Phage-Bacterial Interaction Alters Phenotypes Associated with Virulence in Acinetobacter baumannii.

Bacteriophages exert strong selection on their bacterial hosts to evolve resistance. At the same time, the fitness costs on bacteria following phage resistance may change their virulence, which may affect the therapeutic outcomes of phage therapy. In this study, we set out to assess the costs of phage resistance on the in vitro virulence of priority 1 nosocomial pathogenic bacterium, Acinetobacter baumannii. By subjecting phage-resistant variant Ev5-WHG of A. baumannii WHG40004 to several in vitro virulence profiles, we found that its resistance to phage is associated with reduced fitness in host microenvironments. Also, the mutant exhibited impaired adhesion and invasion to mammalian cells, as well as increased susceptibility to macrophage phagocytosis. Furthermore, the whole-genome sequencing of the mutant revealed that there exist multiple mutations which may play a role in phage resistance and altered virulence. Altogether, this study demonstrates that resistance to phage can significantly alter phenotypes associated with virulence in Acinetobacter baumannii.

Exploring a phage-based real-time PCR assay for diagnosing Acinetobacter baumannii bloodstream infections with high sensitivity.

In the present study, we developed a phage-based real-time quantitative PCR (qPCR) methodology for sensitive diagnosis of bloodstream infection (BSI) caused by Acinetobacter baumannii (A. baumannii). An isolated A. baumannii phage p53 was used for Taqman qPCR through detecting phage replication in live A. baumannii cells in serum samples. At the phage concentration of 103 PFU/mL, the sensitive detection of A. baumannii (down to 10 CFU in 100 µL serum) has been obtained within 4 h in spiked serum samples without bacteria isolation and DNA extraction. Subsequent testing of 22 simulated serum samples spiked by different strains has shown that the results from the phage-based Taqman qPCR method have 100% agreement with the spiked concentrations of the bacteria. The assay built in this study, gathering all the advantages for detections of high rapidity, high sensitivity, good specificity, being able to detect only live bacteria not dead bacteria and no DNA extraction or purifications, can be developed to detecting other bacterial pathogens in serum or other complicated samples through switching to other types of phages and realize the rapid and sensitive detection of bacteria in BSI, which would potentially be applied for fast diagnosis in sepsis clinically.

Highly potent antimicrobial modified peptides derived from the Acinetobacter baumannii phage endolysin LysAB2.

The increase in the prevalence of multidrug-resistant Acinetobacter baumannii (MDRAB) strains is a serious public health concern. Antimicrobial peptides (AMPs) are a possible solution to this problem. In this study, we examined whether AMPs could be derived from phage endolysins. We synthesized four AMPs based on an amphipathic helical region in the C-terminus of endolysin LysAB2 encoded by the A. baumannii phage ΦAB2. These peptides showed potent antibacterial activity against A. baumannii (minimum inhibitory concentration, 4-64 µM), including some MDR and colistin-resistant A. baumannii. Of the four peptides, LysAB2 P3, with modifications that increased its net positive charge and decreased its hydrophobicity, showed high antibacterial activity against A. baumannii but little haemolytic and no cytotoxic activity against normal eukaryotic cells. The results of electron microscopy experiments and a fluorescein isothiocyanate staining assay indicated that this peptide killed A. baumannii through membrane permeabilization. Moreover, in a mouse intraperitoneal infection model, at 4 h after the bacterial injection, LysAB2 P3 decreased the bacterial load by 13-fold in ascites and 27-fold in blood. Additionally, LysAB2 P3 rescued sixty percent of mice heavily infected with A. baumannii from lethal bacteremia. Our results confirmed that bacteriophage endolysins are a promising resource for developing effective AMPs.

Development and Use of Personalized Bacteriophage-Based Therapeutic Cocktails To Treat a Patient with a Disseminated Resistant Acinetobacter baumannii Infection.

Widespread antibiotic use in clinical medicine and the livestock industry has contributed to the global spread of multidrug-resistant (MDR) bacterial pathogens, including Acinetobacter baumannii We report on a method used to produce a personalized bacteriophage-based therapeutic treatment for a 68-year-old diabetic patient with necrotizing pancreatitis complicated by an MDR A. baumannii infection. Despite multiple antibiotic courses and efforts at percutaneous drainage of a pancreatic pseudocyst, the patient deteriorated over a 4-month period. In the absence of effective antibiotics, two laboratories identified nine different bacteriophages with lytic activity for an A. baumannii isolate from the patient. Administration of these bacteriophages intravenously and percutaneously into the abscess cavities was associated with reversal of the patient's downward clinical trajectory, clearance of the A. baumannii infection, and a return to health. The outcome of this case suggests that the methods described here for the production of bacteriophage therapeutics could be applied to similar cases and that more concerted efforts to investigate the use of therapeutic bacteriophages for MDR bacterial infections are warranted.

Potential of a lytic bacteriophage to disrupt Acinetobacter baumannii biofilms in vitro.

AIM: The ability of Acinetobacter baumannii to form biofilms and develop antibiotic resistance makes it difficult to control infections caused by this bacterium. In this study, we explored the potential of a lytic bacteriophage to disrupt A. baumannii biofilms. MATERIALS & METHODS: The potential of the lytic bacteriophage to disrupt A. baumannii biofilms was assessed by performing electron microscopy, live/dead bacterial staining, crystal violet staining and by determining adenosine triphosphate release. RESULTS: The bacteriophage inhibited the formation of and disrupted preformed A. baumannii biofilms. Results of disinfection assay showed that the lytic bacteriophage lysed A. baumannii cells suspended in blood or grown on metal surfaces. CONCLUSION: These results suggest the potential of the lytic bacteriophage to disrupt A. baumannii biofilms.

Genotipificación de Acinetobacter baumannii multi-resistente aislado en el hospital Dr. Domingo Luciani de caracas / Genotypification of multiresistant Acinetobacter baumannii isolated in the Dr. Domingo Luciani Hospital of caracas

Las técnicas de genotipificación tienen un rol fundamental en el estudio de las infecciones nosocomiales. Las infecciones nosocomiales son producidas principalmente por microorganismos que son resistentes a los antimicrobianos, que por lo general han sido seleccionados por el uso inadecuado de la terapia antimicrobiana. Entre las especies que causan frecuentemente este tipo de infecciones se encuentra A. baumannii multi-resistente. En esta investigación se planteó genotipificar mediante las técnicas ERIC-PCR y REP-PCR 19 cepas de A. baumannii multi-resistente aisladas en el hospital Dr. Domingo Luciani de Caracas. La confirmación molecular de la especie A. baumannii se realizó mediante la detección de la oxacilinasa OXA 51 por PCR, el 100% de los aislados incluidos en el estudio resultaron positivos para la detección del gen blaOXA-51-Like. La susceptibilidad antimicrobiana y la detección fenotípica de mecanismos de resistencia se efectuaron de acuerdo a las normas de la CLSI 2009. Se determinó policlonalidad en los 19 aislados de A. baumannii, con el predominio de cuatro clones en la Unidad de Terapia Intensiva de Adultos y el área de Hospitalización del Hospital Dr. Domingo Luciani de Caracas. La correlación de los datos epidemiológicos con las características de la resistencia y la información molecular de cada una de las muestras permitió identificar dos patrones de infección: infecciones de origen endógeno, las cuales se caracterizaron por la diversidad genética de los aislamientos, e infecciones cruzadas, debido al hallazgo de cepas estrechamente relacionadas en espacios cercano o distantes del centro de salud. Se demostró que ERIC-PCR y REP-PCR bajo las condiciones estandarizadas en este estudio son técnicas confiables desde el punto de vista de la estabilidad de los marcadores moleculares y la reproducibilidad para caracterizar brotes ocasionados por A. baumannii, considerándose la técnica REP-PCR más adecuada para estudios de genotipificación...

The genotypification techniques have a fundamental role in the study of nosocomial infections. These infections are produced principally by microorganisms that are antimicrobial resistant, that have benn selected by the inadequate use of antimicrobial therapy. Between the species that frequently cause these type of infections is the A baumannii multi-resistant. In this investigation we established to genotypificate by ERIC-PCR y REP-PCR techniques 19 strains of A baumannii multi-resitant isolated in the Dr. Domingo Luciani Hospital of Caracas. The molecular confirmation of the species was realized by the detection of the oxacilianse OXA 51 by PCR. 100% of the isolates included in the study resulted positive for the gen bla OXA-51-Like. The antimocrobial susceptibility and the phenotypic detection of resistance mechanism were done according the CLSI 2009 normative. We determined policlonality on the 19 isolates of A. baumannii, with the predominance of 4 clones in the Intensive Therapy unit and the hospitalization area of the hospital. The correlation of the epidemiological data with the resistance characteristics and the molecular information of each sample allowed us to identificate two patterns of infections: endogen origin infection, which was charaterized by the genetic diversity of the isolates and cross infections, due to the finding of strains closely related in spaces near o distant ffrom the health center. We demostrated that ERIC-PCR and REP-PCR under standarized conditions in this study are good techiques fron the point of view of the stability of the molecular markers and the reproducibility to characterize outbreaks occasioned by A. baumannii, consideratin the REP-PCR technique, the most adequate for genotypification of this strain.