Your search keyword '"De Carolis, Elena"' showing total 7 results

1. Different detection capabilities by mycological media for Candida isolates from mono- or dual-species cultures

Author

De Angelis, Giulia, Menchinelli, Giulia, Torelli, Riccardo, De Carolis, Elena, Posteraro, P., Sanguinetti, Maurizio, Posteraro, Brunella, De Angelis G. (ORCID:0000-0002-7087-7399), Menchinelli G., Torelli R., De Carolis E. (ORCID:0000-0003-4757-7256), Sanguinetti M. (ORCID:0000-0002-9780-7059), Posteraro B. (ORCID:0000-0002-1663-7546), De Angelis, Giulia, Menchinelli, Giulia, Torelli, Riccardo, De Carolis, Elena, Posteraro, P., Sanguinetti, Maurizio, Posteraro, Brunella, De Angelis G. (ORCID:0000-0002-7087-7399), Menchinelli G., Torelli R., De Carolis E. (ORCID:0000-0003-4757-7256), Sanguinetti M. (ORCID:0000-0002-9780-7059), and Posteraro B. (ORCID:0000-0002-1663-7546)

Abstract

The aim of this study was to compare the Candida bromcresol green (BCG) medium with the chromogenic (CHROM) Brilliance Candida agar and Sabouraud dextrose agar (SDA) media in regard to their capability of detecting Candida isolates from mono- or dual-species cultures. We prepared Candida isolates' suspensions to obtain mono-species (n = 18) or dual-species (n = 153) culture plates per each medium, and three readers independently observed 513 plates at 24-h, 48-h and 72-h incubation time. We scored reading results as correct, over or under detection compared to the expected species number(s). BCG showed significantly higher correct-detection and lower under-detection rates for all Candida species when observed by at least one reader. At 24-h reading, 12 mono-species cultures had correct (or over) detections in all media, whereas 106, 60 and 78 dual-species cultures had correct (or over) detections in BCG, CHROM or SDA, respectively. BCG provides the basis for an accurate laboratory diagnosis of Candida infections.

Published

2020

2. A rapid diagnostic workflow for cefotaxime-resistant Escherichia coli and Klebsiella pneumoniae detection from blood cultures by MALDI-TOF mass spectrometry

Author

De Carolis, Elena, Paoletti, Silvia, Nagel, Domenico Rosario, Vella, Antonietta, Mello Dottoressa, Enrica, Palucci, Ivana, De Angelis, Giulia, D'Inzeo, Tiziana, Sanguinetti, Maurizio, Posteraro, Brunella, Spanu, Teresa, De Carolis, Elena (ORCID:0000-0003-4757-7256), Nagel, Domenico, Mello, Enrica, De Angelis, Giulia (ORCID:0000-0002-7087-7399), D’Inzeo, Tiziana (ORCID:0000-0003-1508-3518), Sanguinetti, Maurizio (ORCID:0000-0002-9780-7059), Posteraro, Brunella (ORCID:0000-0002-1663-7546), Spanu, Teresa (ORCID:0000-0003-1864-5184), De Carolis, Elena, Paoletti, Silvia, Nagel, Domenico Rosario, Vella, Antonietta, Mello Dottoressa, Enrica, Palucci, Ivana, De Angelis, Giulia, D'Inzeo, Tiziana, Sanguinetti, Maurizio, Posteraro, Brunella, Spanu, Teresa, De Carolis, Elena (ORCID:0000-0003-4757-7256), Nagel, Domenico, Mello, Enrica, De Angelis, Giulia (ORCID:0000-0002-7087-7399), D’Inzeo, Tiziana (ORCID:0000-0003-1508-3518), Sanguinetti, Maurizio (ORCID:0000-0002-9780-7059), Posteraro, Brunella (ORCID:0000-0002-1663-7546), and Spanu, Teresa (ORCID:0000-0003-1864-5184)

Abstract

Background: Nowadays, the global spread of resistance to oxyimino-cephalosporins in Enterobacteriaceae implies the need for novel diagnostics that can rapidly target resistant organisms from these bacterial species. Methods: In this study, we developed and evaluated a Direct Mass Spectrometry assay for Beta-Lactamase (D-MSBL) that allows direct identification of (oxyimino)cephalosporin-resistant Escherichia coli or Klebsiella pneumoniae from positive blood cultures (BCs), by using the matrix-assisted laser desorption ionization–time of flight mass spectrometry (MALDI-TOF MS) technology. Results: The D-MSBL assay was performed on 93 E. coli or K. pneumoniae growing BC samples that were shortly co-incubated with cefotaxime (CTX) as the indicator cephalosporin. Susceptibility and resistance defining peaks from the samples’ mass spectra were analyzed by a novel algorithm for bacterial organism classification. The D-MSBL assay allowed discrimination between E. coli and K. pneumoniae that were resistant or susceptible to CTX with a sensitivity of 86.8% and a specificity of 98.2%. Conclusion: The proposed algorithm-based D-MSBL assay, if integrated in the routine laboratory diagnostic workflow, may be useful to enhance the establishment of appropriate antibiotic therapy and to control the threat of oxyimino-cephalosporin resistance in hospital.

Published

2017

3. Comparative performance evaluation of Wako β-glucan test and Fungitell assay for the diagnosis of invasive fungal diseases.

Author

De Carolis, Elena, Marchionni, Federica, Torelli, Riccardo, Angela, Morandotti Grazia, Pagano, Livio, Murri, Rita, De Pascale, Gennaro, De Angelis, Giulia, Sanguinetti, Maurizio, and Posteraro, Brunella

Subjects

*MYCOSES, *PNEUMOCYSTIS pneumonia, *BIOMARKERS, *ASPERGILLOSIS

Abstract

The Fungitell assay (FA) and the Wako β-glucan test (GT) are employed to measure the serum/plasma 1,3-β-D-glucan (BDG), a well-known invasive fungal disease biomarker. Data to convincingly and/or sufficiently support the GT as a valuable alternative to the FA are yet limited. In this study, we evaluated the FA and the GT to diagnose invasive aspergillosis (IA), invasive candidiasis (IC), and Pneumocystis jirovecii pneumonia (PJP). The FA and GT performances were compared in sera of patients with IA (n = 40), IC (n = 78), and PJP (n = 17) with respect to sera of control patients (n = 187). Using the manufacturer's cutoff values of 80 pg/mL and 11 pg/mL, the sensitivity and specificity for IA diagnosis were 92.5% and 99.5% for the FA and 60.0% and 99.5% for the GT, respectively; for IC diagnosis were 100.0% and 97.3% for the FA and 91.0% and 99.5% for the GT, respectively; for PJP diagnosis were 100.0% and 97.3% for the FA and 88.2% and 99.5% for the GT, respectively. When an optimized cutoff value of 7.0 pg/mL for the GT was used, the sensitivity and specificity were 80.0% and 97.3% for IA diagnosis, 98.7% and 97.3% for IC diagnosis, and 94.1% and 97.3% for PJP diagnosis, respectively. At the 7.0-pg/mL GT cutoff, the agreement between the assays remained and/or became excellent for IA (95.1%), IC (97.3%), and PJP (96.5%), respectively. In conclusion, we show that the GT performed as well as the FA only with a lowered cutoff value for positivity. Further studies are expected to establish the equivalence of the two BDG assays. [ABSTRACT FROM AUTHOR]

Published

2020

4. A New Piece of the Shigella Pathogenicity Puzzle: Spermidine Accumulationby Silencing of the speG Gene.

Author

Barbagallo, Marialuisa, Di Martino, Maria Letizia, Marcocci, Lucia, Pietrangeli, Paola, De Carolis, Elena, Casalino, Mariassunta, Colonna, Bianca, and Prosseda, Gianni

Subjects

SHIGELLA, FOOD pathogens, ESCHERICHIA coli, SPERMIDINE, BIOGENIC amines

Abstract

The genome of Shigella, a gram negative bacterium which is the causative agent of bacillary dysentery, shares strong homologies with that of its commensal ancestor, Escherichia coli. The acquisition, by lateral gene transfer, of a large plasmid carrying virulence determinants has been a crucial event in the evolution towards the pathogenic lifestyle and has been paralleled by the occurrence of mutations affecting genes, which negatively interfere with the expression of virulence factors. In this context, we have analysed to what extent the presence of the plasmid-encoded virF gene, the major activator of the Shigella regulon for invasive phenotype, has modified the transcriptional profile of E. coli. Combining results from transcriptome assays and comparative genome analyses we show that in E. coli VirF, besides being able to up-regulate several chromosomal genes, which potentially influence bacterial fitness within the host, also activates genes which have been lost by Shigella. We have focused our attention on the speG gene, which encodes spermidine acetyltransferase, an enzyme catalysing the conversion of spermidine into the physiologically inert acetylspermidine, since recent evidence stresses the involvement of polyamines in microbial pathogenesis. Through identification of diverse mutations, which prevent expression of a functional SpeG protein, we show that the speG gene has been silenced by convergent evolution and that its inactivation causes the marked increase of intracellular spermidine in all Shigella spp. This enhances the survival of Shigella under oxidative stress and allows it to better face the adverse conditions it encounters inside macrophage. This is supported by the outcome of infection assays performed in mouse peritoneal macrophages and of a competitive-infection assay on J774 macrophage cell culture. Our observations fully support the pathoadaptive nature of speG inactivation in Shigella and reveal that the accumulation of spermidine is a key determinant in the pathogenicity strategy adopted by this microrganism. [ABSTRACT FROM AUTHOR]

Published

2011

5. Different detection capabilities by mycological media for Candida isolates from mono- or dual-species cultures.

Author

De Angelis G, Menchinelli G, Torelli R, De Carolis E, Posteraro P, Sanguinetti M, and Posteraro B

Subjects

Candidiasis microbiology, Humans, Microbiological Techniques methods, Agar chemistry, Candida isolation & purification, Candidiasis diagnosis, Culture Media chemistry, Indicators and Reagents chemistry

Abstract

The aim of this study was to compare the Candida bromcresol green (BCG) medium with the chromogenic (CHROM) Brilliance Candida agar and Sabouraud dextrose agar (SDA) media in regard to their capability of detecting Candida isolates from mono- or dual-species cultures. We prepared Candida isolates' suspensions to obtain mono-species (n = 18) or dual-species (n = 153) culture plates per each medium, and three readers independently observed 513 plates at 24-h, 48-h and 72-h incubation time. We scored reading results as correct, over or under detection compared to the expected species number(s). BCG showed significantly higher correct-detection and lower under-detection rates for all Candida species when observed by at least one reader. At 24-h reading, 12 mono-species cultures had correct (or over) detections in all media, whereas 106, 60 and 78 dual-species cultures had correct (or over) detections in BCG, CHROM or SDA, respectively. BCG provides the basis for an accurate laboratory diagnosis of Candida infections., Competing Interests: The authors have declared that no competing interests exist.

Published

2020

6. A rapid diagnostic workflow for cefotaxime-resistant Escherichia coli and Klebsiella pneumoniae detection from blood cultures by MALDI-TOF mass spectrometry.

Author

De Carolis E, Paoletti S, Nagel D, Vella A, Mello E, Palucci I, De Angelis G, D'Inzeo T, Sanguinetti M, Posteraro B, and Spanu T

Subjects

Drug Resistance, Bacterial, Humans, Anti-Bacterial Agents pharmacology, Cefotaxime pharmacology, Escherichia coli drug effects, Klebsiella pneumoniae drug effects, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods

Abstract

Background: Nowadays, the global spread of resistance to oxyimino-cephalosporins in Enterobacteriaceae implies the need for novel diagnostics that can rapidly target resistant organisms from these bacterial species., Methods: In this study, we developed and evaluated a Direct Mass Spectrometry assay for Beta-Lactamase (D-MSBL) that allows direct identification of (oxyimino)cephalosporin-resistant Escherichia coli or Klebsiella pneumoniae from positive blood cultures (BCs), by using the matrix-assisted laser desorption ionization-time of flight mass spectrometry (MALDI-TOF MS) technology., Results: The D-MSBL assay was performed on 93 E. coli or K. pneumoniae growing BC samples that were shortly co-incubated with cefotaxime (CTX) as the indicator cephalosporin. Susceptibility and resistance defining peaks from the samples' mass spectra were analyzed by a novel algorithm for bacterial organism classification. The D-MSBL assay allowed discrimination between E. coli and K. pneumoniae that were resistant or susceptible to CTX with a sensitivity of 86.8% and a specificity of 98.2%., Conclusion: The proposed algorithm-based D-MSBL assay, if integrated in the routine laboratory diagnostic workflow, may be useful to enhance the establishment of appropriate antibiotic therapy and to control the threat of oxyimino-cephalosporin resistance in hospital.

Published

2017

7. A new piece of the Shigella Pathogenicity puzzle: spermidine accumulation by silencing of the speG gene [corrected].

Author

Barbagallo M, Di Martino ML, Marcocci L, Pietrangeli P, De Carolis E, Casalino M, Colonna B, and Prosseda G

Subjects

Animals, Bacterial Proteins genetics, Bacterial Proteins metabolism, Cell Survival, Cells, Cultured, Dysentery, Bacillary microbiology, Escherichia coli genetics, Escherichia coli pathogenicity, Macrophages, Peritoneal metabolism, Male, Mice, Mice, Inbred BALB C, Oxidative Stress, Plasmids genetics, RNA, Messenger genetics, Real-Time Polymerase Chain Reaction, Regulon, Shigella flexneri genetics, Transcriptome, Virulence Factors genetics, Bacterial Proteins antagonists & inhibitors, Dysentery, Bacillary genetics, Gene Silencing, Shigella flexneri pathogenicity, Spermidine metabolism

Abstract

The genome of Shigella, a gram negative bacterium which is the causative agent of bacillary dysentery, shares strong homologies with that of its commensal ancestor, Escherichia coli. The acquisition, by lateral gene transfer, of a large plasmid carrying virulence determinants has been a crucial event in the evolution towards the pathogenic lifestyle and has been paralleled by the occurrence of mutations affecting genes, which negatively interfere with the expression of virulence factors. In this context, we have analysed to what extent the presence of the plasmid-encoded virF gene, the major activator of the Shigella regulon for invasive phenotype, has modified the transcriptional profile of E. coli. Combining results from transcriptome assays and comparative genome analyses we show that in E. coli VirF, besides being able to up-regulate several chromosomal genes, which potentially influence bacterial fitness within the host, also activates genes which have been lost by Shigella. We have focused our attention on the speG gene, which encodes spermidine acetyltransferase, an enzyme catalysing the conversion of spermidine into the physiologically inert acetylspermidine, since recent evidence stresses the involvement of polyamines in microbial pathogenesis. Through identification of diverse mutations, which prevent expression of a functional SpeG protein, we show that the speG gene has been silenced by convergent evolution and that its inactivation causes the marked increase of intracellular spermidine in all Shigella spp. This enhances the survival of Shigella under oxidative stress and allows it to better face the adverse conditions it encounters inside macrophage. This is supported by the outcome of infection assays performed in mouse peritoneal macrophages and of a competitive-infection assay on J774 macrophage cell culture. Our observations fully support the pathoadaptive nature of speG inactivation in Shigella and reveal that the accumulation of spermidine is a key determinant in the pathogenicity strategy adopted by this microrganism.

Published

2011