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1.
Background
The Salmonella genomic island 1 (SGI1) is a 42.4 kb integrative mobilizable element containing several antibiotic resistance determinants embedded in a complex integron segment In104. The numerous SGI1 variants identified so far, differ mainly in this segment and the explanations of their emergence were mostly based on comparative structure analyses. Here we provide experimental studies on the stability, entrapment and variant formation of this peculiar gene cluster originally found in S. Typhimurium.Methodology/Principal Findings
Segregation and conjugation tests and various molecular techniques were used to detect the emerging SGI1 variants in Salmonella populations of 17 Salmonella enterica serovar Typhimurium DT104 isolates from Hungary. The SGI1s in these isolates proved to be fully competent in excision, conjugal transfer by the IncA/C helper plasmid R55, and integration into the E. coli chromosome. A trap vector has been constructed and successfully applied to capture the island on a plasmid. Monitoring of segregation of SGI1 indicated high stability of the island. SGI1-free segregants did not accumulate during long-term propagation, but several SGI1 variants could be obtained. Most of them appeared to be identical to SGI1-B and SGI1-C, but two new variants caused by deletions via a short-homology-dependent recombination process have also been detected. We have also noticed that the presence of the conjugation helper plasmid increased the formation of these deletion variants considerably.Conclusions/Significance
Despite that excision of SGI1 from the chromosome was proven in SGI1+ Salmonella populations, its complete loss could not be observed. On the other hand, we demonstrated that several variants, among them two newly identified ones, arose with detectable frequencies in these populations in a short timescale and their formation was promoted by the helper plasmid. This reflects that IncA/C helper plasmids are not only involved in the horizontal spreading of SGI1, but may also contribute to its evolution. 相似文献2.
Vandenbroucke V Croubels S Martel A Verbrugghe E Goossens J Van Deun K Boyen F Thompson A Shearer N De Backer P Haesebrouck F Pasmans F 《PloS one》2011,6(8):e23871
Background and Aims
Both deoxynivalenol (DON) and nontyphoidal salmonellosis are emerging threats with possible hazardous effects on both human and animal health. The objective of this study was to examine whether DON at low but relevant concentrations interacts with the intestinal inflammation induced by Salmonella Typhimurium.Methodology
By using a porcine intestinal ileal loop model, we investigated whether intake of low concentrations of DON interacts with the early intestinal inflammatory response induced by Salmonella Typhimurium.Results
A significant higher expression of IL-12 and TNFα and a clear potentiation of the expression of IL-1β, IL-8, MCP-1 and IL-6 was seen in loops co-exposed to 1 µg/mL of DON and Salmonella Typhimurium compared to loops exposed to Salmonella Typhimurium alone. This potentiation coincided with a significantly enhanced Salmonella invasion in and translocation over the intestinal epithelial IPEC-J2 cells, exposed to non-cytotoxic concentrations of DON for 24 h. Exposure of Salmonella Typhimurium to 0.250 µg/mL of DON affected the bacterial gene expression level of a limited number of genes, however none of these expression changes seemed to give an explanation for the increased invasion and translocation of Salmonella Typhimurium and the potentiated inflammatory response in combination with DON.Conclusion
These data imply that the intake of low and relevant concentrations of DON renders the intestinal epithelium more susceptible to Salmonella Typhimurium with a subsequent potentiation of the inflammatory response in the gut. 相似文献3.
Background
The Salmonella genomic island 1 (SGI1) is a Salmonella enterica-derived integrative mobilizable element (IME) containing various complex multiple resistance integrons identified in several S. enterica serovars and in Proteus mirabilis. Previous studies have shown that SGI1 transfers horizontally by in trans mobilization in the presence of the IncA/C conjugative helper plasmid pR55.Methodology/Principal Findings
Here, we report the ability of different prevalent multidrug resistance (MDR) plasmids including extended-spectrum β-lactamase (ESBL) gene-carrying plasmids to mobilize the multidrug resistance genomic island SGI1. Through conjugation experiments, none of the 24 conjugative plasmids tested of the IncFI, FII, HI2, I1, L/M, N, P incompatibility groups were able to mobilize SGI1 at a detectable level (transfer frequency <10−9). In our collection, ESBL gene-carrying plasmids were mainly from the IncHI2 and I1 groups and thus were unable to mobilize SGI1. However, the horizontal transfer of SGI1 was shown to be specifically mediated by conjugative helper plasmids of the broad-host-range IncA/C incompatibility group. Several conjugative IncA/C MDR plasmids as well as the sequenced IncA/C reference plasmid pRA1 of 143,963 bp were shown to mobilize in trans SGI1 from a S. enterica donor to the Escherichia coli recipient strain. Depending on the IncA/C plasmid used, the conjugative transfer of SGI1 occurred at frequencies ranging from 10−3 to 10−6 transconjugants per donor. Of particular concern, some large IncA/C MDR plasmids carrying the extended-spectrum cephalosporinase bla CMY-2 gene were shown to mobilize in trans SGI1.Conclusions/Significance
The ability of the IncA/C MDR plasmid family to mobilize SGI1 could contribute to its spread by horizontal transfer among enteric pathogens. Moreover, the increasing prevalence of IncA/C plasmids in MDR S. enterica isolates worldwide has potential implications for the epidemic success of the antibiotic resistance genomic island SGI1 and its close derivatives. 相似文献4.
Background
The objective was to investigate the phenotypic and genotypic resistance and the horizontal transfer of resistance determinants from Salmonella isolates from humans and animals in Vietnam.Methodology/Principal Findings
The susceptibility of 297 epidemiologically unrelated non-typhoid Salmonella isolates was investigated by disk diffusion assay. The isolates were screened for the presence of class 1 integrons and Salmonella genomic island 1 by PCR. The potential for the transfer of resistance determinants was investigated by conjugation experiments. Resistance to gentamicin, kanamycin, chloramphenicol, streptomycin, trimethoprim, ampicillin, nalidixic acid, sulphonamides, and tetracycline was found in 13 to 50% of the isolates. Nine distinct integron types were detected in 28% of the isolates belonging to 11 Salmonella serovars including S. Tallahassee. Gene cassettes identified were aadA1, aadA2, aadA5, bla PSE-1, bla OXA-30, dfrA1, dfrA12, dfrA17, and sat, as well as open reading frames with unknown functions. Most integrons were located on conjugative plasmids, which can transfer their antimicrobial resistance determinants to Escherichia coli or Salmonella Enteritidis, or with Salmonella Genomic Island 1 or its variants. The resistance gene cluster in serovar Emek identified by PCR mapping and nucleotide sequencing contained SGI1-J3 which is integrated in SGI1 at another position than the majority of SGI1. This is the second report on the insertion of SGI1 at this position. High-level resistance to fluoroquinolones was found in 3 multiresistant S. Typhimurium isolates and was associated with mutations in the gyrA gene leading to the amino acid changes Ser83Phe and Asp87Asn.Conclusions
Resistance was common among Vietnamese Salmonella isolates from different sources. Legislation to enforce a more prudent use of antibiotics in both human and veterinary medicine should be implemented by the authorities in Vietnam. 相似文献5.
Background
In comparison to the comprehensive analyses performed on virulence gene expression, regulation and action, the intracellular metabolism of Salmonella during infection is a relatively under-studied area. We investigated the role of the tricarboxylic acid (TCA) cycle in the intracellular replication of Salmonella Typhimurium in resting and activated macrophages, epithelial cells, and during infection of mice.Methodology/Principal Findings
We constructed deletion mutations of 5 TCA cycle genes in S. Typhimurium including gltA, mdh, sdhCDAB, sucAB, and sucCD. We found that the mutants exhibited increased net intracellular replication in resting and activated murine macrophages compared to the wild-type. In contrast, an epithelial cell infection model showed that the S. Typhimurium ΔsucCD and ΔgltA strains had reduced net intracellular replication compared to the wild-type. The glyoxylate shunt was not responsible for the net increased replication of the TCA cycle mutants within resting macrophages. We also confirmed that, in a murine infection model, the S. Typhimurium ΔsucAB and ΔsucCD strains are attenuated for virulence.Conclusions/Significance
Our results suggest that disruption of the TCA cycle increases the ability of S. Typhimurium to survive within resting and activated murine macrophages. In contrast, epithelial cells are non-phagocytic cells and unlike macrophages cannot mount an oxidative and nitrosative defence response against pathogens; our results show that in HeLa cells the S. Typhimurium TCA cycle mutant strains show reduced or no change in intracellular levels compared to the wild-type [1]. The attenuation of the S. Typhimurium ΔsucAB and ΔsucCD mutants in mice, compared to their increased net intracellular replication in resting and activated macrophages suggest that Salmonella may encounter environments within the host where a complete TCA cycle is advantageous. 相似文献6.
Sharon M. Tennant Souleymane Diallo Haim Levy Sofie Livio Samba O. Sow Milagritos Tapia Patricia I. Fields Matthew Mikoleit Boubou Tamboura Karen L. Kotloff James P. Nataro James E. Galen Myron M. Levine 《PLoS neglected tropical diseases》2010,4(3)
Background
In sub-Saharan Africa, non-typhoidal Salmonella (NTS) are emerging as a prominent cause of invasive disease (bacteremia and focal infections such as meningitis) in infants and young children. Importantly, including data from Mali, three serovars, Salmonella enterica serovar Typhimurium, Salmonella Enteritidis and Salmonella Dublin, account for the majority of non-typhoidal Salmonella isolated from these patients.Methods
We have extended a previously developed series of polymerase chain reactions (PCRs) based on O serogrouping and H typing to identify Salmonella Typhimurium and variants (mostly I 4,[5],12:i:-), Salmonella Enteritidis and Salmonella Dublin. We also designed primers to detect Salmonella Stanleyville, a serovar found in West Africa. Another PCR was used to differentiate diphasic Salmonella Typhimurium and monophasic Salmonella Typhimurium from other O serogroup B, H:i serovars. We used these PCRs to blind-test 327 Salmonella serogroup B and D isolates that were obtained from the blood cultures of febrile patients in Bamako, Mali.Principal Findings
We have shown that when used in conjunction with our previously described O-serogrouping PCR, our PCRs are 100% sensitive and specific in identifying Salmonella Typhimurium and variants, Salmonella Enteritidis, Salmonella Dublin and Salmonella Stanleyville. When we attempted to differentiate 171 Salmonella Typhimurium (I 4,[ 5],12:i:1,2) strains from 52 monophasic Salmonella Typhimurium (I 4,[5],12:i:-) strains, we were able to correctly identify 170 of the Salmonella Typhimurium and 51 of the Salmonella I 4,[5],12:i:- strains.Conclusion
We have described a simple yet effective PCR method to support surveillance of the incidence of invasive disease caused by NTS in developing countries. 相似文献7.
Background
Nontyphoidal Salmonellae frequently cause life-threatening bacteremia in sub-Saharan Africa. Young children and HIV-infected adults are particularly susceptible. High case-fatality rates and increasing antibiotic resistance require new approaches to the management of this disease. Impaired cellular immunity caused by defects in the T helper 1 pathway lead to intracellular disease with Salmonella that can be countered by IFNγ administration. This report identifies the lymphocyte subsets that produce IFNγ early in Salmonella infection.Methodology
Intracellular cytokine staining was used to identify IFNγ production in blood lymphocyte subsets of ten healthy adults with antibodies to Salmonella (as evidence of immunity to Salmonella), in response to stimulation with live and heat-killed preparations of the D23580 invasive African isolate of Salmonella Typhimurium. The absolute number of IFNγ-producing cells in innate, innate-like and adaptive lymphocyte subpopulations was determined.Principal Findings
Early IFNγ production was found in the innate/innate-like lymphocyte subsets: γδ-T cells, NK cells and NK-like T cells. Significantly higher percentages of such cells produced IFNγ compared to adaptive αβ-T cells (Student''s t test, P<0.001 and ≤0.02 for each innate subset compared, respectively, with CD4+- and CD8+-T cells). The absolute numbers of IFNγ-producing cells showed similar differences. The proportion of IFNγ-producing γδ-T cells, but not other lymphocytes, was significantly higher when stimulated with live compared with heat-killed bacteria (P<0.0001).Conclusion/Significance
Our findings indicate an inherent capacity of innate/innate-like lymphocyte subsets to produce IFNγ early in the response to Salmonella infection. This may serve to control intracellular infection and reduce the threat of extracellular spread of disease with bacteremia which becomes life-threatening in the absence of protective antibody. These innate cells may also help mitigate against the effect on IFNγ production of depletion of Salmonella-specific CD4+-T lymphocytes in HIV infection. 相似文献8.
de Wit J Souwer Y Jorritsma T Klaasse Bos H ten Brinke A Neefjes J van Ham SM 《PloS one》2010,5(9):e13016
Background
The eradication of facultative intracellular bacterial pathogens, like Salmonella typhi, requires the concerted action of both the humoral immune response and the cytotoxic CD8+ T cell response. Dendritic cells (DCs) are considered to orchestrate the cytotoxic CD8+ T cell response via cross-presentation of bacterial antigens onto MHC class I molecules. Cross-presentation of Salmonella by DCs however, is accompanied by the induction of apoptosis in the DCs. Besides antibody production, B cells are required to clear Salmonella infection for other unknown reasons.Methodology/Principal Findings
Here we show that Salmonella-specific B cells that phagocytose Salmonella upon BCR-ligation reactivate human memory CD8+ T cells via cross-presentation yielding a Salmonella-specific cytotoxic T cell response. The reactivation of CD8+ T cells is dependent on CD4+ T cell help. Unlike the DCs, B cell-mediated cross-presentation of Salmonella does not coincide with apoptosis.Conclusions/Significance
B cells form a new player in the activation of the cytotoxic effector arm of the immune response and the generation of effective adaptive immunity in Salmonella infection. 相似文献9.
Yew Joon Tam Zeenathul Nazariah Allaudin Mohd Azmi Mohd Lila Abdul Rani Bahaman Joo Shun Tan Morvarid Akhavan Rezaei 《BMC biotechnology》2012,12(1):1-15
Background
Solely in Europoe, Salmonella Typhimurium causes more than 100,000 infections per year. Improved detection of livestock colonised with S. Typhimurium is necessary to prevent foodborne diseases. Currently, commercially available ELISA assays are based on a mixture of O-antigens (LPS) or total cell lysate of Salmonella and are hampered by cross-reaction. The identification of novel immunogenic proteins would be useful to develop ELISA based diagnostic assays with a higher specificity.Results
A phage display library of the entire Salmonella Typhimurium genome was constructed and 47 immunogenic oligopeptides were identified using a pool of convalescent sera from pigs infected with Salmonella Typhimurium. The corresponding complete genes of seven of the identified oligopeptids were cloned. Five of them were produced in E. coli. The immunogenic character of these antigens was validated with sera from pigs infeced with S. Tyhimurium and control sera from non-infected animals. Finally, human antibody fragments (scFv) against these five antigens were selected using antibody phage display and characterised.Conclusion
In this work, we identified novel immunogenic proteins of Salmonella Typhimurium and generated antibody fragments against these antigens completely based on phage display. Five immunogenic proteins were validated using a panel of positive and negative sera for prospective applications in diagnostics of Salmonela Typhimurium. 相似文献10.
Alison E. Barnhill Katherine E. Weeks Nalee Xiong Tim A. Day Steve A. Carlson 《Applied and environmental microbiology》2010,76(8):2678-2680
This study assessed the ability of Salmonella (572 isolates) to subsist on 12 different antibiotics. The majority (11/12) of the antibiotics enabled subsistence for at least 1 of 140 isolates. Furthermore, 40 isolates were able to subsist on more than one antibiotic. Antibiotic resistance and antibiotic subsistence do not appear to be equivalent.A recent study found that a diverse group of bacteria, including intrinsically resistant microbes (e.g., Pseudomonadales and Burkholderiales), could subsist on and presumably catabolize antibiotics as a sole carbon source. This group includes bacteria related to the pathogens Burkholderia cepacia and Serratia marcesens (5). This phenotype has also previously been reported for catabolism of chloramphenicol by Streptomyces (1) and beta-lactams by Leptospira (8) and Pseudomonas (7).In the current study, we assessed this subsistence phenotype in multiresistant and antibiotic-sensitive Salmonella isolates. Five hundred seventy-two isolates of Salmonella were obtained from cattle, swine, poultry, equine, beef, pork, chicken, and turkey samples (3, 6). These isolates were obtained from clinical, nonclinical, and food samples. Of the 572 isolates, 179 (31.3%) were Salmonella enterica subspecies enterica serovar Typhimurium harboring the SGI1 integron, encoding multiple antibiotic resistance (2), i.e., definitive type 104 (DT104). All Salmonella isolates were previously derived from single colonies stored at −80°C in 50% glycerol-50% LB broth (Sigma). The isolates were then inoculated into LB broth and grown aerobically for 16 h at 37°C prior to growth on single-carbon-source (SCS) medium.SCS medium was prepared as previously described (5), with 1 mg/ml of antibiotic. Since the isolates were of animal origin, the antibiotics included drugs either used in veterinary medicine or closely related to veterinary antibacterials. The antibiotics chosen were amikacin, ampicillin, cefepime (an extended-spectrum and beta-lactamase-resistant human cephalosporin chosen because of the pending FDA approval of the use of cefquinome in cattle), ceftiofur, ciprofloxacin (a metabolite of the veterinary fluoroquinolone enrofloxacin [10]), florfenicol, kanamycin, streptomycin, sulfisoxazole, tetracycline, trimethoprim, and vancomycin (chosen because of its relationship to the poultry feed additive avoparcin). Except for cefepime (Bristol-Myers Squibb Company) and florfenicol (Schering-Plough), all antibiotics were obtained from Sigma.Approximately 107 CFU were incubated on SCS agar for 16 h at 37°C. Subsistence was ascribed for isolates in which the corresponding plate contained distinct colonies; typically, 10 to 1,000 colonies were observed, i.e., a relatively low frequency (10−6 to 10−4). Representative colonies were then statically incubated in 200 μl SCS broth containing the antibiotic for 16 to 48 h at 37°C. Of the 572 isolates examined, 140 (24.5%) subsisted on at least one antibiotic. Of the 12 antibiotics examined, 11 enabled the growth of at least one Salmonella isolate. All antibiotics that provided sustenance on agar also enabled subsistence in broth. Subsistence was observed fastest in the presence the bacteriostatic agents sulfisoxazole and trimethoprim (Table (Table1).1). Tetracycline did not enable subsistence for any of the 572 isolates examined, and no isolates grew on or in SCS medium lacking an antibiotic.
Open in a separate windowaSubsistence is defined by the observation of individual distinct colonies on SCS agar or an OD600 of >0.1 for SCS broth. The Mueller-Hinton-associated MIC is also presented for each antibiotic and isolate.bNumbers in parentheses represent the cumulative number of isolates exhibiting the subsistence phenotype for a given antibiotic. No isolates exhibited the subsistence phenotype for tetracycline or antibiotic-free SCS agar or broth. (Growth in antibiotic-free broth was assessed only for certain isolates that subsisted on an antibiotic.)cNumbers in parentheses represent the number of isolates exhibiting the corresponding subsistence phenotype when more than one isolate was involved. “SGI1” indicates an isolate bearing SGI1. Of the 201 isolates exhibiting the subsistence phenotype for any antibiotic, 99 were associated with MICs of >1 mg/ml (82 of which were serovar Typhimurium isolates bearing SGI1), and 102 were associated with MICs of ≤1 mg/ml (66 of which were serovar Typhimurium isolates bearing SGI1).dNone of these isolates were able to subsist on clavulanic acid alone.eAll assessed isolates were capable of growth in SCS broth after overnight incubation (16 h), whereas all other isolates demonstrated growth after 48 h in SCS broth.Table Table22 depicts the 40 isolates that subsisted on multiple antibiotics, and 36 of these isolates possessed the SGI1 integron. Fourteen isolates were capable of subsisting on three different antibiotics, and 13 of these isolates contained SGI1.
Open in a separate windowaNumbers in parentheses represent the number of isolates exhibiting the specified multisubsistence phenotype. “SGI1” indicates an isolate bearing SGI1. An asterisk indicates that the isolate subsisted on the combination of sulfisoxasole and trimethoprim after 48 h of incubation in SCS broth but that subsistence was observed after 16 h in the presence of either drug alone.Ninety-one of the 179 SGI1-bearing DT104 isolates exhibited subsistence, while this phenotype was also observed in an SGI1-bearing isolate of Salmonella enterica subspecies enterica serovar Agona (Table (Table1).1). Antibiotic subsistence may be linked to the SGI1 structure since this activity was observed in more than half of the isolates bearing this integron. Subsistence on ampicillin was the most common phenotype in the DT104 isolates, despite uniform resistance to this antibiotic and three others (sulfisoxasole, streptomycin, and tetracycline) in these isolates. SGI1 contains nearly 30 genes unrelated to antibiotic resistance (2), and future mutagenesis studies will attempt to identify which of these elements contribute to the subsistence phenotype.Subsistence was also observed in multiple isolates from seven different non-Typhimurium serovars (Salmonella enterica subspecies enterica serovars Agona, Dublin, Heidelberg, Montevideo, Oranienberg, Typhisuis, and Worthington). Given the smaller numbers of isolates from outside the Typhimurium serotype, no conclusions can be drawn regarding serotype predilection for antibiotic subsistence. However, these results documented that 14% (56/393) of the isolates were able to subsist on an antibiotic when the data from S. Typhimurium were omitted.MICs were determined for all of the isolates that subsisted on SCS medium. Approximately 2 × 105 CFU were used in microbroth (200 μl per well; 96-well microtiter plates) 2-fold serial dilutions in Mueller-Hinton broth (Difco) per CLSI guidelines (4). MICs were ascribed to the lowest concentration of antibiotic that inhibited overnight growth as determined visually, with an approximate optical density at 600 nm (OD600) of <0.1 indicating growth inhibition. Escherichia coli ATCC 25922 was used as the control strain.As shown in Table Table1,1, antibiotic-subsisting isolates of Salmonella exhibited a variety of phenotypes in regard to in vitro antibiotic susceptibility in nutrient-rich medium. Subsistence on seven antibiotics (amikacin, cefepime, ceftiofur, florfenicol, kanamycin, trimethoprim, and vancomycin) was not related to growth at the same concentration (1 mg/ml) of the antibiotic in Mueller-Hinton broth. The majority of sulfisoxazole- and ampicillin-subsisting isolates (37/38 and 58/63, respectively) were capable of growing in Mueller-Hinton medium supplemented with the respective antibiotic at a concentration that equaled or exceeded the concentration used in the SCS medium (1 mg/ml). Streptomycin resistance was noted to occur in all seven isolates capable of subsisting on this drug, although the MIC values were less than 1 mg/ml, the concentration of drug used in the subsistence assay. Conversely, ceftiofur sensitivity was observed in the five isolates that subsisted on this antibiotic.Of the 201 individual subsistence phenotypes, 95 (57 for ampicillin, 37 for sulfisoxazole, and 1 for ciprofloxacin) coincided with growth in the presence of these antibiotics in standard medium containing 1 mg/ml of the antibiotic. The majority of ampicillin-subsisting and sulfisoxazole-subsisting isolates could grow in the presence of the respective antibiotic in nutrient-rich medium. Unlike the beta-lactamase-dependent ampicillin subsistence demonstrated in the Dantas et al. study (5), beta-lactamase activity was not relevant to ampicillin subsistence, since the inclusion of clavulanic acid (16 μg/ml) had no effect on the phenotype (Table (Table1).1). In 30 of the 37 sulfisoxazole-subsisting isolates exhibiting resistance to sulfisoxazole, resistance corresponds with the presence of sul1 on SGI1 (3), as confirmed by PCR (not shown). This gene encodes a sulfonamide-insensitive version of the enzyme targeted by this class of antibacterial agents. That is, antibiotic degradation is not required for sulfonamide resistance. Therefore, resistance mechanisms do not appear to be related to the subsistence activities, especially considering that tetracycline resistance is widespread in Salmonella (near 100% in the isolate collection used herein; data not shown), yet no isolates subsisted on tetracycline. Subsistence may relate only to certain antibiotics, and the subsistence mechanisms, e.g., those involving catabolic enzymes, may be active only during nutrient deprivation in just a small subpopulation of a given isolate. These novel putative enzymes appear to be unrelated to beta-lactamases and do not use tetracycline as a substrate. That is, subsistence and resistance do not appear to be equivalent, as also demonstrated in the Dantas et al. study (5).It is interesting that subsistence in SCS broth ensued fastest in the presence of the bacteriostatic drugs that perturb folate biosynthesis in bacteria. That is, these drugs are unable to kill Salmonella, but all of the other antibiotics examined are bactericidal. This premise is consistent with the longer incubation time required for subsistence of the single sulfisoxasole- and trimethoprim-subsisting isolate in the presence of both antibiotics (Table (Table2).2). That is, the combination of these two antibiotics is bactericidal and thus hinders the expression of subsistence, as observed with the other bactericidal antibiotics.From a clinical perspective, subsistence would be unnecessary in a host due to abundantly available carbon sources. Nonetheless, this finding raises some issues. First, subtherapeutic antibiotics may actually select for these antibiotic-subsisting bacteria, although the rock-paper-scissors paradigm (9) of intestinal microbial dynamics suggests otherwise. That is, multiple opposing forces often maintain long-term equilibria of the profiles of bacteria present in the intestines. Second, antibiotic dispersal into the environment could result in propagation of bacteria that subsist on antibiotics, although this propagation may help to minimize environmental antibiotics and other xenobiotics, including pesticides, toxins, etc. (9). Third, antibiotic-resistant/antibiotic-subsisting bacteria are especially troubling. These microbes can resist the antibiotic while also protecting sensitive cohorts. That is, the “resistant-subsistent” strains can modify and inactivate therapeutic antibiotics until the concentration drops below the MIC for neighboring microbes sensitive to the antibiotic.In summary, Salmonella spp. are able to subsist on antibiotics as a sole carbon source. The DT104 isolates were more likely to display this phenotype than all of the other isolates. This study provides insight into the ability of a food-borne enteric pathogen to subsist on antibiotics. 相似文献
TABLE 1.
Salmonella isolates that subsisted on SCS agar or in SCS broth containing 1 or more of the 12 antibioticsa| Antibiotic or other carbon sourceb | Serovar(s) or subspecies of isolate(s) in indicated MIC groupc | |
|---|---|---|
| MIC > 1 mg/ml | MIC ≤ 1 mg/ml | |
| Ampicillin or ampicillin-clavulanic acid (63)d | Abortus-equi, Clackamas, Dublin (2), Minnesota, Panama, Typhimurium (52)SGI1 | Newport, Norwich, Nottingham, Ordonez, Worthington |
| Kanamycin (51) | Aqua, Berta, Choleraesuis, Duisburg, Enteriditis, Gatow, Heidelberg, Infantis, Oranienburg, Paratyphi B, Paratyphi B var. L(+) tartrate, Paratyphi C, London var. 15+, Ohio, Typhimurium (36)SGI1, Typhisuis | |
| Sulfisoxazole (38)e | AgonaSGI1, Amager, Clackamas, Derby, Infantis, Montevideo, Typhimurium (30)SGI1, Worthington | TyphimuriumSGI1 |
| Trimethoprim (21)e | Agona, Aqua, Choleraesuis var. Decatur, Heidelberg, Montevideo, Oranienburg, Saint-paul, Typhimurium (14)SGI1 | |
| Vancomycin (11) | Derby, Mbandaka, Schwarzengrund, Sendai, Typhimurium (7)SGI1 | |
| Streptomycin (7) | Typhimurium (7)SGI1 | |
| Ceftiofur (5) | Aqua, Bietri, Durham, Havana, subsp. houtanae | |
| Ciprofloxacin (2) | Kingston | Hartford |
| Amikacin (1) | Typhisuis | |
| Florfenicol (1) | Typhisuis | |
| Cefepime (1) | TyphimuriumSGI1 | |
| Tetracycline (0) | ||
TABLE 2.
Salmonella isolates that subsisted on two or more antibiotics| Antibiotics that enabled subsistence | Serovar(s)a |
|---|---|
| Amikacin and florfenicol | Typhisuis (1) |
| Ampicillin and kanamycin | Typhimurium (7)SGI1 |
| Ampicillin, kanamycin, and streptomycin | Typhimurium (7)SGI1 |
| Ampicillin, kanamycin, and trimethoprim | Typhimurium (5)SGI1 |
| Ampicillin and sulfisoxasole | Typhimurium (5)SGI1, Clackamas (1) |
| Ampicillin and trimethoprim | Typhimurium (2)SGI1 |
| Ceftiofur, kanamycin, and trimethoprim | Aqua (1) |
| Kanamycin and sulfisoxasole | Typhimurium (1)SGI1 |
| Kanamycin and trimethoprim | Typhimurium (2)SGI1, Oranienburg (1) |
| Kanamycin, sulfisoxasole, and trimethoprim | Typhimurium* (1)SGI1 |
| Sulfisoxasole and vancomycin | Typhimurium (6)SGI1 |
11.
Tabu C Breiman RF Ochieng B Aura B Cosmas L Audi A Olack B Bigogo G Ongus JR Fields P Mintz E Burton D Oundo J Feikin DR 《PloS one》2012,7(2):e31237
Background
The epidemiology of non-Typhi Salmonella (NTS) bacteremia in Africa will likely evolve as potential co-factors, such as HIV, malaria, and urbanization, also change.Methods
As part of population-based surveillance among 55,000 persons in malaria-endemic, rural and malaria-nonendemic, urban Kenya from 2006–2009, blood cultures were obtained from patients presenting to referral clinics with fever ≥38.0°C or severe acute respiratory infection. Incidence rates were adjusted based on persons with compatible illnesses, but whose blood was not cultured.Results
NTS accounted for 60/155 (39%) of blood culture isolates in the rural and 7/230 (3%) in the urban sites. The adjusted incidence in the rural site was 568/100,000 person-years, and the urban site was 51/100,000 person-years. In both sites, the incidence was highest in children <5 years old. The NTS-to-typhoid bacteremia ratio in the rural site was 4.6 and in the urban site was 0.05. S. Typhimurium represented >85% of blood NTS isolates in both sites, but only 21% (urban) and 64% (rural) of stool NTS isolates. Overall, 76% of S. Typhimurium blood isolates were multi-drug resistant, most of which had an identical profile in Pulse Field Gel Electrophoresis. In the rural site, the incidence of NTS bacteremia increased during the study period, concomitant with rising malaria prevalence (monthly correlation of malaria positive blood smears and NTS bacteremia cases, Spearman''s correlation, p = 0.018 for children, p = 0.16 adults). In the rural site, 80% of adults with NTS bacteremia were HIV-infected. Six of 7 deaths within 90 days of NTS bacteremia had HIV/AIDS as the primary cause of death assigned on verbal autopsy.Conclusions
NTS caused the majority of bacteremias in rural Kenya, but typhoid predominated in urban Kenya, which most likely reflects differences in malaria endemicity. Control measures for malaria, as well as HIV, will likely decrease the burden of NTS bacteremia in Africa. 相似文献12.
Xiaojian Yang Jennifer Brisbin Hai Yu Qi Wang Fugui Yin Yonggang Zhang Parviz Sabour Shayan Sharif Joshua Gong 《PloS one》2014,9(4)
Background
Probiotics have been used to control Salmonella colonization/infection in chickens. Yet the mechanisms of probiotic effects are not fully understood. This study has characterized our previously-selected lactic acid-producing bacterial (LAB) isolates for controlling Salmonella infection in chickens, particularly the mechanism underlying the control.Methodology/Principal Findings
In vitro studies were conducted to characterize 14 LAB isolates for their tolerance to low pH (2.0) and high bile salt (0.3–1.5%) and susceptibility to antibiotics. Three chicken infection trials were subsequently carried out to evaluate four of the isolates for reducing the burden of Salmonella enterica serovar Typhimurium in the broiler cecum. Chicks were gavaged with LAB cultures (106–7 CFU/chick) or phosphate-buffered saline (PBS) at 1 day of age followed by Salmonella challenge (104 CFU/chick) next day. Samples of cecal digesta, spleen, and liver were examined for Salmonella counts on days 1, 3, or 4 post-challenge. Salmonella in the cecum from Trial 3 was also assessed for the expression of ten virulence genes located in its pathogenicity island-1 (SPI-1). These genes play a role in Salmonella intestinal invasion. Tested LAB isolates (individuals or mixed cultures) were unable to lower Salmonella burden in the chicken cecum, but able to attenuate Salmonella infection in the spleen and liver. The LAB treatments also reduced almost all SPI-1 virulence gene expression (9 out of 10) in the chicken cecum, particularly at the low dose. In vitro treatment with the extracellular culture fluid from a LAB culture also down-regulated most SPI-1 virulence gene expression.Conclusions/Significance
The possible correlation between attenuation of Salmonella infection in the chicken spleen and liver and reduction of Salmonella SPI-1 virulence gene expression in the chicken cecum by LAB isolates is a new observation. Suppression of Salmonella virulence gene expression in vivo can be one of the strategies for controlling Salmonella infection in chickens. 相似文献13.
14.
Lae-seung Jung Tian Ding Juhee Ahn 《Annals of clinical microbiology and antimicrobials》2017,16(1):66
Background
The emergence of antibiotic-resistant bacteria can cause serious clinical and public health problems. This study describes the possibility of using bacteriophages as an alternative agent to control multidrug-resistant Salmonella Typhimurium.Methods
The potential lytic bacteriophages (P22-B1, P22, PBST10, PBST13, PBST32, and PBST 35) were characterized by morphological property, heat and pH stability, optimum multiplicity of infection (MOI), and lytic activity against S. Typhimurium KCCM 40253, S. Typhimurium ATCC 19585, ciprofloxacin-induced antibiotic-resistant S. Typhimurium ATCC 19585, and S. Typhimurium CCARM 8009.Results
P22-B1 and P22 belong to Podoviridae family and PBST10, PBST13, PBST32, and PBST 35 show a typical structure with polyhedral head and long tail, belonging to Siphoviridae family. Salmonella bacteriophages were highly stable at the temperatures (< 60 °C) and pHs (5.0–11.0). The reduction rates of host cells were increased at the MOI-dependent manner, showing the highest reduction rate at MOI of 10. The host cells were most effectively reduced by P22, while P22-B1 showed the least lytic activity. The ciprofloxacin-induced antibiotic-resistant S. Typhimurium ATCC 19585, and clinically isolated antibiotic-resistant S. Typhimurium CCARM 8009 were resistant to ciprofloxacin, levofloxacin, norfloxacin, and tetracycline. P22 showed the highest lytic activity against S. Typhimurium KCCM 40253 (> 5 log reduction), followed by S. Typhimurium ATCC 19585 (4 log reduction) and ciprofloxacin-induced antibiotic-resistant S. Typhimurium ATCC 19585 (4 log reduction).Conclusion
The results would provide vital insights into the application of lytic bacteriophages as an alternative therapeutics for the control of multidrug-resistant pathogens.15.
Park M Lee JH Shin H Kim M Choi J Kang DH Heu S Ryu S 《Applied and environmental microbiology》2012,78(1):58-69
Salmonella enterica and Escherichia coli O157:H7 are major food-borne pathogens causing serious illness. Phage SFP10, which revealed effective infection of both S. enterica and E. coli O157:H7, was isolated and characterized. SFP10 contains a 158-kb double-stranded DNA genome belonging to the Vi01 phage-like family Myoviridae. In vitro adsorption assays showed that the adsorption constant rates to both Salmonella enterica serovar Typhimurium and E. coli O157:H7 were 2.50 × 10−8 ml/min and 1.91 × 10−8 ml/min, respectively. One-step growth analysis revealed that SFP10 has a shorter latent period (25 min) and a larger burst size (>200 PFU) than ordinary Myoviridae phages, suggesting effective host infection and lytic activity. However, differential development of resistance to SFP10 in S. Typhimurium and E. coli O157:H7 was observed; bacteriophage-insensitive mutant (BIM) frequencies of 1.19 × 10−2 CFU/ml for S. Typhimurium and 4.58 × 10−5 CFU/ml for E. coli O157:H7 were found, indicating that SFP10 should be active and stable for control of E. coli O157:H7 with minimal emergence of SFP10-resistant pathogens but may not be for S. Typhimurium. Specific mutation of rfaL in S. Typhimurium and E. coli O157:H7 revealed the O antigen as an SFP10 receptor for both bacteria. Genome sequence analysis of SFP10 and its comparative analysis with homologous Salmonella Vi01 and Shigella phiSboM-AG3 phages revealed that their tail fiber and tail spike genes share low sequence identity, implying that the genes are major host specificity determinants. This is the first report identifying specific infection and inhibition of Salmonella Typhimurium and E. coli O157:H7 by a single bacteriophage. 相似文献
16.
Background
Motility is an important component of Salmonella enterica serovar Typhimurium (ST) pathogenesis allowing the bacteria to move into appropriate niches, across the mucus layer and invade the intestinal epithelium. In vitro, flagellum-associated motility is closely related to the invasive properties of ST. The probiotic yeast Saccharomyces boulardii BIOCODEX (S.b-B) is widely prescribed for the prophylaxis and treatment of diarrheal diseases caused by bacteria or antibiotics. In case of Salmonella infection, S.b-B has been shown to decrease ST invasion of T84 colon cell line. The present study was designed to investigate the impact of S.b-B on ST motility.Methodology/Principal Findings
Experiments were performed on human colonic T84 cells infected by the Salmonella strain 1344 alone or in the presence of S.b-B. The motility of Salmonella was recorded by time-lapse video microscopy. Next, a manual tracking was performed to analyze bacteria dynamics (MTrackJ plugin, NIH image J software). This revealed that the speed of bacterial movement was modified in the presence of S.b-B. The median curvilinear velocity (CLV) of Salmonella incubated alone with T84 decreased from 43.3 µm/sec to 31.2 µm/sec in the presence of S.b-B. Measurement of track linearity (TL) showed similar trends: S.b-B decreased by 15% the number of bacteria with linear tract (LT) and increased by 22% the number of bacteria with rotator tract (RT). Correlation between ST motility and invasion was further established by studying a non-motile flagella-deficient ST strain. Indeed this strain that moved with a CLV of 0.5 µm/sec, presented a majority of RT and a significant decrease in invasion properties. Importantly, we show that S.b-B modified the motility of the pathogenic strain SL1344 and significantly decreased invasion of T84 cells by this strain.Conclusions
This study reveals that S.b-B modifies Salmonella''s motility and trajectory which may account for the modification of Salmonella''s invasion. 相似文献17.
Hanna K. De Jong Ahmed Achouiti Gavin C. K. W. Koh Christopher M. Parry Stephen Baker Mohammed Abul Faiz Jaap T. van Dissel Albert M. Vollaard Ester M. M. van Leeuwen Joris J. T. H. Roelofs Alex F. de Vos Johannes Roth Tom van der Poll Thomas Vogl Willem Joost Wiersinga 《PLoS neglected tropical diseases》2015,9(4)
Background
Typhoid fever, caused by the Gram-negative bacterium Salmonella enterica serovar Typhi, is a major cause of community-acquired bacteremia and death worldwide. S100A8 (MRP8) and S100A9 (MRP14) form bioactive antimicrobial heterodimers (calprotectin) that can activate Toll-like receptor 4, promoting lethal, endotoxin-induced shock and multi-organ failure. We aimed to characterize the expression and function of S100A8/A9 in patients with typhoid fever and in a murine invasive Salmonella model.Methods and principal findings
S100A8/A9 protein levels were determined in acute phase plasma or feces from 28 Bangladeshi patients, and convalescent phase plasma from 60 Indonesian patients with blood culture or PCR-confirmed typhoid fever, and compared to 98 healthy control subjects. To functionally characterize the role of S100A8/A9, we challenged wildtype (WT) and S100A9-/- mice with S. Typhimurium and determined bacterial loads and inflammation 2- and 5- days post infection. We further assessed the antimicrobial function of recombinant S100A8/A9 on S. Typhimurium and S. Typhi replication in vitro. Typhoid fever patients demonstrated a marked increase of S100A8/A9 in acute phase plasma and feces and this increases correlated with duration of fever prior to admission. S100A8/A9 directly inhibited the growth of S. Typhimurium and S. Typhi in vitro in a dose and time dependent fashion. WT mice inoculated with S. Typhimurium showed increased levels of S100A8/A9 in both the liver and the systemic compartment but S100A9-/- mice were indistinguishable from WT mice with respect to bacterial growth, survival, and inflammatory responses, as determined by cytokine release, histopathology and organ injury.Conclusion
S100A8/A9 is markedly elevated in human typhoid, correlates with duration of fever prior to admission and directly inhibits the growth of S. Typhimurium and S. Typhi in vitro. Despite elevated levels in the murine invasive Salmonella model, S100A8/A9 does not contribute to an effective host response against S. Typhimurium in mice. 相似文献18.
Saggers EJ Waspe CR Parker ML Waldron KW Brocklehurst TF 《Journal of applied microbiology》2008,105(5):1239-1245
Aims: The aims of the current study were to explore the site of bacterial attachment to vegetable tissues and to investigate the hypothesis that Salmonella must be living in order to attach to this site(s). Methods and Results: Scanning electron micrographs of intact potato cells showed that Salm. serotype Typhimurium attached to cell-wall junctions; suggesting a high-level of site selectivity. Inactivation of Salm. Typhimurium using heat, ethanol, formalin or Kanamycin resulted in cells that could be no longer attached to these sites. Attachment of a Gfp+ strain of Salm. Typhimurium to cell-wall material (CWM) was examined via flow cytometric analysis. Only live Salm. Typhimurium attached to the CWM. Conclusions: Salmonella serotype Typhimurium must be metabolically active to ensure attachment to vegetable tissues. Attachment preferentially occurs at the plant cell-wall junction and the cell-wall components found here, including pectate, may provide a receptor site for bacterial attachment. Significance and Impact of the Study: Further studies into individual plant cell-wall components may yield the specific bacterial receptor site in vegetable tissues. This information could in turn lead to the development of more targeted and effective decontamination protocols that block this site of attachment. 相似文献
19.
Background
The large serine recombinase phiC31 from broad host range Streptomyces temperate phage, catalyzes the site-specific recombination of two recognition sites that differ in sequence, typically known as attachment sites attB and attP. Previously, we characterized the phiC31 catalytic activity and modes of action in the fission yeast Schizosaccharomyces pombe. 相似文献20.