Providencia Stuartii, a Hospital Pathogen: Potential Factors for Its Emergence and Transmission

Wenzel, Richard P.; Hunting, Kathryn J.; Osterman, Charles A.; Sande, Merle A.

doi:10.1093/oxfordjournals.aje.a112287

Cited by 30 publications

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“…The bacteria of the genus Providencia are gram negative and rod shaped and belong to the family Enterobacteriaceae. They have been reported to cause infections of the intestinal tract (1, 12) and the urinary tract (6, 15) and have been implicated in the establishment of nosocomial infections (3,7,12,14,16,17).Our interest in these bacteria has led us to establish serotyping schemes, and we have serotyped numerous isolates ofeach species during the course of other investigations (8)(9)(10) (4). A collection of 630 P. stuartii isolates included both urea-negative and ureapositive isolates from different hospitals as described previously (10), and the 537 P. rettgeri isolates in our collection were mostly those that were described earlier (9) and included isolates from different hospitals, public health laboratories, animals, and polluted water.…”

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confidence: 99%

Differences among Providencia species in their in vitro susceptibilities to five antibiotics

Penner¹,

Preston²

1980

Antimicrob Agents Chemother

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Significant differences among the three Providencia species (P. alcalifaciens, P. stuartii, and P. rettgeri) in antimicrobial susceptibilities to five antibiotics were shown. P. stuartii was the most resistant of the three species, and P. alcalifaciens was the most susceptible. P. rettgeri was similar to P. stuartii in susceptibilities to cefoxitin, cephalothin, and cefamandole but differed in showing greater susceptibilities to tobramycin and gentamicin. Cefoxitin (16 jAg/ml) and cefamandole (16 yg/ml) inhibited a greater proportion of P. stuartii isolates than did cephalothin, tobramycin, or gentamicin. The susceptibilities of urea-positive isolates of P. stuartii resembled more closely the susceptibilities of urea-negative isolates of this species than those of P. rettgeri isolates, a finding consistent with the recent recommendation for transferring such urea-positive strains to P. stuartii. Among P. stuartii isolates, marked resistance to cefoxitin accompanied by susceptibility to cefamandole was predominantly restricted to isolates of one serotype (055). The use of isolates that had been serotyped and clafied according to recent proposals for taxonomic changes in the Proteeae provided for clearer demonstration of species differences in susceptibility.The genus Providencia, according to recent proposals for reclasification (2), includes three species, namely, P. alcalifaciens, P. stuartii, and P. rettgeri. The latter species was previously included in the genus Proteus, and some ureapositive isolates now classified as P. stuartii were usually classified also as Proteus rettgeri (11). The bacteria of the genus Providencia are gram negative and rod shaped and belong to the family Enterobacteriaceae. They have been reported to cause infections of the intestinal tract (1, 12) and the urinary tract (6, 15) and have been implicated in the establishment of nosocomial infections (3,7,12,14,16,17).Our interest in these bacteria has led us to establish serotyping schemes, and we have serotyped numerous isolates ofeach species during the course of other investigations (8)(9)(10) (4). A collection of 630 P. stuartii isolates included both urea-negative and ureapositive isolates from different hospitals as described previously (10), and the 537 P. rettgeri isolates in our collection were mostly those that were described earlier (9) and included isolates from different hospitals, public health laboratories, animals, and polluted water. All isolates were serotyped in connection with previous studies or at the request of the contributors. Currently, 46, 17, and 93 0 serotypes have been reported for P. alcalifaciens (8), P. stuartii (10), and P. rettgeri (9), respectively, and isolates of each serotype were included in the respective collections. The distribution of the isolates according to their serotypes has been published previously (8)(9)(10).Antibiotics.

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confidence: 99%

Differences among Providencia species in their in vitro susceptibilities to five antibiotics

Penner¹,

Preston²

1980

Antimicrob Agents Chemother

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“…In the past decades, Gram-negative organisms have emerged as the most common etiologic agents of invasive infections, and antibiotic-resistant organisms have increasingly been isolated in burn units (10). However, very few studies have reported endemic or epidemic situations due to P. stuartii in these wards (11,41,53). Most patients of this study suffered from severe burn injury (mean TBSA, greater than 40%) and thus exhibited risk factors for acquiring multidrug-resistant bacteria, i.e., antibiotic receipt, extended duration of hospitalization, and invasive procedures, together with immunosuppression induced by the burn injury (10,50).…”

Section: Discussionmentioning

confidence: 99%

“…Indeed, this opportunistic pathogen is essentially responsible for urinary tract infections, particularly in long-term care populations (33). P. stuartii is intrinsically resistant to aminopenicillins and narrow-spectrum cephalosporins due to a chromosomally encoded Ambler class C cephalosporinase (12,22,53). Overexpression of AmpC usually confers to this species a low-level resistance to broad-spectrum cephalosporins such as ceftazidime (12).…”

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confidence: 99%

Evolution of an Incompatibility Group IncA/C Plasmid Harboring bla _CMY-16 and qnrA6 Genes and Its Transfer through Three Clones of Providencia stuartii during a Two-Year Outbreak in a Tunisian Burn Unit

Arpin

Thabet²,

Yassine

et al. 2012

Antimicrob Agents Chemother

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During a 2-year period in 2005 and 2006, 64 multidrug-resistant Providencia stuartii isolates, including 58 strains from 58 patients and 6 strains obtained from the same tracheal aspirator, were collected in a burn unit of a Tunisian hospital. They divided into four antibiotypes (ATB1 to ATB4) and three SmaI pulsotypes (PsA to PsC), including 49 strains belonging to clone PsA (48 of ATB1 and 1 of ATB4), 11 strains to clone PsB (7 of ATB2 and 4 of ATB3), and 4 strains to clone PsC (ATB3). All strains, except for the PsA/ATB4 isolate, were highly resistant to broad-spectrum cephalosporins due to the production of the plasmidmediated CMY-16 ␤-lactamase. In addition, the 15 strains of ATB2 and ATB3 exhibited decreased quinolone susceptibility associated with QnrA6. Most strains (ATB1 and ATB3) were gentamicin resistant, related to an AAC(6=)-Ib= enzyme. All these genes were located on a conjugative plasmid belonging to the incompatibility group IncA/C 2 of 195, 175, or 100 kb. Despite differences in size and in number of resistance determinants, they derived from the same plasmid, as demonstrated by similar profiles in plasmid restriction analysis and strictly homologous sequences of repAIncA/C 2 , unusual antibiotic resistance genes (e.g., aphA-6), and their genetic environments. Further investigation suggested that deletions, acquisition of the ISCR1 insertion sequence, and integron cassette mobility accounted for these variations. Thus, this outbreak was due to both the spread of three clonal strains and the dissemination of a single IncA/C 2 plasmid which underwent a remarkable evolution during the epidemic period.

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“…The development of bacterial resistance to silver nitrate (Cason et al 1966;Cason and Lowburry 1968) prompted a change in formulation and the use of silver sulphadiazine -a combination of silver and sulphonamide (Fox 1968;Modax and Fox 1974;Modak et al 1988). In the 1970s, outbreaks of burn wound infection or colonization by Gram-negative isolates resistant to ionic silver and silver sulphadiazine were reported for a number of bacteria; in Enterobacter cloacae (Gayle et al 1978), Providencia stuartii (Wenzel et al 1976), Pseudomonas aeruginosa (Bridges et al 1979) and Salmonella typhimurium (Mchugh et al 1975). Bacterial resistance to silver sulphadiazine developed rapidly mainly because of the antibiotic component (Klasen 2000).…”

Section: Bacterial Resistance To Silver and Ag-npmentioning

confidence: 99%

“…In vitro evidence of bacterial resistance to ionic silver Exposure to silver may contribute to the selection of bacteria that are intrinsically resistant to silver (Wenzel et al 1976;Bridges and Lowburry 1977;Haefeli et al 1984;Silver 2003;Davis et al 2005). Emerging silver-resistance from environmental bacterial isolates has been documented in Enterobacteriaceae (Hendry et al 1979;Kaur and Vadehra 1986;Trevors 1989, 1990) and in Acinetobacter baumanii (Deshpande and Chopade 1994) under experimental conditions.…”

Section: Bacterial Resistance To Silver and Ag-npmentioning

confidence: 99%

Potential risks and benefits of nanotechnology: perceptions of risk in sunscreens

Wright

2016

Medical Journal of Australia

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Providencia Stuartii, a Hospital Pathogen: Potential Factors for Its Emergence and Transmission

Cited by 30 publications

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Differences among Providencia species in their in vitro susceptibilities to five antibiotics

Differences among Providencia species in their in vitro susceptibilities to five antibiotics

Evolution of an Incompatibility Group IncA/C Plasmid Harboring bla _CMY-16 and qnrA6 Genes and Its Transfer through Three Clones of Providencia stuartii during a Two-Year Outbreak in a Tunisian Burn Unit

Potential risks and benefits of nanotechnology: perceptions of risk in sunscreens

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Providencia Stuartii, a Hospital Pathogen: Potential Factors for Its Emergence and Transmission

Cited by 30 publications

References 0 publications

Differences among Providencia species in their in vitro susceptibilities to five antibiotics

Differences among Providencia species in their in vitro susceptibilities to five antibiotics

Evolution of an Incompatibility Group IncA/C Plasmid Harboring bla CMY-16 and qnrA6 Genes and Its Transfer through Three Clones of Providencia stuartii during a Two-Year Outbreak in a Tunisian Burn Unit

Potential risks and benefits of nanotechnology: perceptions of risk in sunscreens

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Evolution of an Incompatibility Group IncA/C Plasmid Harboring bla _CMY-16 and qnrA6 Genes and Its Transfer through Three Clones of Providencia stuartii during a Two-Year Outbreak in a Tunisian Burn Unit