Transposons Tn
            <i>1696</i>
            and Tn
            <i>21</i>
            and Their Integrons In4 and In2 Have Independent Origins

Partridge, Sally R.; Brown, Heidi J.; Stokes, H. W.; Hall, Ruth M.

doi:10.1128/aac.45.4.1263-1270.2001

Cited by 169 publications

(171 citation statements)

References 53 publications

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“…However, the estimated sizes of the products (3.5 kb, 2.0 kb, and 1.0 kb, respectively) were all about 0.7 kb smaller than predicted for the standard In4-type integron configuration (26), which is present at the right-hand end of In104 in SGI1 (Fig. 1) and SGI1-A to SGI1-J.…”

Section: Resultsmentioning

confidence: 93%

SGI1-K, a Variant of the SGI1 Genomic Island Carrying a Mercury Resistance Region, in Salmonella enterica Serovar Kentucky

Levings

Partridge

Djordjevic

et al. 2007

Antimicrob Agents Chemother

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A multiple-antibiotic-resistant Salmonella enterica serovar Kentucky strain was found to contain SGI1-K, a variant form of the Salmonella genomic island 1 (SGI1) with an In4-type class 1 integron that contains only one cassette array, aacCA5-aadA7, and an adjacent mercury resistance module. Part of the 3 -conserved segment (3 -CS) of the integron, together with the inverted short segment from the right-hand end of the integron transposition module normally found between the 3 -CS and IS6100 in In4 family integrons, has been removed by an IS6100-mediated deletion. IRt, the right-hand inverted repeat found at the outer end of the integron, abuts a mercury resistance region instead of the usual SGI1 backbone segment. The mer module is a hybrid of those found in Tn501 and Tn21. This mer region and a further uncharacterized segment of at least 10 kb appear to have been incorporated between IRt and the SGI1 backbone. These findings demonstrate that the multidrug resistance region in SGI1 can incorporate new DNA segments in the same way as multiple antibiotic resistance regions in plasmids.

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Section: Resultsmentioning

confidence: 93%

SGI1-K, a Variant of the SGI1 Genomic Island Carrying a Mercury Resistance Region, in Salmonella enterica Serovar Kentucky

Levings

Partridge

Djordjevic

et al. 2007

Antimicrob Agents Chemother

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“…P. putida SP1 possessed a mer operon as a mercury-resistant determinant like most of the other mercury-resistant bacteria, and the mer operon of P. putida SP1 was located on the chromosomal DNA as described in other strains (De et al 2003;Bafana et al 2010). Because multiple resistance genes are often located on mobile genetic elements (Mindlin et al 2001;Partridge et al 2001;Barkay et al 2003) and genes encoding for heavy metal resistance are often linked to antibiotic resistance genes on the same mobile element (Mindlin et al 2002;Barkay et al 2003), the similarity between the mer operon of P. putida SP1 and the mer operon located on Tn5041 suggested that the environmental bacterium P. putida SP1 may have acquired this chromosomal mer operon and other heavy metal or antibiotic resistance determinants through transposable elements that confer resistance to HgCl 2 and a variety of other xenobiotics.…”

Section: Discussionmentioning

confidence: 99%

Characterization of a marine-isolated mercury-resistant Pseudomonas putida strain SP1 and its potential application in marine mercury reduction

Zhang

Chen

Liu

2011

Appl Microbiol Biotechnol

127

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The Pseudomonas putida strain SP1 was isolated from marine environment and was found to be resistant to 280 μM HgCl 2 . SP1 was also highly resistant to other metals, including CdCl 2 , CoCl 2 , CrCl 3 , CuCl 2 , PbCl 2 , and ZnSO 4 , and the antibiotics ampicillin (Ap), kanamycin (Kn), chloramphenicol (Cm), and tetracycline (Tc). mer operon, possessed by most mercury-resistant bacteria, and other diverse types of resistant determinants were all located on the bacterial chromosome. Cold vapor atomic absorption spectrometry and a volatilization test indicated that the isolated P. putida SP1 was able to volatilize almost 100% of the total mercury it was exposed to and could potentially be used for bioremediation in marine environments. The optimal pH for the growth of P. putida SP1 in the presence of HgCl 2 and the removal of HgCl 2 by P. putida SP1 was between 8.0 and 9.0, whereas the optimal pH for the expression of merA, the mercuric reductase enzyme in mer operon that reduces reactive Hg 2+ to volatile and relatively inert monoatomic Hg 0 vapor, was around 5.0. LD 50 of P. putida SP1 to flounder and turbot was 1.5× 10 9 CFU. Biofilm developed by P. putida SP1 was 1-to 3-fold lower than biofilm developed by an aquatic pathogen Pseudomonas fluorescens TSS. The results of this study indicate that P. putida SP1 is a low virulence strain that can potentially be applied in the bioremediation of HgCl 2 contamination over a broad range of pH.

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“…2C). Multiple resistance genes are most often located in mobile genetic elements [2,4,15], able to spread among the bacterial community very rapidly [6,12]. Considering that 62.96% of the Hgresistant bacterial strains harbored large, potentially conjugative plasmids, we were concerned by the potential acquisition of multiple resistances by human pathogens through conjugation with indigenous bacteria.…”

Section: Discussionmentioning

confidence: 99%

Mercury Resistance in Bacterial Strains Isolated from Tailing Ponds in a Gold Mining Area Near El Callao (Bolívar State, Venezuela)

et al. 2007

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Abstract. Bacterial resistance to mercury (Hg) was investigated in strains isolated from Hg-contaminated tailing ponds located in the gold mining area of El Callao (Bolívar State, Venezuela). High frequencies of resistance were detected to both inorganic-Hg and organomercurials among these strains. A broad range of resistance levels was observed when determining minimal inhibitory concentrations of Hg 2+ . Some strains were able to grow in liquid medium containing 25 lM Hg 2+ , whereas others grew at 300 lM Hg 2+ . Of 190 Hg-resistant strains tested, 58.2% were additionally shown to be resistant to ampicillin (40 mg/L), 33.3% to chloramphenicol (30 mg/L), 24.9% to streptomycin (30 mg/L), 23.3% to tetracycline (30 mg/L), and 1.6% to kanamycin (30 mg/L). Furthermore, we found that 20% of the Hgresistant strains were simultaneously resistant to as many as four of these antibiotics, at the concentrations tested. The presence of large plasmids in 62.9% of 53 Hg-resistant strains screened prompted us to investigate the horizontal transfer of resistance determinants. Mating experiments were performed using Escherichia coli and Pseudomonas aeruginosa as recipient strains. The results obtained confirmed that indigenous Hg-resistant bacteria colonizing the tailing ponds can effectively transfer the phenotype to potentially pathogenic species.

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Transposons Tn 1696 and Tn 21 and Their Integrons In4 and In2 Have Independent Origins

Cited by 169 publications

References 53 publications

SGI1-K, a Variant of the SGI1 Genomic Island Carrying a Mercury Resistance Region, in Salmonella enterica Serovar Kentucky

SGI1-K, a Variant of the SGI1 Genomic Island Carrying a Mercury Resistance Region, in Salmonella enterica Serovar Kentucky

Characterization of a marine-isolated mercury-resistant Pseudomonas putida strain SP1 and its potential application in marine mercury reduction

Mercury Resistance in Bacterial Strains Isolated from Tailing Ponds in a Gold Mining Area Near El Callao (Bolívar State, Venezuela)

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