Your search keyword '"Antypas H"' showing total 14 results

1. Assistive technology for older persons – analyses of data from WHO's rapid assistive technology assessment

Author

Eide, A. H., primary, Müller, S., additional, Khasnabis, C., additional, Borg, J., additional, Blakstad, M., additional, Mannan Antypas, H., additional, Loeb, K. M., additional, and Zhang, W., additional

Published

2022

2. Reducing background cytokine expression in epithelial cells without serum starvation

Author

Antypas, H., Libberton, B., and Melican, K.

Published

2014

3. A universal platform for selection and high-resolution phenotypic screening of bacterial mutants using the nanowell slide

Author

Antypas, H., Veses-Garcia, M., Weibull, Emelie, Svahn Andersson, Helene, Richter-Dahlfors, A., Antypas, H., Veses-Garcia, M., Weibull, Emelie, Svahn Andersson, Helene, and Richter-Dahlfors, A.

Abstract

The Petri dish and microtiter plate are the golden standard for selection and screening of bacteria in microbiological research. To improve on the limited resolution and throughput of these methods, we developed a universal, user-friendly platform for selection and high-resolution phenotypic screening based on the nanowell slide. This miniaturized platform has an optimal ratio between throughput and assay complexity, holding 672 nanowells of 500 nl each. As monoclonality is essential in bacterial genetics, we used FACS to inoculate each nanowell with a single bacterium in 15 min. We further extended the protocol to select and sort only bacteria of interest from a mixed culture. We demonstrated this by isolating single transposon mutants generated by a custom-made transposon with dual selection for GFP fluorescence and kanamycin resistance. Optical compatibility of the nanowell slide enabled phenotypic screening of sorted mutants by spectrophotometric recording during incubation. By processing the absorbance data with our custom algorithm, a phenotypic screen for growth-associated mutations was performed. Alternatively, by processing fluorescence data, we detected metabolism-associated mutations, exemplified by a screen for -galactosidase activity. Besides spectrophotometry, optical compatibility enabled us to perform microscopic analysis directly in the nanowells to screen for mutants with altered morphologies. Despite the miniaturized format, easy transition from nano- to macroscale cultures allowed retrieval of bacterial mutants for downstream genetic analysis, demonstrated here by a cloning-free single-primer PCR protocol. Taken together, our FACS-linked nanowell slide replaces manual selection of mutants on agar plates, and enables combined selection and phenotypic screening in a one-step process. The versatility of the nanowell slide, and the modular workflow built on mainstream technologies, makes our universal platform widely applicable in microbiological res, QC 20180824

Published

2018

4. A universal platform for selection and high-resolution phenotypic screening of bacterial mutants using the nanowell slide

Author

Antypas, H., primary, Veses-Garcia, M., additional, Weibull, E., additional, Andersson-Svahn, H., additional, and Richter-Dahlfors, A., additional

Published

2018

5. Dynamic single cell analysis in a proximal-tubule-on-chip reveals heterogeneous epithelial colonization strategies of uropathogenic Escherichia coli under shear stress.

Author

Antypas H, Zhang T, Choong FX, Melican K, and Richter-Dahlfors A

Abstract

The urinary tract is a hydrodynamically challenging microenvironment and uropathogenic Escherichia coli (UPEC) must overcome several physiological challenges in order to adhere and establish a urinary tract infection. Our previous work in vivo revealed a synergy between different UPEC adhesion organelles, which facilitated effective colonization of the renal proximal tubule. To allow high-resolution real-time analysis of this colonization behavior, we established a biomimetic proximal-tubule-on-chip (PToC). The PToC allowed for single-cell resolution analysis of the first stages of bacterial interaction with host epithelial cells, under physiological flow. Time-lapse microscopy and single-cell trajectory analysis in the PToC revealed that while the majority of UPEC moved directly through the system, a minority population initiated heterogeneous adhesion, identified as either rolling or bound. Adhesion was predominantly transient and mediated by P pili at the earliest time-points. These bound bacteria initiated a founder population which rapidly divided, leading to 3D microcolonies. Within the first hours, the microcolonies did not express extracellular curli matrix, but rather were dependent on Type 1 fimbriae as the key element in the microcolony structure. Collectively, our results show the application of Organ-on-chip technology to address bacterial adhesion behaviors, demonstrating a well-orchestrated interplay and redundancy between adhesion organelles that enables UPEC to form microcolonies and persist under physiological shear stress., Competing Interests: T.Z. and K.M. declare no competing interests. H.A., F.X.C., and A.R.D. are coinventors of patents relevant to this work. Intellectual properties are owned by Richter Life Science Development AB, founded by A.R.D. F.X.C. and A.R.D. have engagement in Ebba Biotech AB, which commercializes optotracers for uses as described in this article., (© The Author(s) 2023. Published by Oxford University Press on behalf of FEMS.)

Published

2023

6. Mitoxantrone targets both host and bacteria to overcome vancomycin resistance in Enterococcus faecalis .

Author

da Silva RAG, Wong JJ, Antypas H, Choo PY, Goh K, Jolly S, Liang C, Tay Kwan Sing L, Veleba M, Hu G, Chen J, and Kline KA

Subjects

Animals, Mice, Vancomycin Resistance genetics, Vancomycin pharmacology, Mitoxantrone pharmacology, Anti-Bacterial Agents pharmacology, Enterococcus faecalis genetics, Vancomycin-Resistant Enterococci genetics

Abstract

Antibiotic resistance critically limits treatment options for infection caused by opportunistic pathogens such as enterococci. Here, we investigate the antibiotic and immunological activity of the anticancer agent mitoxantrone (MTX) in vitro and in vivo against vancomycin-resistant Enterococcus faecalis (VRE). We show that, in vitro, MTX is a potent antibiotic against Gram-positive bacteria through induction of reactive oxygen species and DNA damage. MTX also synergizes with vancomycin against VRE, rendering the resistant strains more permeable to MTX. In a murine wound infection model, single-dose MTX treatment effectively reduces VRE numbers, with further reduction when combined with vancomycin. Multiple MTX treatments accelerate wound closure. MTX also promotes macrophage recruitment and proinflammatory cytokine induction at the wound site and augments intracellular bacterial killing in macrophages by up-regulating the expression of lysosomal enzymes. These results show that MTX represents a promising bacterium- and host-targeted therapeutic for overcoming vancomycin resistance.

Published

2023

7. UPEC kidney infection triggers neuro-immune communication leading to modulation of local renal inflammation by splenic IFNγ.

Author

Steiner SE, Choong FX, Antypas H, Morado-Urbina CE, Schulz A, Bersellini Farinotti A, Bas DB, Svensson CI, Richter-Dahlfors A, and Melican K

Subjects

Animals, Epithelial Cells microbiology, Inflammation etiology, Inflammation metabolism, Male, Rats, Rats, Sprague-Dawley, Uropathogenic Escherichia coli physiology, Escherichia coli Infections complications, Host-Pathogen Interactions, Inflammation pathology, Interferon-gamma metabolism, Kidney microbiology, Neuroimmunomodulation, Spleen metabolism

Abstract

Bacterial infection results in a veritable cascade of host responses, both local and systemic. To study the initial stages of host-pathogen interaction in living tissue we use spatially-temporally controlled in vivo models. Using this approach, we show here that within 4 h of a uropathogenic Escherichia coli (UPEC) infection in the kidney, an IFNγ response is triggered in the spleen. This rapid infection-mediated inter-organ communication was found to be transmitted via nerve signalling. Bacterial expression of the toxin α-hemolysin directly and indirectly activated sensory neurons, which were identified in the basement membrane of renal tubules. Nerve activation was transmitted via the splenic nerve, inducing upregulation of IFNγ in the marginal zones of the spleen that led to increasing concentrations of IFNγ in the circulation. We found that IFNγ modulated the inflammatory signalling generated by renal epithelia cells in response to UPEC infection. This demonstrates a new concept in the host response to kidney infection; the role of nerves in sensing infection and rapidly triggering a systemic response which can modulate inflammation at the site of infection. The interplay between the nervous and immune systems is an exciting, developing field with the appealing prospect of non-pharmaceutical interventions. Our study identifies an important role for systemic neuro-immune communication in modulating inflammation during the very first hours of a local bacterial infection in vivo., Competing Interests: The authors have declared that no competing interests exist.

Published

2021

8. Overcoming the challenge of establishing biofilms in vivo: a roadmap for Enterococci.

Author

Tan CAZ, Antypas H, and Kline KA

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Enterococcus faecalis genetics, Quorum Sensing, Biofilms, Enterococcus faecalis physiology

Abstract

Enterococcus faecalis forms single and mixed-species biofilms on both tissue and medical devices in the host, often under exposure to fluid flow, giving rise to infections that are recalcitrant to treatment. The factors that drive enterococcal biofilm formation in the host, however, remain unclear. Recent reports in other pathogens show how surface sensing by bacteria can trigger the transition from planktonic to sessile lifestyle. Fluid flow can enhance initial adhesion, but also influence quorum sensing. Biofilm-specific factors, as well as biofilm size and extracellular polymeric substances, can compromise opsonization and phagocytosis. Bacterial interspecies synergy can create favorable conditions in the host for biofilm formation. Through these concepts, we define the knowledge gaps in understanding host-associated E. faecalis biofilm formation and propose a roadmap for future investigations., (Copyright © 2020 Elsevier Ltd. All rights reserved.)

Published

2020

9. Conjugated Oligo- and Polymers for Bacterial Sensing.

Author

Löffler S, Antypas H, Choong FX, Nilsson KPR, and Richter-Dahlfors A

Abstract

Fast and accurate detection of bacteria and differentiation between pathogenic and commensal colonization are important keys in preventing the emergence and spread of bacterial resistance toward antibiotics. As bacteria undergo major lifestyle changes during colonization, bacterial sensing needs to be achieved on different levels. In this review, we describe how conjugated oligo- and polymers are used to detect bacterial colonization. We summarize how oligothiophene derivatives have been tailor-made for detection of biopolymers produced by a wide range of bacteria upon entering the biofilm lifestyle. We further describe how these findings are translated into diagnostic approaches for biofilm-related infections. Collectively, this provides an overview on how synthetic biorecognition elements can be used to produce fast and easy diagnostic tools and new methods for infection control.

Published

2019

10. Protective vascular coagulation in response to bacterial infection of the kidney is regulated by bacterial lipid A and host CD147.

Author

Schulz A, Chuquimia OD, Antypas H, Steiner SE, Sandoval RM, Tanner GA, Molitoris BA, Richter-Dahlfors A, and Melican K

Subjects

Animals, Biomarkers, Cell Line, Cytokines metabolism, Disease Models, Animal, Epithelial Cells metabolism, Epithelial Cells microbiology, Humans, Inflammation Mediators metabolism, Male, Proteome, Proteomics methods, Rats, Signal Transduction, Bacterial Infections blood, Bacterial Infections immunology, Bacterial Infections metabolism, Basigin metabolism, Blood Coagulation, Lipid A immunology, Nephritis etiology, Nephritis metabolism

Abstract

Bacterial infection of the kidney leads to a rapid cascade of host protective responses, many of which are still poorly understood. We have previously shown that following kidney infection with uropathogenic Escherichia coli (UPEC), vascular coagulation is quickly initiated in local perivascular capillaries that protects the host from progressing from a local infection to systemic sepsis. The signaling mechanisms behind this response have not however been described. In this study, we use a number of in vitro and in vivo techniques, including intravital microscopy, to identify two previously unrecognized components influencing this protective coagulation response. The acylation state of the Lipid A of UPEC lipopolysaccharide (LPS) is shown to alter the kinetics of local coagulation onset in vivo. We also identify epithelial CD147 as a potential host factor influencing infection-mediated coagulation. CD147 is expressed by renal proximal epithelial cells infected with UPEC, contingent to bacterial expression of the α-hemolysin toxin. The epithelial CD147 subsequently can activate tissue factor on endothelial cells, a primary step in the coagulation cascade. This study emphasizes the rapid, multifaceted response of the kidney tissue to bacterial infection and the interplay between host and pathogen during the early hours of renal infection.

Published

2018

11. Rapid diagnostic assay for detection of cellulose in urine as biomarker for biofilm-related urinary tract infections.

Author

Antypas H, Choong FX, Libberton B, Brauner A, and Richter-Dahlfors A

Abstract

The ability of uropathogenic Escherichia coli (UPEC) to adopt a biofilm lifestyle in the urinary tract is suggested as one cause of recurrent urinary tract infections (UTIs). A clinical role of UPEC biofilm is further supported by the presence of bacterial aggregates in urine of UTI patients. Yet, no diagnostics exist to differentiate between the planktonic and biofilm lifestyle of bacteria. Here, we developed a rapid diagnostic assay for biofilm-related UTI, based on the detection of cellulose in urine. Cellulose, a component of biofilm extracellular matrix, is detected by a luminescent-conjugated oligothiophene, which emits a conformation-dependent fluorescence spectrum when bound to a target molecule. We first defined the cellulose-specific spectral signature in the extracellular matrix of UPEC biofilm colonies, and used these settings to detect cellulose in urine. To translate this optotracing assay for clinical use, we composed a workflow that enabled rapid isolation of urine sediment and screening for the presence of UPEC-derived cellulose in <45 min. Using multivariate analysis, we analyzed spectral information obtained between 464 and 508 nm by optotracing of urine from 182 UTI patients and 8 healthy volunteers. Cellulose was detected in 14.8% of UTI urine samples. Using cellulose as a biomarker for biofilm-related UTI, our data provide direct evidence that UPEC forms biofilm in the urinary tract. Clinical implementation of this rapid, non-invasive and user-friendly optotracing diagnostic assay will potentially aid clinicians in the design of effective antibiotic treatment., Competing Interests: H.A., F.X.C., B.L., and A.R.-D are co-inventors of patents relevant to this work. Intellectual properties are owned by Richter Life Science Development AB, founded by A.R.-D. F.X.C., and B.L. are shareholders of Furcifer AB. A.B. declares no competing interests.

Published

2018

12. Rapid Phenotypic Antibiotic Susceptibility Testing of Uropathogens Using Optical Signal Analysis on the Nanowell Slide.

Author

Veses-Garcia M, Antypas H, Löffler S, Brauner A, Andersson-Svahn H, and Richter-Dahlfors A

Abstract

Achieving fast antimicrobial susceptibility results is a primary goal in the fight against antimicrobial resistance. Standard antibiotic susceptibility testing (AST) takes, however, at least a day from patient sample to susceptibility profile. Here, we developed and clinically validated a rapid phenotypic AST based on a miniaturized nanotiter plate, the nanowell slide, that holds 672 wells in a 500 nl format for bacterial cultivation. The multitude of nanowells allows multiplexing with a panel of six antibiotics relevant for urinary tract infections. Inclusion of seven concentrations per antibiotic plus technical replicates enabled us to determine a precise minimum inhibitory concentration for 70 clinical uropathogenic Escherichia coli isolates. By combining optical recordings of bacterial growth with an algorithm for optical signal analysis, we calculated T lag , the point of transition from lag to exponential phase, in each nanoculture. Algorithm-assisted analysis determined antibiotic susceptibility as early as 3 h 40 min. In comparison to standard disk diffusion assays, the nanowell AST showed a total categorical agreement of 97.9% with 2.6% major errors and 0% very major errors for all isolate-antibiotic combination tested. Taking advantage of the optical compatibility of the nanowell slide, we performed microscopy to illustrate its potential in defining susceptibility profiles based on bacterial morphotyping. The excellent clinical performance of the nanowell AST, combined with a short detection time, morphotyping, and the very low consumption of reagents clearly show the advantage of this phenotypic AST as a diagnostic tool in a clinical setting.

Published

2018

13. Integrated Pathophysiology of Pyelonephritis.

Author

Choong FX, Antypas H, and Richter-Dahlfors A

Subjects

Animals, Disease Models, Animal, Humans, Urogenital System microbiology, Urogenital System pathology, Host-Pathogen Interactions, Pyelonephritis microbiology, Pyelonephritis physiopathology, Urinary Tract Infections complications

Abstract

Pyelonephritis represents a subset of urinary tract infections that occur from bacteria ascending from the lower to the upper reaches of the genitourinary system, such as the kidney. The renal system contains a range of hydrodynamically and immunologically challenging, interconnected microenvironments where the invading pathogen may populate during the course of the infection. The situation at the infection foci changes dynamically, vacillating between bacterial colonization and clearance, to which the outcome is a summation of all host-pathogen elements in play. A selection of important determinants includes factors of microbial origin, effects of eukaryotic cell signaling, physiological facets of the infected organ, and signals from distal organs. Improved understanding of the multifactorial aspects of molecular pathogenesis of infection requires intravital, cross-disciplinary approaches with high spatio-temporal resolution. The advancement of such approaches promises to eventually provide a comprehensive understanding of the integrated pathophysiology of pyelonephritis.

Published

2015

14. Bacterial nanoscale cultures for phenotypic multiplexed antibiotic susceptibility testing.

Author

Weibull E, Antypas H, Kjäll P, Brauner A, Andersson-Svahn H, and Richter-Dahlfors A

Subjects

Humans, Nanotechnology instrumentation, Nanotechnology methods, Time Factors, Anti-Bacterial Agents pharmacology, High-Throughput Screening Assays instrumentation, High-Throughput Screening Assays methods, Microbial Sensitivity Tests instrumentation, Microbial Sensitivity Tests methods, Uropathogenic Escherichia coli drug effects

Abstract

An optimal antimicrobial drug regimen is the key to successful clinical outcomes of bacterial infections. To direct the choice of antibiotic, access to fast and precise antibiotic susceptibility profiling of the infecting bacteria is critical. We have developed a high-throughput nanowell antibiotic susceptibility testing (AST) device for direct, multiplexed analysis. By processing in real time the optical recordings of nanoscale cultures of reference and clinical uropathogenic Escherichia coli strains with a mathematical algorithm, the time point when growth shifts from lag phase to early logarithmic phase (Tlag) was identified for each of the several hundreds of cultures tested. Based on Tlag, the MIC could be defined within 4 h. Heatmap presentation of data from this high-throughput analysis allowed multiple resistance patterns to be differentiated at a glance. With a possibility to enhance multiplexing capacity, this device serves as a high-throughput diagnostic tool that rapidly aids clinicians in prescribing the optimal antibiotic therapy., (Copyright © 2014, American Society for Microbiology. All Rights Reserved.)

Published

2014