Showing total 22,678 results

1. Enhancing antibacterial characteristics of paper through silver-exchanged zeolite coating for packaging paper

Author

Wanitpinyo, Kapphapaphim, Nanta, Kawinthida, Chitbanyong, Korawit, Pisutpiched, Sawitree, Khantayanuwong, Somwang, Yimlamai, Piyawan, Sukyai, Prakit, and Puangsin, Buapan

Published

2024

2. Genetically engineered bacterial biofilm materials enhances portable whole cell sensing.

Author

Köksaldı İÇ, Avcı E, Köse S, Özkul G, Kehribar EŞ, and Şafak Şeker UÖ

Subjects

Genetic Engineering, Paper, Environmental Monitoring instrumentation, Biosensing Techniques instrumentation, Biosensing Techniques methods, Biofilms, Escherichia coli isolation & purification, Copper chemistry, Escherichia coli Proteins genetics, Escherichia coli Proteins chemistry

Abstract

In recent years, whole-cell biosensors (WCBs) have emerged as a potent approach for environmental monitoring and on-site analyte detection. These biosensors harness the biological apparatus of microorganisms to identify specific analytes, offering advantages in sensitivity, specificity, and real-time monitoring capabilities. A critical hurdle in biosensor development lies in ensuring the robust attachment of cells to surfaces, a crucial step for practical utility. In this study, we present a comprehensive approach to tackle this challenge via engineering Escherichia coli cells for immobilization on paper through the Curli biofilm pathway. Furthermore, incorporating a cellulose-binding peptide domain to the CsgA biofilm protein enhances cell adhesion to paper surfaces, consequently boosting biosensor efficacy. To demonstrate the versatility of this platform, we developed a WCB for copper, optimized to exhibit a discernible response, even with the naked eye. To confirm its suitability for practical field use, we characterized our copper sensor under various environmental conditions-temperature, salinity, and pH-to mimic real-world scenarios. The biosensor-equipped paper discs can be freeze-dried for deployment in on-site applications, providing a practical method for long-term storage without loss of sensitivity paper discs demonstrate sustained functionality and viability even after months of storage with 5 μM limit of detection for copper with visible-to-naked-eye signal levels. Biofilm-mediated surface attachment and analyte sensing can be independently engineered, allowing for flexible utilization of this platform as required. With the implementation of copper sensing as a proof-of-concept study, we underscore the potential of WCBs as a promising avenue for the on-site detection of a multitude of analytes., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: Urartu Ozgur Safak Seker reports financial support was provided by "The Scientific and Technological Research Council of Turkey". If there are other authors, they declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

3. Nano-lantern on paper for smartphone-based ATP detection.

Author

Calabretta MM, Álvarez-Diduk R, Michelini E, Roda A, and Merkoçi A

Subjects

Equipment Design, Humans, Limit of Detection, Luminescent Measurements instrumentation, Smartphone instrumentation, Urinary Tract Infections diagnosis, Adenosine Triphosphate analysis, Biosensing Techniques instrumentation, Escherichia coli isolation & purification, Paper, Urinary Tract Infections urine

Abstract

ATP-driven bioluminescence relying on the D-luciferin-luciferase reaction is widely employed for several biosensing applications where bacterial ATP detection allows to verify microbial contamination for hygiene monitoring in hospitals, food processing and in general for cell viability studies. Several ATP kit assays are already commercially available but an user-friendly ATP biosensor characterized by low-cost, portability, and adequate sensitivity would be highly valuable for rapid and facile on site screening. Thanks to an innovative freeze-drying procedure, we developed a user-friendly, ready-to-use and stable ATP sensing paper biosensor that can be combined with smartphone detection. The ATP sensing paper includes a lyophilized "nano-lantern" with reaction components being rapidly reconstituted by 10 μL sample addition, enabling detection of 10 -14  mol of ATP within 10 min. We analysed urinary microbial ATP as a biomarker of urinary tract infection (UTI), confirming the capability of the ATP sensing paper to detect the threshold for positivity corresponding to 10 5  colony-forming units of bacteria per mL of urine., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2020

4. Combining the geometry of folded paper with liquid-infused polymer surfaces to concentrate and localize bacterial solutions.

Author

Regan DP, Lilly C, Weigang A, White LR, LeClair EJ, Collins A, and Howell C

Subjects

Bacterial Adhesion, Bacteriological Techniques methods, Escherichia coli isolation & purification, Paper, Polymers chemistry, Staphylococcus aureus isolation & purification, Surface Properties, Suspensions

Abstract

Point-of-care (POC) detection and diagnostic platforms provide critical information about health and safety conditions in austere and resource-limited settings in which medical, military, and disaster relief operations are conducted. In this work, low-cost paper materials commonly used in POC devices are coated with liquid-infused polymer surfaces and folded to produce geometries that precisely localize complex liquid samples undergoing concentration by evaporation. Liquid-infused polymer surfaces were fabricated by infusing silicone-coated paper with a chemically compatible polydimethylsiloxane oil to create a liquid overlayer. Tests on these surfaces showed no remaining bacterial cells after exposure to a sliding droplet containing a concentrated solution of Escherichia coli or Staphylococcus aureus, while samples without a liquid layer showed adhesion of both microdroplets and individual bacterial cells. Folding of the paper substrates with liquid-infused polymer surfaces into several functional 3D geometries enabled a clean separation and simultaneous concentration of a liquid containing rhodamine dye into discrete, predefined locations. When used with bacteria, which are known for their ability to adhere to nearly any surface type, functional geometries with liquid-infused polymer surfaces concentrated the cells at levels significantly higher than geometries with dry control surfaces. These results show the potential of synergistically combining paper-based materials with liquid-infused polymer surfaces for the manipulation and handling of complex samples, which may help the future engineering of POC devices.

Published

2019

5. Multifunctional Paper-Based Analytical Device for In Situ Cultivation and Screening of Escherichia coli Infections.

Author

Noiphung J and Laiwattanapaisal W

Subjects

Escherichia coli growth & development, Escherichia coli Infections microbiology, Microscopy, Electron, Scanning, Nitrites analysis, Nitrites chemistry, Point-of-Care Testing, Colorimetry methods, Escherichia coli isolation & purification, Escherichia coli Infections diagnosis, Paper

Abstract

Point-of-care testing (POCT) for uropathogen detection and chemical screening has great benefits for the diagnosis of urinary tract infections (UTIs). The goal of this study was to develop a portable and inexpensive paper-based analytical device (PAD) for cultivating bacteria in situ and rapidly testing for nitrite on the same device. The PAD was fabricated using a wax printing technique to create a pattern on Whatman No. 1 filter paper, which was then combined with a cotton sheet to support bacterial growth. Nitrite detection was based on the principle of the Griess reaction, and a linear detection range of 0-1.6 mg/dL (R 2  = 0.989) was obtained. Scanning electron microscopy (SEM) analysis demonstrated that the bacteria were able to grow and formed a cluster on the cellulose fibres within 2 hours. The enzyme β-glucuronidase, which is specifically produced by Escherichia coli, was able to convert the pre-immobilized 5-bromo-4-chloro-3-indolyl-β-D-glucuronide sodium salt (X-GlcA), a colourless substrate, generating a blue colour. Under optimum conditions, the proposed device allowed bacterial concentrations in the range of 10 4 -10 7 colony forming units (CFU)/mL to be quantified within 6 hours. Moreover, the use of this device enables the identification of E. coli pathogens with selectivity in real urine samples. In conclusion, the PAD developed in this study for UTI screening provides a rapid, cost-effective diagnostic method for use in remote areas.

Published

2019

6. Versatile Polypeptide-Functionalized Plasmonic Paper as Synergistic Biocompatible and Antimicrobial Nanoplatform.

Author

Tie L, Răileanu M, Bacalum M, Codita I, Negrea ȘM, Caracoti CȘ, Drăgulescu EC, Campu A, Astilean S, and Focsan M

Subjects

Biofilms drug effects, Cell Line, Humans, Paper, Anti-Bacterial Agents chemistry, Anti-Bacterial Agents pharmacology, Biocompatible Materials chemistry, Biocompatible Materials pharmacology, Escherichia coli drug effects, Gold pharmacology, Metal Nanoparticles chemistry, Peptides pharmacology, Staphylococcus aureus drug effects

Abstract

Nowadays, thanks to nanotechnological progress, which itself guides us more and more closely toward not only the efficient design of innovative nanomaterials or nanostructures, but to the improvement of their functionality, we benefit from an important asset in the battle against pathogenic illnesses. Herein, we report a versatile biocompatible plasmonic nanoplatform based on a Whatman paper incorporating positively-charged gold nanospherical particles via the immersion approach. The morphological characterization of the as-engineered-plasmonic paper was examined by SEM (scanning electron microscopy) and HRTEM (high-resolution transmission electron microscopy) investigations, while its surface chemical modification with a synthetic polypeptide, specifically RRWHRWWRR-NH2 (P2), was proved by monitoring the plasmonic response of loaded gold nanospheres and the emission signal of P2 via fluorescence spectroscopy. The as-functionalized plasmonic paper is non-cytotoxic towards BJ fibroblast human cells at bactericidal concentrations. Finally, the antimicrobial activity of the P2-functionalized plasmonic paper on both planktonic bacteria and biofilms was tested against two reference strains: Gram-positive Bacteria, i.e., Staphylococcus aureus and the Gram-negative Bacteria, i.e., Escherichia coli , determining microbial inhibition of up to 100% for planktonic bacteria. In line with the above presented nanoplatform's proper design, followed by their functionalization with active antimicrobial peptides, new roads can be open for determining antibiotic-free treatments against different relevant pathogens.

Published

2020

7. Paper-based plasma sanitizers.

Author

Xie J, Chen Q, Suresh P, Roy S, White JF, and Mazzeo AD

Subjects

Porosity, Disinfection methods, Escherichia coli growth & development, Paper, Plasma Gases chemistry, Saccharomyces cerevisiae growth & development

Abstract

This work describes disposable plasma generators made from metallized paper. The fabricated plasma generators with layered and patterned sheets of paper provide a simple and flexible format for dielectric barrier discharge to create atmospheric plasma without an applied vacuum. The porosity of paper allows gas to permeate its bulk volume and fuel plasma, while plasma-induced forced convection cools the substrate. When electrically driven with oscillating peak-to-peak potentials of ±1 to ±10 kV, the paper-based devices produced both volume and surface plasmas capable of killing microbes. The plasma sanitizers deactivated greater than 99% of Saccharomyces cerevisiae and greater than 99.9% of Escherichia coli cells with 30 s of noncontact treatment. Characterization of plasma generated from the sanitizers revealed a detectable level of UV-C (1.9 nW⋅cm -2 ⋅nm -1 ), modest surface temperature (60 °C with 60 s of activation), and a high level of ozone (13 ppm with 60 s of activation). These results deliver insights into the mechanisms and suitability of paper-based substrates for active antimicrobial sanitization with scalable, flexible sheets. In addition, this work shows how paper-based generators are conformable to curved surfaces, appropriate for kirigami-like "stretchy" structures, compatible with user interfaces, and suitable for sanitization of microbes aerosolized onto a surface. In general, these disposable plasma generators represent progress toward biodegradable devices based on flexible renewable materials, which may impact the future design of protective garments, skin-like sensors for robots or prosthetics, and user interfaces in contaminated environments., Competing Interests: Conflict of interest statement: US Provisional Patent was filed (62/291,082) for “Low-Cost, Flexible, Paper-Based Plasma Sterilizer” on February 4, 2016. US Patent Application was filed (15/425,474) for “Flexible Plasma Applicators Based on Fibrous Layers” on February 6, 2017.

Published

2017

8. Quantitative E. coli Enzyme Detection in Reporter Hydrogel-Coated Paper Using a Smartphone Camera.

Author

Kaur K, Chelangat W, Druzhinin SI, Karuri NW, Müller M, and Schönherr H

Subjects

Escherichia coli enzymology, Escherichia coli Proteins analysis, Hydrogels chemistry, Kinetics, Lysogeny, Phosphates chemistry, Point-of-Care Systems, Smartphone, Video Recording, Biosensing Techniques instrumentation, Chitosan chemistry, Escherichia coli isolation & purification, Glucuronidase analysis

Abstract

There is a growing demand for rapid and sensitive detection approaches for pathogenic bacteria that can be applied by non-specialists in non-laboratory field settings. Here, the detection of the typical E. coli enzyme β-glucuronidase using a chitosan-based sensing hydrogel-coated paper sensor and the detailed analysis of the reaction kinetics, as detected by a smartphone camera, is reported. The chromogenic reporter unit affords an intense blue color in a two-step reaction, which was analyzed using a modified Michaelis-Menten approach. This generalizable approach can be used to determine the limit of detection and comprises an invaluable tool to characterize the performance of lab-in-a-phone type approaches. For the particular system analyzed, the ratio of reaction rate and equilibrium constants of the enzyme-substrate complex are 0.3 and 0.9 pM -1 h -1 for β-glucuronidase in phosphate buffered saline and lysogeny broth, respectively. The minimal degree of substrate conversion for detection of the indigo pigment formed during the reaction is 0.15, while the minimal time required for detection in this particular system is ~2 h at an enzyme concentration of 100 nM. Therefore, this approach is applicable for quantitative lab-in-a-phone based point of care detection systems that are based on enzymatic substrate conversion via bacterial enzymes.

Published

2021

9. Electrically-receptive and thermally-responsive paper-based sensor chip for rapid detection of bacterial cells.

Author

Khan MS, Misra SK, Dighe K, Wang Z, Schwartz-Duval AS, Sar D, and Pan D

Subjects

Acrylic Resins chemistry, Animals, Biosensing Techniques economics, Electricity, Electrodes, Lab-On-A-Chip Devices, Limit of Detection, Nanostructures chemistry, Nanostructures ultrastructure, Paper, Reproducibility of Results, Temperature, Bacillus subtilis isolation & purification, Biosensing Techniques instrumentation, Escherichia coli isolation & purification, Graphite chemistry, Lakes microbiology, Milk microbiology, Streptococcus mutans isolation & purification

Abstract

Although significant technological advancements have been made in the development of analytical biosensor chips for detecting bacterial strains (E. coli, S. Mutans and B. Subtilis), critical requirements i.e. limit of detection (LOD), fast time of response, ultra-sensitivity with high reproducibility and good shelf-life with robust sensing capability have yet to be met within a single sensor chip. In order to achieve these criteria, we present an electrically-receptive thermally-responsive (ER-TR) sensor chip comprised of simple filter paper used as substrate coated with composite of poly(N-isopropylacrylamide) polymer (PNIPAm) - graphene nanoplatelet (GR) followed by evaporation of Au electrodes for capturing both Gram-positive (S. mutans and B. subtilis) and Gram-negative (E. coli) bacterial cells in real-time. Autoclave water, tap water, lake water and milk samples were tested with ER-TR chip with and without bacterial strains at varying concentration range 10 1 -10 5 cells/mL. The sensor was integrated with in-house built printed circuit board (PCB) to transmit/receive electrical signals. The interaction of E. coli, S. mutans and B. subtilis cells with fibers of PNIPAm-GR resulted in a change of electrical resistance and the readout was monitored wirelessly in real-time using MATLAB algorithm. Finally, prepared ER-TR chip exhibited the reproducibility of 85-97% with shelf-life of up to four weeks after testing with lake water sample., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2018

10. Sterilization of paper during crisis

Author

Alshammari, Fwzah H. and Hussein, Hebat-Allah A.

Published

2022

11. Antibacterial cellulose paper made with silver-coated gold nanoparticles.

Author

Tsai TT, Huang TH, Chang CJ, Yi-Ju Ho N, Tseng YT, and Chen CF

Subjects

Adsorption, Anti-Bacterial Agents chemistry, Cellulose chemistry, Escherichia coli growth & development, Gold chemistry, Humans, Membranes, Artificial, Metal Nanoparticles ultrastructure, Microbial Sensitivity Tests, Paper, Silver chemistry, Anti-Bacterial Agents pharmacology, Escherichia coli drug effects, Food Packaging methods, Gold pharmacology, Metal Nanoparticles chemistry, Silver pharmacology

Abstract

In this study, we investigated the antibacterial activity of silver-coated gold nanoparticles (Au-Ag NPs) immobilized on cellulose paper. Ag NPs are known to have strong antibacterial properties, while Au NPs are biocompatible and relatively simple to prepare. We made the Au-Ag NPs using a facile process called Ag enhancement, in which Au NPs serve as the nuclei for precipitation of a Ag coating, the thickness of which can be easily controlled by varying the ratio of the reactants. After synthesis, electron microscopy showed that the Au-Ag NPs displayed a core-shell structure, and that they could be successfully immobilized onto a cellulose membrane by heat treatment. We then investigated the antibacterial properties of this NP-coated cellulose paper against E. coli JM109. The inhibition rate, growth curve, and AATCC 100 activity test showed that cellulose paper coated with 15 nm Au-Ag NPs possessed excellent antibacterial activity against E. coli JM109. These results suggest that Au-Ag NPs immobilized on cellulose paper could be a valuable antibacterial technology for applications such as food packaging, clothing, wound dressings, and other personal care products.

Published

2017

12. Bacteria survival probability in bactericidal filter paper.

Author

Mansur-Azzam N, Hosseinidoust Z, Woo SG, Vyhnalkova R, Eisenberg A, and van de Ven TG

Subjects

Colony Count, Microbial, Escherichia coli drug effects, Escherichia coli growth & development, Filtration, Fluorescence, Micelles, Microbial Sensitivity Tests, Triclosan pharmacology, Anti-Bacterial Agents pharmacology, Escherichia coli physiology, Microbial Viability drug effects, Paper, Probability

Abstract

Bactericidal filter papers offer the simplicity of gravity filtration to simultaneously eradicate microbial contaminants and particulates. We previously detailed the development of biocidal block copolymer micelles that could be immobilized on a filter paper to actively eradicate bacteria. Despite the many advantages offered by this system, its widespread use is hindered by its unknown mechanism of action which can result in non-reproducible outcomes. In this work, we sought to investigate the mechanism by which a certain percentage of Escherichia coli cells survived when passing through the bactericidal filter paper. Through the process of elimination, the possibility that the bacterial survival probability was controlled by the initial bacterial load or the existence of resistant sub-populations of E. coli was dismissed. It was observed that increasing the thickness or the number of layers of the filter significantly decreased bacterial survival probability for the biocidal filter paper but did not affect the efficiency of the blank filter paper (no biocide). The survival probability of bacteria passing through the antibacterial filter paper appeared to depend strongly on the number of collision between each bacterium and the biocide-loaded micelles. It was thus hypothesized that during each collision a certain number of biocide molecules were directly transferred from the hydrophobic core of the micelle to the bacterial lipid bilayer membrane. Therefore, each bacterium must encounter a certain number of collisions to take up enough biocide to kill the cell and cells that do not undergo the threshold number of collisions are expected to survive., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2014

13. Improvement in thermostability of metagenomic GH11 endoxylanase (Mxyl) by site-directed mutagenesis and its applicability in paper pulp bleaching process.

Author

Satyanarayana DV

Subjects

Amino Acid Sequence, Amino Acid Substitution, Arginine chemistry, Arginine genetics, Catalysis, Endo-1,4-beta Xylanases genetics, Enzyme Stability, Escherichia coli genetics, Kinetics, Metagenomics, Molecular Dynamics Simulation, Molecular Sequence Data, Mutagenesis, Site-Directed, Protein Structure, Tertiary, Recombinant Proteins genetics, Recombinant Proteins metabolism, Temperature, Endo-1,4-beta Xylanases chemistry, Escherichia coli enzymology, Industrial Microbiology, Paper

Abstract

An attempt has been made for enhancing the thermostability of xylanase (Mxyl) retrieved from a compost-soil-based metagenomic library. The analysis of the structure of xylanase by molecular dynamics simulation revealed more structural fluctuations in β-sheets. When the surface of β-sheets was enriched with arginine residues by substituting serine/threonine by site-directed mutagenesis, the enzyme with four arginine substitutions (MxylM4) exhibited enhanced thermostability at 80 °C. The T 1/2 of MxylM4 at 80 °C, in the presence of birchwood xylan, increased from 130 to 150 min at 80 °C without any alteration in optimum pH and temperature and molecular mass. Improvement in thermostability of MxylM4 was corroborated by increase in T m by 6 °C over that of Mxyl. The K m of MxylM4, however, increased from 8.01 ± 0.56 of Mxyl to 12.5 ± 0.32 mg ml(-1), suggesting a decrease in the affinity as well as specific enzyme activity. The Mxyl as well as MxylM4 liberated chromophores and lignin-derived compounds from kraft pulp, indicating their applicability in pulp bleaching.

Published

2013

14. Printable QR code paper microfluidic colorimetric assay for screening volatile biomarkers.

Author

Burklund A, Saturley-Hall HK, Franchina FA, Hill JE, and Zhang JXJ

Subjects

Colorimetry, Escherichia coli pathogenicity, Escherichia coli Infections microbiology, Gas Chromatography-Mass Spectrometry, Indoles chemistry, Microfluidics, Solid Phase Microextraction, Volatile Organic Compounds chemistry, Biosensing Techniques, Escherichia coli isolation & purification, Escherichia coli Infections blood, Volatile Organic Compounds isolation & purification

Abstract

We present a QR code paper microfluidic colorimetric assay that can exploit the hardware and software on mobile devices, and circumvent sample preparation by directly targeting volatile biomarkers. Our platform is a printable microarray of well-defined reaction regions, which outputs an instant diagnosis by directing the user to a URL containing their test result, while simultaneously storing epidemiological data for remote access and bioinformatics. To assist in the rapid identification of Escherichia coli in bloodstream infections, we employed an existing colorimetric reagent (p-dimethylaminocinnamaldehyde) and adapted its use to detect volatile indole, a biomarker produced by E. coli. Our assay was able to quantitatively detect indole in the headspace of E. coli culture after 12 h of growth (27.0 ± 3.1 ppm), assisting in species-level identification hours earlier than existing methods. Results were confirmed with headspace solid-phase microextraction (HS-SPME) two-dimensional gas chromatography time-of-flight mass spectrometry (GC×GC-ToFMS), which estimated indole concentration in E. coli culture to average 32.3 ± 5.2 ppm after 12 h of growth. This QR paper microfluidic platform represents a novel development in both telemedicine and diagnostics using volatile biomarkers. We envision that our QR code platform can be extended to other colorimetric assays for real-time diagnostics in low-resource environments., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2019

15. Efficient Enzymatic Hydrolysis and Polyhydroxybutyrate Production from Non-Recyclable Fiber Rejects from Paper Mills by Recombinant Escherichia coli.

Author

Jia, Linjing, Juneja, Ankita, Majumder, Erica L.-W., Ramarao, Bandaru V., and Kumar, Deepak

Subjects

ESCHERICHIA coli, HOT water, PAPER mills, CARBOHYDRATES, THERMAL properties, BIODEGRADABLE plastics, POLYHYDROXYBUTYRATE

Abstract

Non-recyclable fiber rejects from paper mills, particularly those from recycled linerboard mills, contain high levels of structural carbohydrates but are currently landfilled, causing financial and environmental burdens. The aim of this study was to develop efficient and sustainable bioprocess to upcycle these rejects into polyhydroxybutyrate (PHB), a biodegradable alternative to degradation-resistant petroleum-based plastics. To achieve high yields of PHB per unit biomass, the specific objective of the study was to investigate various approaches to enhance the hydrolysis yields of fiber rejects to maximize sugar recovery and evaluate the fermentation performance of these sugars using Escherichia coli LSBJ. The investigated approaches included size reduction, surfactant addition, and a chemical-free hydrothermal pretreatment process. A two-step hydrothermal pretreatment, involving a hot water pretreatment (150 °C and 15% solid loading for 10 min) followed by three cycles of disk refining, was found to be highly effective and resulted in an 83% cellulose conversion during hydrolysis. The hydrolysate obtained from pretreated biomass normally requires a detoxification step to enhance fermentation efficiency. However, the hydrolysate obtained from the pretreated biomass contained minimal to no inhibitory compounds, as indicated by the efficient sugar fermentation and high PHB yields, which were comparable to those from fermenting raw biomass hydrolysate. The structural and thermal properties of the extracted PHB were analyzed using various techniques and consistent with standard PHB. [ABSTRACT FROM AUTHOR]

Published

2024

16. Multiplexed paper test strip for quantitative bacterial detection.

Author

Hossain SM, Ozimok C, Sicard C, Aguirre SD, Ali MM, Li Y, and Brennan JD

Subjects

Colorimetry, Food Microbiology, Escherichia coli isolation & purification, Paper

Abstract

Rapid, sensitive, on-site detection of bacteria without a need for sophisticated equipment or skilled personnel is extremely important in clinical settings and rapid response scenarios, as well as in resource-limited settings. Here, we report a novel approach for selective and ultra-sensitive multiplexed detection of Escherichia coli (non-pathogenic or pathogenic) using a lab-on-paper test strip (bioactive paper) based on intracellular enzyme (β-galactosidase (B-GAL) or β-glucuronidase (GUS)) activity. The test strip is composed of a paper support (0.5 × 8 cm), onto which either 5-bromo-4-chloro-3-indolyl-β-D: -glucuronide sodium salt (XG), chlorophenol red β-galactopyranoside (CPRG) or both and FeCl(3) were entrapped using sol-gel-derived silica inks in different zones via an ink-jet printing technique. The sample was lysed and assayed via lateral flow through the FeCl(3) zone to the substrate area to initiate rapid enzyme hydrolysis of the substrate, causing a change from colorless-to-blue (XG hydrolyzed by GUS, indication of nonpathogenic E. coli) and/or yellow to red-magenta (CPRG hydrolyzed by B-GAL, indication of total coliforms). Using immunomagnetic nanoparticles for selective preconcentration, the limit of detection was ~5 colony-forming units (cfu) per milliliter for E. coli O157:H7 and ~20 cfu/mL for E. coli BL21, within 30 min without cell culturing. Thus, these paper test strips could be suitable for detection of viable total coliforms and pathogens in bathing water samples. Moreover, inclusion of a culturing step allows detection of less than 1 cfu in 100 mL within 8 h, making the paper tests strips relevant for detection of multiple pathogens and total coliform bacteria in beverage and food samples.

Published

2012

17. Method for lysis and paper-based elution-free DNA extraction with colourimetric isothermal amplification.

Author

Lee, Soo Min, Doeven, Egan H., Yuan, Dan, and Guijt, Rosanne M.

Subjects

NUCLEIC acid amplification techniques, ESCHERICHIA coli, MILK proteins, DNA, LYSIS, CELLULOSE esters, NUCLEIC acids, OCHRATOXINS

Abstract

Nucleic acid amplification testing has great potential for point-of-need diagnostic testing with high detection sensitivity and specificity. Current sample preparation is limited by a tedious workflow requiring multiple steps, reagents and instrumentation, hampering nucleic acid testing at point of need. In this study, we present the use of mixed cellulose ester (MCE) paper for DNA binding by ionic interaction under molecular crowding conditions and fluid transport by wicking. The poly(ethylene) glycol-based (PEG) reagent simultaneously provides the high pH for alkaline lysis and crowding effects for ionic binding of the DNA under high salt conditions. In this study, we introduce Paper-based Abridged Solid-Phase Extraction with Alkaline Poly(ethylene) Glycol Lysis (PASAP). The anionic mixed cellulose ester (MCE) paper is used as solid phase and allows for fluid transport by wicking, eliminating the need for pipetting skills and the use of a magnet to retain beads. Following the release of DNA from the cells due to the lytic activity of the PASAP solution, the DNA binds to the anionic surface of the MCE paper, concentrating at the bottom while the sample matrix is transported towards the top by wicking. The paper was washed by dipping it in 40% isopropanol for 10 s. After air-drying for 30 s, the bottom section of the paper (3 mm × 4 mm) was snapped off using the cap of a PCR tube and immersed in the colourimetric loop-mediated isothermal amplification (cLAMP) solution for direct amplification and colourimetric detection. The total sample processing was completed in 15 min and ready for amplification. cLAMP enabled the detection of 102 CFU/mL of Escherichia coli (E. coli) from culture media and the detection of E. coli in milk < 103 CFU/mL (10 CFU) after incubation at 68 °C for 60 min, demonstrating applicability of the method to complex biological samples. [ABSTRACT FROM AUTHOR]

Published

2024

18. Investigation of pathogenic Escherichia coli and microbial pathogens in pulp and paper mill biosolids.

Author

Croteau MC, Renner VE, Archibald F, Langlois VS, Cahn J, Ridal J, Trudeau VL, and Lean DR

Subjects

Biological Assay methods, Electrophoresis methods, Escherichia coli growth & development, Escherichia coli pathogenicity, Polymerase Chain Reaction methods, Serotyping methods, Escherichia coli isolation & purification, Industrial Waste analysis, Paper, Refuse Disposal, Water Microbiology

Abstract

Biosolids produced from pulp and paper mill wastewater treatment have excellent properties as soil conditioners, but often contain high levels of Escherichia coli. E. coli are commonly used as indicators of fecal contamination and health hazard; therefore, their presence in biosolids causes concern and has lead to restrictions in land-spreading. The objectives of this study were to determine the following: (1) if E. coli from the biosolids of a wastewater-free pulp and paper mill were enteric pathogens, and (2) if other waterborne microbial pathogens were present. E. coli were screened for heat-labile and heat-stable enterotoxin and verocytotoxin virulence genes using a polymerase chain reaction. Ten isolates were also screened for invasion-associated locus and invasion plasmid antigen H genes. None of the 120 isolates carried these genes. Tests for seven other microbial pathogens were negative. Effluents and biosolids from this mill do not contain common microbial pathogens and are unlikely to pose a health hazard.

Published

2007

19. Sterilization of paper during crisis

Author

Fwzah H. Alshammari and Hebat-Allah A. Hussein

Subjects

Gamma radiation, Dry heating, Respiratory pathogen, Paper structure, Escherichia coli, Salmonella typhi, Biotechnology, TP248.13-248.65, Microbiology, QR1-502

Abstract

Abstract Paper sheets represent one of the infection risk sources inside educational and administrative institutions under biological pandemics. So, the present study aimed to validate the efficiency of gamma radiation or dry heat techniques to sterilize contaminated paper sheets with different indicator pathogens while retaining their structure. The results showed that gamma radiation at 6, 12, or 24 kGy can successfully kill Gram-positive bacteria such as Bacillus cereus and Staphylococcus aureus, Gram-negative bacteria such as Escherichia coli and Salmonella typhi, and fungi such as Candida albicans. Moreover, dry heating at 100 °C for 60 min, 150 °C for 30 min, or 200 °C for 15 min can be successful in paper decontamination of all tested species. Surprisingly, scanning electron microscopy (SEM) micrographs proved that gamma radiation at 6 kGy, dry heat at 100 °C for 60 min or 150 °C for 30 min or 200 °C for 15 min, is suitable for paper sheet sterilization while maintaining their structure. Ultimately, dry heat is a simple, effective, fast, safe, and inexpensive technique for paper sterilization. It may be used as a precautionary step inside educational institutions, especially during written examination periods, to ensure a safe life for academic members during biological pandemics such as COVID-19.

Published

2022

20. DipTest: A litmus test for E. coli detection in water.

Author

Gunda NSK, Dasgupta S, and Mitra SK

Subjects

Color, Culture Media, Escherichia coli growth & development, Escherichia coli isolation & purification, Microbiological Techniques methods, Paper, Water Microbiology

Abstract

We have developed a new litmus paper test (DipTest) for detecting Escherichia coli (E. coli) in water samples by performing enzymatic reactions directly on the porous paper substrate. The paper strip consists of a long narrow piece of cellulose blotting paper coated with chemoattractant (at bottom edge), wax hydrophobic barrier (at the top edge), and custom formulated chemical reagents (at reaction zone immediately below the wax hydrophobic barrier). When the paper strip is dipped in water, E. coli in the water sample is attracted toward the paper strip due to a chemotaxic mechanism followed by the ascent along the paper strip toward the reaction zone due to a capillary wicking mechanism, and finally the capillary motion is arrested at the top edge of the paper strip by the hydrophobic barrier. The E. coli concentrated at the reaction zone of the paper strip will react with custom formulated chemical reagents to produce a pinkish-red color. Such a color change on the paper strip when dipped into water samples indicates the presence of E. coli contamination in potable water. The performance of the DipTest device has been checked with different known concentrations of E. coli contaminated water samples using different dip and wait times. The DipTest device has also been tested with different interfering bacteria and chemical contaminants. It has been observed that the different interfering contaminants do not have any impact on the DipTest, and it can become a potential solution for screening water samples for E. coli contamination at the point of source.

Published

2017

21. Advancing Food Preservation: Sustainable Green-AgNPs Bionanocomposites in Paper-Starch Flexible Packaging for Prolonged Shelf Life.

Author

Trotta, Federico, Da Silva, Sidonio, Massironi, Alessio, Mirpoor, Seyedeh Fatemeh, Lignou, Stella, Ghawi, Sameer Khalil, and Charalampopoulos, Dimitris

Subjects

*FOOD preservation, *FLEXIBLE packaging, *FOOD packaging, *ESCHERICHIA coli, *FOOD waste, *CORNSTARCH

Abstract

In the pursuit of enhancing food packaging, nanotechnology, particularly green silver nanoparticles (G-AgNPs), have gained prominence for its remarkable antimicrobial properties with high potential for food shelf-life extension. Our study aims to develop corn starch-based coating materials reinforced with G-AgNPs. The mechanical properties were examined using a uniaxial tensile tester, revealing that starch coated with the highest G-AgNPs concentration (12.75 ppm) exhibited UTS of 87.6 MPa compared to 48.48 MPa of control paper, a significant (p < 0.02) 65% increase. The assessment of the WVP showcased a statistical reduction in permeability by up to 8% with the incorporation of the hydrophobic layer. Furthermore, antibacterial properties were assessed following ISO 22196:2011, demonstrating a strong and concentration-dependent activity of G-AgNPs against E. coli. All samples successfully disintegrated in both simulated environments (soil and seawater), including samples presenting G-AgNPs. In the food trial analysis, the presence of starch and G-AgNPs significantly reduced weight loss after 6 days, with cherry tomatoes decreasing by 8.59% and green grapes by 6.77% only. The results of this study contribute to the advancement of environmentally friendly packaging materials, aligning with the UN sustainable development goals of reducing food waste and promoting sustainability. [ABSTRACT FROM AUTHOR]

Published

2024

22. Bioengineering bacteriophages to enhance the sensitivity of phage amplification-based paper fluidic detection of bacteria.

Author

Alcaine SD, Law K, Ho S, Kinchla AJ, Sela DA, and Nugen SR

Subjects

Alkaline Phosphatase genetics, Bacterial Proteins genetics, Escherichia coli genetics, Genetic Engineering methods, Limit of Detection, Maltose-Binding Proteins genetics, Up-Regulation, Bacteriophage T7 genetics, Bioengineering methods, Biosensing Techniques methods, Environmental Monitoring methods, Escherichia coli isolation & purification, Escherichia coli virology, Rivers microbiology

Abstract

Bacteriophage (phage) amplification is an attractive method for the detection of bacteria due to a narrow phage-host specificity, short amplification times, and the phages' ability to differentiate between viable and non-viable bacterial cells. The next step in phage-based bacteria detection is leveraging bioengineered phages to create low-cost, rapid, and easy-to-use detection platforms such as lateral flow assays. Our work establishes the proof-of-concept for the use of bioengineered T7 phage strains to increase the sensitivity of phage amplification-based lateral flow assays. We have demonstrated a greater than 10-fold increase in sensitivity using a phage-based protein reporter, maltose-binding protein, over the detection of replicated T7 phage viron itself, and a greater then 100-fold increase in sensitivity using a phage-based enzymatic reporter, alkaline phosphatase. This increase in sensitivity enabled us to detect 10(3)CFU/mL of Escherichia coli in broth after 7h, and by adding a filter concentration step, the ability to detect a regulatory relevant E. coli concentration of 100CFU/100mL in inoculated river water after 9h, where the current standard requires days for results. The combination of the paper fluidic format with phage-based detection provides a platform for the development of novel diagnostics that are sensitive, rapid, and easy to use., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

23. Pick Your Poisson: An Educational Primer for Luria and Delbrück's Classic Paper.

Author

Meneely PM

Subjects

History, 20th Century, Humans, Immunity genetics, Mutation Rate, Poisson Distribution, Escherichia coli genetics, Genetics history, Models, Genetic, Mutation

Abstract

The origin of beneficial mutations is fundamentally important in understanding the processes by which natural selection works. Using phage-resistant mutants in Escherichia coli as their model for identifying the origin of beneficial mutations, Luria and Delbrück distinguished between two different hypotheses. Under the first hypothesis, which they termed "acquired immunity," the phages induced bacteria to mutate to immunity; this predicts that none of the resistant mutants were present before infection by the phages. Under the second hypothesis, termed "mutation to immunity," resistant bacteria arose from random mutations independent of the presence of the phages; this predicts that resistant bacteria were present in the population before infection by the phages. These two hypotheses could be distinguished by calculating the frequencies at which resistant mutants arose in separate cultures infected at the same time and comparing these frequencies to the theoretical results under each model. The data clearly show that mutations arise at a frequency that is independent of the presence of the phages. By inference, natural selection reveals the genetic variation that is present in a population rather than inducing or causing this variation., (Copyright © 2016 by the Genetics Society of America.)

Published

2016

24. An inexpensive, high-throughput μPAD assay of microbial growth rate and motility on solid surfaces using Saccharomyces cerevisiae and Escherichia coli as model organisms.

Author

Levy AF, Labrador A, Knecht L, and Van Dyken JD

Subjects

Equipment Design, Lab-On-A-Chip Devices economics, Microbial Viability, Models, Biological, Paper, Reproducibility of Results, Waxes, Escherichia coli growth & development, Microfluidic Analytical Techniques instrumentation, Saccharomyces cerevisiae growth & development

Abstract

Many microbial phenotypes are differentially or exclusively expressed on agar surfaces, including biofilms, motility, and sociality. However, agar-based assays are limited by their low throughput, which increases costs, lab waste, space requirements, and the time required to conduct experiments. Here, we demonstrate the use of wax-printed microfluidic paper-based analytical devices (μPADs) to measure linear growth rate of microbes on an agar growth media as a means of circumventing the aforementioned limitations. The main production materials of the proposed μPAD design are a wax printer, filter paper, and empty pipet boxes. A single wax-printed μPAD allowing 8 independent, agar-grown colonies costs $0.07, compared to $0.20 and $9.37 for the same number of replicates on traditional microtiter/spectrophotometry and Petri dish assays, respectively. We optimized the μPAD design for channel width (3 mm), agar volume (780 μL/channel), and microbe inoculation method (razor-blade). Comparative analyses of the traditional and proposed μPAD methods for measuring growth rate of nonmotile (Saccharomyces cerevisiae) and motile (flagellated Escherichia coli) microorganisms suggested the μPAD assays conferred a comparable degree of accuracy and reliability to growth rate measurements as their traditional counterparts. We substantiated this claim with strong, positive correlations between the traditional and μPAD assay, a significant nonzero slope in the model relating the two assays, a nonsignificant difference between the relative standard errors of the two techniques, and an analysis of inter-device reliability. Therefore, μPAD designs merit consideration for the development of enhanced-throughput, low-cost microbial growth and motility assays., Competing Interests: The authors have declared that no competing interests exist.

Published

2020

25. Toxicity of Graphene Shells, Graphene Oxide, and Graphene Oxide Paper Evaluated with Escherichia coli Biotests.

Author

Efremova LV, Vasilchenko AS, Rakov EG, and Deryabin DG

Subjects

Cell Survival drug effects, Escherichia coli ultrastructure, Microscopy, Atomic Force, Oxidative Stress drug effects, Oxides toxicity, Reactive Oxygen Species, Escherichia coli drug effects, Graphite toxicity, Nanoshells toxicity, Nanostructures toxicity

Abstract

The plate-like graphene shells (GS) produced by an original methane pyrolysis method and their derivatives graphene oxide (GO) and graphene oxide paper (GO-P) were evaluated with luminescent Escherichia coli biotests and additional bacterial-based assays which together revealed the graphene-family nanomaterials' toxicity and bioactivity mechanisms. Bioluminescence inhibition assay, fluorescent two-component staining to evaluate cell membrane permeability, and atomic force microscopy data showed GO expressed bioactivity in aqueous suspension, whereas GS suspensions and the GO-P surface were assessed as nontoxic materials. The mechanism of toxicity of GO was shown not to be associated with oxidative stress in the targeted soxS::lux and katG::lux reporter cells; also, GO did not lead to significant mechanical disruption of treated bacteria with the release of intracellular DNA contents into the environment. The well-coordinated time- and dose-dependent surface charge neutralization and transport and energetic disorders in the Escherichia coli cells suggest direct membrane interaction, internalization, and perturbation (i.e., "membrane stress") as a clue to graphene oxide's mechanism of toxicity.

Published

2015

26. Writing the Scientific Paper in the Investigative Lab

Author

Gubanich, Alan A.

Published

1977

27. Preparation and Application of In-Situ Loaded Silver Nanoparticles Antibacterial Fresh-Keeping Composite Paper.

Author

Lin, Guangzhi, Li, Xia, and Zhao, Chuanshan

Subjects

SILVER nanoparticles, SWEET cherry, ESCHERICHIA coli, CHERRIES, FRUIT packaging, PAPER products, FRUIT

Abstract

The freshness and safety of fruits and vegetables affect our daily life. Paper products are often used in the packaging and transportation of fruits and vegetables, and these can provide other functions besides packaging after certain modifications and additions. In this study, the AgNPs/1-MCP antibacterial fresh-keeping composite paper was prepared by in-situ loaded silver nanoparticles and spraying 1-MCP solution. Moreover, the prepared paper was used to preserve sweet cherries. It was found that the prepared AgNPs/1-MCP antibacterial fresh-keeping composite paper could effectively inhibit E. coli and S. aureus. When the addition of 1-MCP in the paper was 0.05 g, the fresh-keeping effect on cherries was the best. Under this optimal condition, the weight loss ratio of the cherries was reduced by 1.93%, the firmness was increased by 27.7%, and the soluble solid content was increased by 25%. The preservation time was extended from 4 days to 12 days, three times that of the untreated ones. The prepared fresh-keeping material is environmentally friendly, non-toxic and harmless, simple to prepare and convenient to use, and is expected to become one of the important fresh-keeping methods for fruits. [ABSTRACT FROM AUTHOR]

Published

2022

28. Protein Science "Best Paper" awards to Youngil Chang and Liam Longo.

Author

Matthews BW

Subjects

Humans, Adenosine Triphosphate metabolism, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Fibroblast Growth Factor 1 chemistry, Protein Folding, Proteome metabolism, Proteomics methods

Published

2013

29. Development of a Tetrazolium-Derived Paper-Based Diagnostic Device as an Early, Alternative Bacteria Screening Tool

Author

Michael Muljadi, Chao-Min Cheng, and Ching-Ju Shen

Subjects

bacterial detection, paper-based diagnostics, MTT-PMS, Escherichia coli, Mechanical engineering and machinery, TJ1-1570

Abstract

(1) Background: The complexity, amount of time, and the large amount of resource required to perform gold-standard bacteria culture procedures makes it difficult to perform timely pathogenic analyses, especially in areas where such resources are not readily available. A paper-based biochemical analytical tool can potentially tackle problems economically in terms of time and convenience, potentially finding utility in applications where simple and timely detection of bacteria is necessary; (2) Methods: The utility of paper-based MTT-PMS strips was tested using a simple colorimetric analytical methodology; (3) Results: Sufficient evidence was obtained to suggest that the strips can potentially be used as a rapid and convenient early, alternative bacteria screening tool for a variety of applications; (4) Conclusions: The potential of strips for the rapid detection of bacteria compared to standard bacteria culture is a key advantage in certain clinical, agricultural, and environmental applications.

Published

2021

30. Ionic Liquid Aqueous Two-Phase Systems for the Enhanced Paper-Based Detection of Transferrin and Escherichia coli

Author

Yee, Matthew F, Emmel, Grace N, Yang, Eric J, Lee, Eumene, Paek, Justin H, Wu, Benjamin M, and Kamei, Daniel T

Subjects

Chemical Sciences, ionic liquid, aqueous two-phase systems, lateral-flow immunoassay, transferrin, Escherichia coli, Chemical sciences

Abstract

Aqueous two-phase systems (ATPSs) have been widely utilized for liquid-liquid extraction and purification of biomolecules, with some studies also demonstrating their capacity as a biomarker concentration technique for use in diagnostic settings. As the limited polarity range of conventional polymer-based ATPSs can restrict their use, ionic liquid (IL)-based ATPSs have been recently proposed as a promising alternative to polymer-based ATPSs, since ILs are regarded as tunable solvents with excellent solvation capabilities for a variety of natural compounds and proteins. This study demonstrates the first application of IL ATPSs to point-of-care diagnostics. ATPSs consisting of 1-butyl-3-methylimidazolium tetrafluoroborate ([Bmim][BF4]) and sodium phosphate salt were utilized to quickly concentrate biomarkers prior to detection using the lateral-flow immunoassay (LFA). We found the phase separation speed of the IL ATPS to be very rapid and a significant improvement upon the separation speed of both polymer-salt and micellar ATPSs. This system was successfully applied to both sandwich and competitive LFA formats and enhanced the detection of both Escherichia coli bacteria and the transferrin protein up to 8- and 20-fold, respectively. This system's compatibility with a broad range of biomolecules, rapid phase separation speed, and tunability suggest wide applicability for a large range of different antigens and biomarkers.

Published

2018

31. Evolution of restraint in a structured rock-paper-scissors community.

Author

Nahum JR, Harding BN, and Kerr B

Subjects

Altruism, Selection, Genetic, Computer Simulation, Escherichia coli genetics, Evolution, Molecular

Abstract

It is not immediately clear how costly behavior that benefits others evolves by natural selection. By saving on inherent costs, individuals that do not contribute socially have a selective advantage over altruists if both types receive equal benefits. Restrained consumption of a common resource is a form of altruism. The cost of this kind of prudent behavior is that restrained individuals give up resources to less-restrained individuals. The benefit of restraint is that better resource management may prolong the persistence of the group. One way to dodge the problem of defection is for altruists to interact disproportionately with other altruists. With limited dispersal, restrained individuals persist because of interaction with like types, whereas it is the unrestrained individuals that must face the negative long-term consequences of their rapacity. Here, we study the evolution of restraint in a community of three competitors exhibiting a nontransitive (rock-paper-scissors) relationship. The nontransitivity ensures a form of negative feedback, whereby improvement in growth of one competitor has the counterintuitive consequence of lowering the density of that improved player. This negative feedback generates detrimental long-term consequences for unrestrained growth. Using both computer simulations and evolution experiments with a nontransitive community of Escherichia coli, we find that restrained growth can evolve under conditions of limited dispersal in which negative feedback is present. This research, thus, highlights a set of ecological conditions sufficient for the evolution of one form of altruism.

Published

2011

32. Anti-bacterial activity of ethanolic extract of Indoneesiella echioides (L) nees. evaluated by the filter paper disc method.

Author

Qadrie ZL, Jacob B, Anandan R, Rajkapoor B, and Rahamathulla M

Subjects

Colony Count, Microbial, Disk Diffusion Antimicrobial Tests, Escherichia coli growth & development, Ethanol chemistry, Solvents chemistry, Staphylococcus aureus growth & development, Anti-Bacterial Agents pharmacology, Escherichia coli drug effects, Plant Extracts pharmacology, Plants, Medicinal, Staphylococcus aureus drug effects

Abstract

The study was carried out to investigate the antibacterial activity of the ethanolic extracts of Indoneesiella echioides (L) Nees. was evaluated by the filter paper disc method. This method is based on the diffusion of an antibiotic from a filter paper disc through the solidified culture media of a Petri dish used for study. The growth of inoculated is inhibited entirely in a circular area "Zone around the filter" paper disc containing a solution of antibiotic and the plant extract. The microorganisms used were: 1. Staphylococcus aureus (Gram positive 2. Escherichia coli (Gram negative). The organisms were maintained on nutrient agar slants. These were tested using nutrient broth. One loop full of the respective cultures was taken in slants which were maintained below 40 degrees C were taken and inoculated in the broth and incubated at 37 degrees C for 24 hrs and were observed for the growth of the organism with naked eye for their turbid nature. It was compared with that of sterile broth. The presence of turbidity indicated growth and suitability of the culture for further work.

Published

2009

33. Antibiotic-mediated antagonism leads to a bacterial game of rock-paper-scissors in vivo.

Author

Kirkup BC and Riley MA

Subjects

Animals, Colon microbiology, Escherichia coli drug effects, Escherichia coli isolation & purification, Feces microbiology, Game Theory, Housing, Animal, Male, Mice, Streptomycin pharmacology, Anti-Bacterial Agents metabolism, Colicins metabolism, Drug Resistance, Bacterial, Escherichia coli classification, Escherichia coli physiology, Models, Biological

Abstract

Colicins are narrow-spectrum antibiotics produced by and active against Escherichia coli and its close relatives. Colicin-producing strains cannot coexist with sensitive or resistant strains in a well-mixed culture, yet all three phenotypes are recovered in natural populations. Recent in vitro results conclude that strain diversity can be promoted by colicin production in a spatially structured, non-transitive interaction, as in the classic non-transitive model rock-paper-scissors (RPS). In the colicin version of the RPS model, strains that produce colicins (C) kill sensitive (S) strains, which outcompete resistant (R) strains, which outcompete C strains. Pairwise in vitro competitions between these three strains are resolved in a predictable order (C beats S, S beats R, and R beats C), but the complete system of three strains presents the opportunity for dynamic equilibrium. Here we provide conclusive evidence of an in vivo antagonistic role for colicins and show that colicins (and potentially other bacteriocins) may promote, rather than eliminate, microbial diversity in the environment.

Published

2004

34. Local dispersal promotes biodiversity in a real-life game of rock-paper-scissors.

Author

Kerr B, Riley MA, Feldman MW, and Bohannan BJ

Subjects

Antidotes metabolism, Cell Division, Drug Resistance, Bacterial, Environment, Escherichia coli cytology, Selection, Genetic, Colicins metabolism, Ecosystem, Escherichia coli classification, Escherichia coli physiology, Models, Biological

Abstract

One of the central aims of ecology is to identify mechanisms that maintain biodiversity. Numerous theoretical models have shown that competing species can coexist if ecological processes such as dispersal, movement, and interaction occur over small spatial scales. In particular, this may be the case for non-transitive communities, that is, those without strict competitive hierarchies. The classic non-transitive system involves a community of three competing species satisfying a relationship similar to the children's game rock-paper-scissors, where rock crushes scissors, scissors cuts paper, and paper covers rock. Such relationships have been demonstrated in several natural systems. Some models predict that local interaction and dispersal are sufficient to ensure coexistence of all three species in such a community, whereas diversity is lost when ecological processes occur over larger scales. Here, we test these predictions empirically using a non-transitive model community containing three populations of Escherichia coli. We find that diversity is rapidly lost in our experimental community when dispersal and interaction occur over relatively large spatial scales, whereas all populations coexist when ecological processes are localized.

Published

2002

35. Application of paper chromatograms to the study of inducers of lambda bacteriophage in Escherichia coli.

Author

Heinemann B, Howard AJ, and Hollister ZJ

Subjects

Antineoplastic Agents analysis, Mitomycins analysis, Paromomycin analysis, Chromatography, Paper, Coliphages, Escherichia coli

Abstract

A procedure has been developed whereby paper chromatograms of agents which induce lambda bacteriophage in Escherichia coli can be developed using bioautographs with a lysogenic test system. Well-defined plaque-forming zones are produced indicating the area on the paper chromatogram where the active inducing material can be located. A mixture of the bacteriophage-inducing antibiotic, mitomycin C, and the noninducing antibiotic, paromomycin, was resolved into its components on paper strips with an ethyl acetate-methanol solvent system. The location of both antibiotics could thus be readily observed. Antibacterial and inducing activities were found to be identical with a crude fermentation solid, NSC-B-158,791. The use of this procedure for resolution of multicomponent inducing activities in antibiotic beers and for characterization of active components which may be potential antitumor antibiotics is indicated.

Published

1967

36. Validation of quantitative loop-mediated isothermal amplification assay using a fluorescent distance-based paper device for detection of Escherichia coli in urine.

Author

Saengsawang, Natkrittaya, Ruang-areerate, Panthita, Kaeothaisong, Nuanlaong, Leelayoova, Saovanee, Mungthin, Mathirut, Juntanawiwat, Piraporn, Hanyanunt, Patomroek, Potisuwan, Patsanun, Kesakomol, Piyanate, Butsararattanagomen, Pornphan, Wichaiwong, Pattarawadee, Dungchai, Wijitar, and Ruang-areerate, Toon

Subjects

*ESCHERICHIA coli, *RESOURCE-limited settings, *URINARY tract infections, *HEALTH facilities, *BACTERIAL diseases, *FEMALES

Abstract

Uropathogenic Escherichia coli (UPEC) causes up to 90% of urinary tract infections (UTI) which is more prevalent among females than males. In urine, patients with symptomatic UTI usually have a high concentration of bacterial infection, ≥ 105 colony-forming units (CFU) per mL, in which the culture method is regularly the gold standard diagnosis. In this study, a simple and inexpensive distance-based paper device (dPAD) combined with the fluorescent closed tube LAMP assay was validated for simultaneously screening and semi-quantifying the infection level of E. coli in 440 urine samples of patients with UTI. The dPAD could measure the LAMP amplicons and semi-quantify the levels of E. coli infection in heavy (≥ 104 CFU/mL), light (≤ 103 CFU/mL) and no infection. The sensitivity and specificity had reliable performances, achieving as high as 100 and 92.7%, respectively. The one step LAMP assay could be performed within 3 h, which was 7.5 times faster than the culture method. To empower early UTI diagnosis and fast treatment, this inexpensive dPAD tool combined with the fluorescent closed tube LAMP assay is simple, reliably fast and practically portable for point-of-care settings, particularly in resource-limited areas, which can be set up in all levels of healthcare facilities. [ABSTRACT FROM AUTHOR]

Published

2023

37. Turntable Paper-Based Device to Detect Escherichia coli

Author

Yung-Chih Wang, Yao-Hung Tsai, Ching-Fen Shen, Ming-Yao He, Yi-Chen Fu, Chen-Yu Sang, Yi-Tzu Lee, and Chao-Min Cheng

Subjects

Escherichia coli, paper-based ELISA, point-of-care, turntable, Mechanical engineering and machinery, TJ1-1570

Abstract

Escherichia coli has been known to cause a variety of infectious diseases. The conventional enzyme-linked immunosorbent assay (ELISA) is a well-known method widely used to diagnose a variety of infectious diseases. This method is expensive and requires considerable time and effort to conduct and complete multiple integral steps. We previously proposed the use of paper-based ELISA to rapidly detect the presence of E. coli. This approach has demonstrated utility for point-of-care (POC) urinary tract infection diagnoses. Paper-based ELISA, while advantageous, still requires the execution of several procedural steps. Here, we discuss the design and experimental implementation of a turntable paper-based device to simplify the paper-based ELISA protocols for the detection of E. coli. In this process, antibodies or reagents are preloaded onto zones of a paper-based device and allowed to dry before use. We successfully used this device to detect E. coli with a detection limit of 105 colony-forming units (colony-forming unit [CFU])/mL.

Published

2021

38. Quantitative E. coli Enzyme Detection in Reporter Hydrogel-Coated Paper Using a Smartphone Camera

Author

Kawaljit Kaur, Winny Chelangat, Sergey I. Druzhinin, Nancy Wangechi Karuri, Mareike Müller, and Holger Schönherr

Subjects

bacteria detection, paper-based biosensors, Escherichia coli, β-glucuronidase, reporter hydrogels, lab-in-a-phone, Biotechnology, TP248.13-248.65

Abstract

There is a growing demand for rapid and sensitive detection approaches for pathogenic bacteria that can be applied by non-specialists in non-laboratory field settings. Here, the detection of the typical E. coli enzyme β-glucuronidase using a chitosan-based sensing hydrogel-coated paper sensor and the detailed analysis of the reaction kinetics, as detected by a smartphone camera, is reported. The chromogenic reporter unit affords an intense blue color in a two-step reaction, which was analyzed using a modified Michaelis–Menten approach. This generalizable approach can be used to determine the limit of detection and comprises an invaluable tool to characterize the performance of lab-in-a-phone type approaches. For the particular system analyzed, the ratio of reaction rate and equilibrium constants of the enzyme–substrate complex are 0.3 and 0.9 pM−1h−1 for β-glucuronidase in phosphate buffered saline and lysogeny broth, respectively. The minimal degree of substrate conversion for detection of the indigo pigment formed during the reaction is 0.15, while the minimal time required for detection in this particular system is ~2 h at an enzyme concentration of 100 nM. Therefore, this approach is applicable for quantitative lab-in-a-phone based point of care detection systems that are based on enzymatic substrate conversion via bacterial enzymes.

Published

2021

39. Bacterial contamination of Ugandan paper currency notes possessed by food vendors around Mulago Hospital complex, Uganda

Author

Muhumuza Allan, Catherine Atuhaire, Musisi Nathan, Francis Ejobi, and Samuel Nambile Cumber

Subjects

bacterial contamination, pathogens, food vendors, escherichia coli, staphylococcus aureus, paper notes, Medicine

Abstract

INTRODUCTION: Paper currency notes, exchangeable fomite, that is continuously contaminated because of the poor handling and storage practices. Objective: the general objective of the study was to determine the bacterial contamination of paper currency notes possessed by food vendors around Mulago National Referral Hospital Complex.

Published

2018

40. Preparation and characterization of a sustained-release antibacterial melamine-impregnated paper based on Ag-BTC.

Author

He, Jinrong, Feng, Yun, Jiang, Jinrui, Qu, Wei, Wu, Yuzhang, and Peng, Limin

Subjects

*CONTROLLED release preparations, *MELAMINE, *ESCHERICHIA coli, *PARTICLE size distribution, *THERMAL stability, *MELAMINE-formaldehyde resins

Abstract

Melamine-impregnated paper is made by impregnating paper with melamine-formaldehyde resin and can be hot-pressed and laminated onto the surface of wood boards. If the paper has antibacterial activity, it can prevent the spread of indoor bacteria, but impregnated paper with a long-term antibacterial effect has not been proposed. Metal–organic frameworks (MOFs) have been studied as a reservoir of metal ions. In this study, a silver-metal organic framework (Ag-BTC) was synthesized by a green and scalable method at 60 °C (A-60) and at room temperature (A-25). The structure and thermal stability of the Ag-BTC were characterized. Compared with A-25, the structure and particle size distribution of A-60 were more regular and uniform. The thermal stability and the compatibility of Ag-BTC and MF resin were suitable for hot-pressing process. Ag-BTC in the cured impregnated paper exhibited the sustained-release performance of Ag+. The antibacterial ratio of decorated blockboards with 0.10 wt% A-25 to E. coli and S. aureus exceeded 99.99%, reaching Level I antibacterial grade. Compared with A-60-decorated blockboards, the better antibacterial activity of A-25-decorated blockboards was due to the release of more Ag+. This study provides new ideas for the design of antibacterial melamine-impregnated paper. [ABSTRACT FROM AUTHOR]

Published

2023

41. An Origami Paper-Based Device Printed with DNAzyme-Containing DNA Superstructures for Escherichia coli Detection

Author

Yating Sun, Yangyang Chang, Qiang Zhang, and Meng Liu

Subjects

colorimetric, DNAzyme, Escherichia coli, paper-based device, rolling circle amplification, Mechanical engineering and machinery, TJ1-1570

Abstract

Rapid detection of pathogenic bacteria is extremely important for public health and safety. Here, we describe for the first time an integrated origami paper-based analytical device (PAD) incorporating cell lysis, molecular recognition, amplification and visual detection of Escherichia coli (E. coli). The device features three components: paper for its ability to extract protein molecules nonspecifically from cells, DNA superstructures for their ability to immobilize RNA-cleaving DNAzymes (RCDs) but undergo target-induced RNA cleavage on paper, and isothermal rolling circle amplification (RCA) for its ability to amplify each cleavage event into repetitive sequence units that can be detected by naked eye. This device can achieve detection of E. coli K12 with a detection limit of as low as 103 CFU·mL−1 in a total turnaround time of 35 min. Furthermore, this device allowed the sensitive detection of E. coli in complex sample matrices such as juice and milk. Given that more specific RCDs can be evolved for diverse bacteria, the integrated PAD holds great potential for rapid, sensitive and highly selective detection of pathogenic bacteria in resource-limited settings.

Published

2019

42. Comparison of paired whole milk and dried filter paper samples for anti-enterotoxin and anti-rotavirus activities.

Author

Brown SE 3rd, Sauer KT, Nations-Shields M, Shields DS, Araujo JG, and Guerrant RL

Subjects

Animals, Cattle, Cholera Toxin, Escherichia coli Infections immunology, Female, Humans, Lactation, Microbiological Techniques, Paper, Pregnancy, Antibodies, Bacterial analysis, Antibodies, Viral analysis, Colostrum immunology, Enterotoxins isolation & purification, Escherichia coli immunology, Milk immunology, Milk, Human immunology, Reoviridae immunology, Rotavirus immunology, Vibrio cholerae immunology

Abstract

Milk specimens, 75 from cows immunized against cholera toxin and 35 from a human population in which enterotoxigenic Escherichia coli and rotaviral infections are endemic, were collected as paired filter paper and frozen whole milk samples. Each pair was tested for antibody activity against heat-labile E. coli and Vibrio cholerae enterotoxins. Additionally, 12 of the 35 paired human milk samples stored as frozen whole milk and dried on filter paper were tested for anti-rotavirus immunoglobulin A. Anti-enterotoxin and anti-rotavirus immunoglobulin A titers in milk dried on filter paper compared favorably with those of their frozen whole milk pairs. Filter paper samples offered considerable advantages for field collection, transportation, and storage over frozen liquid samples.

Published

1982

43. Lysis and direct detection of coliforms on printed paper-based microfluidic devices

Author

J. Scott VanEpps, Chao Li, Mathew Boban, Sarah A. Snyder, Anish Tuteja, and Geeta Mehta

Subjects

Lysis, Materials science, Microfluidics, Water contamination, Biomedical Engineering, Bioengineering, 02 engineering and technology, Water safety, 010402 general chemistry, 01 natural sciences, Biochemistry, Article, Lab-On-A-Chip Devices, Escherichia coli, Process engineering, Direct printing, business.industry, Multiple applications, food and beverages, General Chemistry, Paper based, Contamination, 021001 nanoscience & nanotechnology, 0104 chemical sciences, 0210 nano-technology, business

Abstract

Coliforms are one of the most common families of bacteria responsible for water contamination. Certain coliform strains can be extremely toxic, and even fatal if consumed. Current technologies for coliform detection are expensive, require multiple complicated steps, and can take up to 24 hours to produce accurate results. Recently, open-channel, paper-based microfluidic devices have become popular for rapid, inexpensive, and accurate bioassays. In this work, we have created an integrated microfluidic coliform lysis and detection device by fabricating customizable omniphilic regions via direct printing of omniphilic channels on an omniphobic, fluorinated paper. This paper-based device is the first of its kind to demonstrate successful cell lysing on-chip, as it can allow for the flow and control of both high and low surface tension liquids, including different cell lysing agents. The fabricated microfluidic device was able to successfully detect E. coli, via the presence of the coliform-specific enzyme, β-galactosidase, at a concentration as low as ~10(4) CFU/mL. Further, E. coli at an initial concentration of 1 CFU mL(−1) could be detected after only 6 hours of incubation. We believe that these devices can be readily utilized for real world E. coli contamination detection in multiple applications, including food and water safety.

Published

2020

44. Design and fabrication of microfibrous composite scaffold by coating clindamycin and chitosan onto cellulose filter paper for wound dressing applications.

Author

Haider, Sajjad, Farooq, Nadia, khan, Rawaiz, Jamal, Syed Babar, alotaibi, Dalal, Bano, Bushra, Jamila, Nargis, Naeem, Muhammad, alrahlah, Ali, Khan, Muhammad Umar Aslam, Haider, Adnan, and Khan, Naeem

Subjects

COMPOSITE coating, FILTER paper, RHO factor, ESCHERICHIA coli, CHITOSAN, PENICILLIN-binding proteins, CLINDAMYCIN, POLYCAPROLACTONE

Abstract

Wounds often develop infections caused by microbes. Preventing these microbes from causing infection is essential for wound healing. The current study therefore focuses on the preparation of an Fp (cellulose) scaffold coated with antimicrobial clindamycin drug (Cl) and chitosan (Cs) for use in wound dressings. Fp was used as a control. Before testing the efficacy of ClCFp scaffolds against bacterial strains and evaluating their cytocompatibility, they were thoroughly characterized using microscopic, spectroscopic, BET, and X-ray techniques. These methods confirmed coating of Cs and Cl drug on Fp. No significant structural damage to the Fp was observed. The porosity and surface area were found to decrease with coating. Invitro studies with HGF cells showed that the cells not only adhered to the scaffolds and proliferated, but also exhibited good viability. The results of the antibacterial tests showed that ClCFp scaffold was effective against both E. coli, "gram-negative" bacteria, and S. aureus, "gram-positive bacteria". Docking studies performed for the transcription termination factor Rho of E. coli and penicillin-binding protein 2 of S. aureus against the Cl drug confirmed the interaction between the Cl drug and bacterial proteins. Therefore, the ClCFp composite scaffolds have good prospects for biomedical applications and especially for wound dressings. [ABSTRACT FROM AUTHOR]

Published

2022

45. Multiple synergistic antibacterial melamine-impregnated paper based on nano Ag-doped ZIF-8.

Author

He, Jinrong, Qu, Wei, Feng, Yun, Jiang, Jinrui, Luo, Jiaming, Wu, Yuzhang, and Peng, Limin

Subjects

*MELAMINE, *SURFACE plasmon resonance, *DOPING agents (Chemistry), *ESCHERICHIA coli, *ION exchange (Chemistry), *EXCHANGE reactions

Abstract

[Display omitted] • A simple synthesis method has been developed for Ag@ZIF-8, involving controlling the loading and size of Ag NPs. • Ag@ZIF-8 meet the requirements for antibacterial agent used in the melamine-impregnated paper. • The multiple synergistic antibacterial mechanism of Ag@ZIF-8 was verified. • The decorated blockboards with 0.20 wt% Ag@ZIF-8 reached Level Ⅰ antibacterial grade. Melamine-impregnated paper, a decorative material in furniture and interior design, could potentially impede the spread of indoor bacteria if it possesses antibacterial properties. Here, nano Ag-doped ZIF-8 (Ag@ZIF-8) was synthesized using ion exchange and in-situ chemical reduction strategies, followed by incorporating it into melamine-impregnated paper. The ion exchange mechanism of Zn2+ and Ag+ during ion exchange reactions was investigated. The structure of Ag@ZIF-8 was well-defined, with Ag nanoparticles evenly distributed on the surface of ZIF-8. Ag@ZIF-8 showed good thermal stability at 400 °C, meeting the requirements for the hot-pressing process of the melamine-impregnated paper. Ag@ZIF-8 exhibited enhanced ROS generation under visible light compare to ZIF-8, which was attributed to its reinforced light absorption and charge carrier separation facilitated by the localized surface plasmon resonance (LSPR) effect. The antibacterial activity of Ag@ZIF-8 was better than ZIF-8, owing to the multiple-synergistic antibacterial mechanisms of the ion release and ROS generation. Specifically, the 10-Ag@ZIF-8 exhibited MIC of 128 μg/mL and 64 μg/mL against E. coli and S. aureus , respectively. The signal intensity of •O 2 − induced by 10-Ag@ZIF-8 was 4.38 times higher than that of ZIF-8. As the addition of Ag@ZIF-8 increased, the antibacterial performance of melamine-impregnated paper improved. Considering the antibacterial property and economy of melamine-impregnated paper, 0.20 wt% was the optimal amount for 10-Ag@ZIF-8 decorated blockboard. This study proposes a novel approach for synthesizing MOF-based melamine-impregnated paper with antibacterial properties, aiming to reduce bacterial spread, minimize disease risks, and contribute to lowering overall healthcare costs. [ABSTRACT FROM AUTHOR]

Published

2024

46. Fabrication of Paper Sheets Coatings Based on Chitosan/Bacterial Nanocellulose/ZnO with Enhanced Antibacterial and Mechanical Properties

Author

Rafał Rakoczy, Magdalena Onyszko, Ewa Mijowska, Adrian Augustyniak, Maciej Konopacki, and Joanna Jabłońska

Subjects

Nanofibers, Nanoparticle, Metal Nanoparticles, biopolymers, 02 engineering and technology, 01 natural sciences, Nanocellulose, Nanocomposites, Chitosan, chemistry.chemical_compound, Anti-Infective Agents, X-Ray Diffraction, Product Packaging, Biology (General), automotive_engineering, Spectroscopy, Antibacterial Response, General Medicine, 021001 nanoscience & nanotechnology, Computer Science Applications, Chemistry, Bacterial cellulose, ddc:540, Zinc Oxide, 0210 nano-technology, Materials science, Fabrication, Surface Properties, QH301-705.5, 010402 general chemistry, Catalysis, Article, Inorganic Chemistry, Microscopy, Electron, Transmission, Tensile Strength, Ultimate tensile strength, paper packaging, Escherichia coli, Physical and Theoretical Chemistry, Cellulose, Molecular Biology, QD1-999, antimicrobial activity, Organic Chemistry, 0104 chemical sciences, chemistry, Chemical engineering, Nanofiber, Mechanical Tests, Microscopy, Electron, Scanning, nanoparticles

Abstract

Here, we designed the composition of the coating of the paper sheets composed of chitosan, bacterial cellulose (nanofibres), and ZnO with boosted antibacterial and mechanical activity. We investigated the compositions with ZnO exhibiting two different sizes/shapes: (1) rods and (2) irregular sphere-like particles. The proposed processing of bacterial cellulose resulted in the formation of nanofibers. Antimicrobial behavior was tested using E. coli ATCC® 25922™ following ASTM E2149-13a standard. Mechanical properties of the paper sheets were measured by comparison of tearing resistance, tensile strength, and bursting strength according to ISO 5270 standard. The increased antibacterial response is assigned to the combination of chitosan and ZnO (independently of its shape and size), while the boosted mechanical behavior is due to bacterial cellulose nanofibers. Therefore, the proposed composition is an interesting multifunctional mixture for coatings in food packaging applications.

Published

2021

47. Turntable Paper-Based Device to Detect Escherichia coli

Author

Ching Fen Shen, Yi Chen Fu, Yung Chih Wang, Chen Yu Sang, Yi Tzu Lee, Chao-Min Cheng, Ming Yao He, and Yao Hung Tsai

Subjects

Computer science, lcsh:Mechanical engineering and machinery, medicine.disease_cause, 01 natural sciences, Article, 03 medical and health sciences, medicine, Escherichia coli, lcsh:TJ1-1570, Electrical and Electronic Engineering, 030304 developmental biology, Point of care, 0303 health sciences, turntable, business.industry, Mechanical Engineering, 010401 analytical chemistry, Paper based, 0104 chemical sciences, Control and Systems Engineering, point-of-care, business, Computer hardware, paper-based ELISA

Abstract

Escherichia coli has been known to cause a variety of infectious diseases. The conventional enzyme-linked immunosorbent assay (ELISA) is a well-known method widely used to diagnose a variety of infectious diseases. This method is expensive and requires considerable time and effort to conduct and complete multiple integral steps. We previously proposed the use of paper-based ELISA to rapidly detect the presence of E. coli. This approach has demonstrated utility for point-of-care (POC) urinary tract infection diagnoses. Paper-based ELISA, while advantageous, still requires the execution of several procedural steps. Here, we discuss the design and experimental implementation of a turntable paper-based device to simplify the paper-based ELISA protocols for the detection of E. coli. In this process, antibodies or reagents are preloaded onto zones of a paper-based device and allowed to dry before use. We successfully used this device to detect E. coli with a detection limit of 105 colony-forming units (colony-forming unit [CFU])/mL.

Published

2021

48. Characterization of efficient xylanases from industrial-scale pulp and paper wastewater treatment microbiota

Author

Jia Wang, Jiawei Liang, Yonghong Li, Lingmin Tian, and Yongjun Wei

Subjects

lcsh:Biotechnology, Microorganism, lcsh:QR1-502, Biophysics, engineering.material, Biology, medicine.disease_cause, Applied Microbiology and Biotechnology, lcsh:Microbiology, Xylan, Rumen, lcsh:TP248.13-248.65, medicine, Food science, Gene, Escherichia coli, chemistry.chemical_classification, Xylanase, Pulp (paper), GH10 family, Enzyme, chemistry, Metagenomics, Pulp and paper wastewater, engineering, Metagenome, Original Article

Abstract

Xylanases are widely used enzymes in the food, textile, and paper industries. Most efficient xylanases have been identified from lignocellulose-degrading microbiota, such as the microbiota of the cow rumen and the termite hindgut. Xylanase genes from efficient pulp and paper wastewater treatment (PPWT) microbiota have been previously recovered by metagenomics, assigning most of the xylanase genes to the GH10 family. In this study, a total of 40 GH10 family xylanase genes derived from a certain PPWT microbiota were cloned and expressed in Escherichia coli BL21 (DE3). Among these xylanase genes, 14 showed xylanase activity on beechwood substrate. Two of these, PW-xyl9 and PW-xyl37, showed high activities, and were purified to evaluate their xylanase properties. Values of optimal pH and temperature for PW-xyl9 were pH 7 and 60 ℃, respectively, while those for PW-xyl37 were pH 7 and 55 ℃, respectively; their specific xylanase activities under optimal conditions were 470.1 U/mg protein and 113.7 U/mg protein, respectively. Furthermore, the Km values of PW-xyl9 and PW-xyl37 were determined as 8.02 and 18.8 g/L, respectively. The characterization of these two xylanases paves the way for potential application in future pulp and paper production and other industries, indicating that PPWT microbiota has been an undiscovered reservoir of efficient lignocellulase genes. This study demonstrates that a metagenomic approach has the potential to screen efficient xylanases of uncultured microorganisms from lignocellulose-degrading microbiota. In a similar way, other efficient lignocellulase genes might be identified from PPWT treatment microbiota in the future.

Published

2021

49. Mining, Identification, and Characterization of Three Xylanases from the Microbiota of T. fuciformis with Its Companion Strains.

Author

Lin, Yanhuan, Li, Changle, Wei, Chenxin, Lin, Hui, and Zhang, Liaoyuan

Subjects

XYLANASES, ESCHERICHIA coli, POST-translational modification, MOLECULAR cloning, PAPER industry, AGRICULTURAL development

Abstract

Microbial xylanase has wide application in bioenergy, animal feed, environmental protection, the pulp and paper industry, and agricultural development. In this study, three xylanases from the microbiota of T. fuciformis with its companion strains were identified by metagenomics sequencing. The three enzymes were subjected to cloning and expression in E. coli or P. pastoris, purification, and characterization for their properties. The results showed that AsXyn1, from Annulohypoxylon stygium, among the three enzymes possessed high thermostability at 40 °C and broad pH tolerance in the range of 2.0–10.0, exhibiting its application potential. Furthermore, it was found that post-translational modification (such as glycosylation) of AsXyn1 enzyme modulated its activity, kinetic parameters, and thermostability. These results and findings provided a hint for enzyme modification and design in future. [ABSTRACT FROM AUTHOR]

Published

2024

50. Persistence of Salmonella and E. coli on the surface of restaurant menus.

Author

Sirsat SA, Choi JK, Almanza BA, and Neal JA

Subjects

Adult, Bacterial Load, Escherichia coli isolation & purification, Foodborne Diseases microbiology, Humans, Middle Aged, Paper, Plastics, Salmonella isolation & purification, Texas, Time Factors, Escherichia coli growth & development, Fomites microbiology, Food Microbiology, Foodborne Diseases prevention & control, Restaurants, Salmonella growth & development

Abstract

To the authors' knowledge, the role of restaurant menus as a vehicle for pathogens has not been explored. Menus, however, can pose as a vector for bacterial contamination and transfer. Sampling menus from two restaurants in the Houston, Texas, area showed the presence of up to 100 CFU/cm2 aerobic bacteria. Follow-up studies designed to investigate the ability of Salmonella and E. coli to persist on paper and laminated menus at various time points (0, 6, 24, 48, and 72 hours) demonstrated that bacteria persist more efficiently on laminated menus as compared to paper menus. Transfer studies performed to quantitatively determine the ability of bacteria to transfer from menus to fingertips and from fingertips to clean menus showed that bacteria can be transferred for up to 24 hours. The study described here showed that restaurant menus may serve as vehicles for pathogens and hence present a public health issue within the retail food environment.

Published

2013