. (13.) Levesque C, Piche L, Larose C, Roy PH. PCR mapping of integrons reveals several novel combinations of resistance genes. Antimicrob Agents Chemother 1995;39: 185-91. (14.) White PA, McIver CJ, Rawlinson WD. Integrons and gene cassettes in the enterobacteriaceae. Antimicrob Agents Chemother 2001;45:2658-61. (15.) Mazel D, Dychinco B, Webb VA, Davies J. Antibiotic resistance in the ECOR ECOR Engineering Committee on Oceanic Resources ECOR Escherichia coli Reference Collection collection: integrons and identification of a novel aad gene. Antimicrob Agents Chemother 2000;44:1568-74. (16.) Huang X, Madan A. CAP3: a DNA sequence assembly program. Genome Res 1999;9:868-77. (17.) Altschul SF, Gish W, Miller W, Myers EW, Lipman DJ. Basic local alignment search tool. J Mol Biol 1990;215:403-10. (18.) Thompson JD, Higgins DG, Gibson TJ. CLUSTAL W: improving the sensitivity of progressive multiple sequence alignment through sequence weighting, position-specific gap penalties and weight matrix choice. Nucleic Acids Res 1994;22:4673-80. (19.) Ash RJ. Antibiotic resistance of gram-negative bacteria in rivers, United States. Emerg Infect Dis 2002;8:713-6. (20.) Goni-Urriza M, Capdepuy M, Arpin C, Raymond N, Caumette P, Quentin C, et al. Impact of an urban effluent on antibiotic resistance of riverine riv·er·ine adj. 1. Relating to or resembling a river. 2. Located on or inhabiting the banks of a river; riparian: "Members of a riverine tribe ... Enterobacteriaceae and Aeromonas spp. Appl Environ Microbiol 2000;66:125-32. (21.) American Academy of Microbiology. Antimicrobial resistance: an ecological perspective. Washington: American Society for Microbiology; 1999. p. 1-14. (22.) Wegener HC, Aarestrup FM, Jensen LB, Hammerum AM, Bager F. Use of antimicrobial growth promoters in food animals and Enterococcus faecium resistance to therapeutic antimicrobial drugs in Europe. Emerg Infect Dis 1999;5:329-35. (23.) Hall RM, Collis CM. Antibiotic resistance in gram-negative bacteria: the role of gene cassettes and integrons. Drug Resist Updat 1998;1:109-19. (24.) Bass L, Liebert CA, Lee MD, Summers AO, White DG, Thayer SG, et al. Incidence and characterization of integrons, genetic elements mediating multiple-drug resistance, in avian Escherichia coli. Antimicrob Agent Chemother 1999;43:2925-9. (25.) Cech I, Essman A. Water sanitation practices on the Texas-Mexico border: implications for physicians on both sides. South Med J 1992;85:1053-64. (26.) McEwen SA, Fedorka-Cray PJ. Antimicrobial use and resistance in animals. Clin Infect Dis 2002;34(Suppl 3):S93-106. (27.) Schwarz S, Chaslus-Dancla E. Use of antimicrobials in veterinary medicine and mechanisms of resistance. Vet Res 2001;32:201-25. (28.) Texas Water Development Board. New Mexico Water Resources Research Institute. Transboundary aquifers of the El Paso/Ciudad Juarez/Las Cruces region. El Paso (TX): The Institute; 1997. p. 152. (29.) Simpson JM, Santo Domingo JW, Reasoner DJ. Microbial source tracking: state of the science. Environ Sci Technol 2002;36:5279-88. (30.) Rosser SJ, Young HK. Identification and characterization of class 1 integrons in bacteria from an aquatic environment. J Antimicrob Chemother 1999;44:11-8. (31.) Sundstrom L, Radstrom P, Swedberg G, Skold O. Site-specific recombination promotes linkage between trimethoprim- and sulfonamideresistance genes. Sequence characterization of dhfrV and sull n. 1. A plow. and a recombination active locus of Tn21. Mol Gen Genet 1988;213:191-201. (32.) Pillai SD, Pepper IL. Transposon Tn5 as an identifiable marker in Rhizobia Rhizobia (from the Greek words rhiza = root and bios = Life) are soil bacteria that fix nitrogen (diazotrophy) after becoming established inside root nodules of legumes (Fabaceae). The rhizobia cannot independently fix nitrogen, and require a plant host. : survival and genetic stability of Tn5 mutant bean Rhizobia under temperature stressed conditions in desert soils. Microb Ecol 1990;21:21-33. (33.) Sundstrom L, Roy PH, Skold O. Site-specific insertion of three structural gene cassettes in transposon Tn7. J Bacteriol 1991;173:3025-8. (34.) Hansson K, Sundstrom L, Pelletier A, Roy PH. IntI2 integron integrase in Tn7. J Bacteriol 2002;184:1712-21. (35.) Huovinen P, Sundstrom L, Swedberg G, Skold O. Trimethoprim and sulfonamide resistance. Antimicrob Agents Chemother 1995;39:279-89. Address for correspondence: Suresh D. Pillai, Department of Poultry Science, 418D Kleberg Center, MS 2472 TAMUS, Texas A&M University, College Station, Texas College Station is a city in Brazos County, Texas, situated in Central Texas. It is located in the heart of the Brazos Valley. The city is located within the most populated region of Texas, near to three of the 10 largest cities in the United States - Houston, Dallas, and San 77843-2472, USA; fax: 979-845-1921; email: spillai@poultry.tamu.edu Matthew T. Roe, * Everardo Vega, * and Suresh D. Pillai * * Texas A&M University, College Station, Texas, USA Mr. Roe conducted this study while an M.S. student in the Food Safety and Environmental Microbiology Laboratory in the Poultry Science Department at Texas A&M University. His research interests are in environmental microbiology and food safety. |
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