Your search keyword '"Bacteriophages chemistry"' showing total 858 results

1. Phage LysSA163-CBD mediated specific recognition coupled with ATP bioluminescence for the sensitive detection of viable Staphylococcus aureus in food matrices.

Author

Guan P, Li R, Ding Y, Huang C, Wang J, Pan H, Shao Y, and Wang X

Subjects

Animals, Limit of Detection, Endopeptidases chemistry, Endopeptidases metabolism, Milk microbiology, Milk chemistry, Bacteriophages chemistry, Food Contamination analysis, Staphylococcus aureus isolation & purification, Adenosine Triphosphate metabolism, Luminescent Measurements methods, Food Microbiology methods

Abstract

Background: Staphylococcus aureus is a significant foodborne pathogen, commonly detected in milk and meat products. Conventional detection methods have limited sensitivity and specificity, which are time-consuming and susceptible to background interference from complex samples, and cannot effectively distinguish live and dead bacteria., Results: Herein, we developed a novel adenosine triphosphate (ATP) bioluminescence method coupled with magnetic separation, which is based on phage-encoded endolysin LysSA163-CBD (CBD 163) for rapid and specific detection of viable Staphylococcus aureus. The expressed protein (CBD 163) was derived from the phage LSA2301 and was successfully expressed in Escherichia coli BL21 following an induction period of 4 h at 37 °C, with a molecular weight approximating 40 kDa. The optimal conditions for CBD-magnetic beads (cMBs) to capture S. aureus cells were determined to be 100 μL/mL cMBs at 25 °C for 30 min. The viable S. aureus cells were disrupted by the Cetyl trimethyl ammonium bromide (CTAB) to release intracellular ATP. Then, the ATP reacted with the firefly luciferase and D-Luciferin-based bioluminescence (BL) reagents solution to generate intensive BL signal. The CBD-magnetic separation-ATP bioluminescence (cMS-BL) assay was able to quickly detect viable S. aureus via ATP bioluminescence in 45 min, with a detection range from 5 × 10 3 to 5 × 10 7  CFU/mL and limit of detection (LOD) of 190 CFU/mL. Additionally, the cMS-BL method exhibited high specificity and anti-interference ability, which has been successfully applied to quantify S. aureus cells in crayfish-tail, chicken, and skim milk., Significance and Novelty: These results demonstrate the potential of CBD 163 as a versatile and robust biorecognition element for rapid and specific detection of viable S. aureus in food matrices. The proposed phage-derived bacteria-binding proteins-based protocol for BL detection shows various advantages, including high sensitivity, simple operation, and the capability to distinguish live bacteria, providing a strategy for designing high-quality biorecognition element toward foodborne pathogens., Competing Interests: Declaration of competing interest The authors 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

2. Formulation of three tailed bacteriophages by spray-drying and atomic layer deposition for thermal stability and controlled release.

Author

Coleman HJ, Yang Q, Robert A, Padgette H, Funke HH, Catalano CE, and Randolph TW

Subjects

Spray Drying, Anti-Bacterial Agents chemistry, Anti-Bacterial Agents administration & dosage, Anti-Bacterial Agents pharmacology, Bone Cements chemistry, Phage Therapy methods, Drug Compounding methods, Temperature, Delayed-Action Preparations chemistry, Bacteriophages chemistry, Bacteriophages physiology

Abstract

Deep infection is the second most common complication of arthroplasty following loosening of the implant. Antibiotic-loaded bone cements (ALBCs) and high concentrations of systemic broad-spectrum antibiotics are commonly used to prevent infections following injury and surgery. However, clinical data fails to show that ALBCs are effective against deep infection, and negative side effects can result following prolonged administration of antibiotics. Additionally, the rise of multidrug resistant (MDR) bacteria provides an urgent need for alternatives to broad-spectrum antibiotics. Phage therapy, or the use of bacteriophages (viruses that infect bacteria) to target pathogenic bacteria, might offer a safe alternative to combat MDR bacteria. Application of phage therapy in the setting of deep infections requires formulation strategies that would stabilize bacteriophage against chemical and thermal stress during bone-cement polymerization, that maintain bacteriophage activity for weeks or months at physiological temperatures, and that allow for sustained release of phage to combat slow-growing, persistent bacteria. Here, we demonstrate the formulation of three phages that target diverse bacterial pathogens, which includes spray-drying of the particles for enhanced thermal stability at 37 °C and above. Additionally, we use atomic layer deposition (ALD) to coat spray-dried powders with alumina to allow for delayed release of phage from the dry formulations, and potentially protect phage against chemical damage during bone cement polymerization. Together, these findings present a strategy to formulate phages that possess thermal stability and sustained release properties for use in deep infections., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: The University of Colorado has licensed intellectual property related to thermal stabilization and ALD coatings of vaccines to VitriVax, Inc., a company in which the Regents of the University of Colorado and TWR hold equity., (Copyright © 2024 American Pharmacists Association. Published by Elsevier Inc. All rights reserved.)

Published

2024

3. Formulation of Dual-Functional Nonionic Cetomacrogol Creams Incorporated with Bacteriophage and Human Platelet Lysate for Effective Targeting of MDR P. aeruginosa and Enhanced Wound Healing.

Author

Mary AS, Muthuchamy M, Thillaichidambaram M, Lee S, Sivaraj B, Magar S, Ghosh S, Roy CL, Sundaresan S, Kannan M, Govindarajan S, Cho WS, and Rajaram K

Subjects

Humans, Anti-Bacterial Agents chemistry, Anti-Bacterial Agents pharmacology, Animals, Particle Size, Polyethylene Glycols chemistry, Microbial Sensitivity Tests, Rats, Wound Healing drug effects, Pseudomonas aeruginosa drug effects, Pseudomonas aeruginosa virology, Blood Platelets, Materials Testing, Bacteriophages chemistry, Biocompatible Materials chemistry, Biocompatible Materials pharmacology

Abstract

Successful development of phage-based therapeutics and their utility predominantly depend on the mode and route of phage administration. Topical and site-directed phage application evokes minimal immune clearance and allows more phage-host adsorption, thereby ensuring higher phage efficacy. However, a notable drawback of conventional topical phage applications is the absence of sustained release. Occlusive emollients guarantee the controlled release of active pharmaceutical ingredients (APIs), thereby facilitating administration, preventing moisture loss, and acting as a skin barrier. In this study, we developed phage and human platelet lysate (h-PL) incorporated cetomacrogol-based creams for combined phage therapy and wound healing. The base material for phage immobilization was formulated by emulsifying paraffin and sterile water with cetomacrogol (emulsifying agent). Specifically, we incorporated a Pseudomonas aeruginosa -infecting lytic phage vB_PaeM_M12PA in the formulation and characterized its genome in this study. Cetomacrogol, a nonionic PEG (polyethylene glycol) based ether, rendered phage stability and allowed initial burst release followed by continuous controlled release of phages from the embedding matrix in the initial 6-8 h. Rheological studies showed that the material has elastic properties with storage moduli ( G ') values ranging from 109.51 ± 2.10 to 126.02 ± 3.13 kPa, indicating frequency-independent deformation. Platelet lysates in the cream acted as wound healing agents, and in vitro evaluation of cell migration and wound healing capacity of h-PL showed a significant enhancement by the sixth hour compared to untreated groups. The phage-incorporated cream showed sustained phage release in solid media and a significant reduction in bacterial growth in liquid cultures. In vivo wound healing studies in 6-week-old Wistar rats with full-thickness excision wounds and subsequent histopathological studies showed that the formulation enhanced wound healing and tissue restoration efficiency. In conclusion, the study unveils a promising approach for integrated phage therapy and wound healing strategies.

Published

2024

4. In vivo safety evaluation and tracing of arginylglycylaspartic acid-engineered phage nanofiber in murine model.

Author

Shrestha KR, Kim S, Jo A, Ragothaman M, and Yoo SY

Subjects

Animals, Mice, Bacteriophages chemistry, Female, Nanofibers chemistry

Abstract

The engineered phage YSY184, mimicking the extracellular matrix nanofiber, effectively promotes stem cell differentiation and angiogenesis. This study evaluated its safety in a mouse model, monitoring weight, immunogenicity, spleen immune responses, and macrophage infiltration. Rapid clearance of YSY184 was observed, with peak tissue presence within three hours, significantly reduced by 24 hours, and negligible after one month. No adverse physiological or pathological effects were detected post-administration, affirming YSY184's safety and underscore its potential for therapeutic use, warranting further clinical exploration.

Published

2024

5. Phage-Modified Clear Hydrogel for Simultaneous Detection of Multiple Bacteria.

Author

Cao C, Yu Q, Yu Z, Tang K, and Gan N

Subjects

Luminescent Measurements, Food Microbiology methods, Adenosine Triphosphate analysis, Limit of Detection, Hydrogels chemistry, Bacteriophages chemistry, Escherichia coli isolation & purification, Escherichia coli virology, Escherichia coli chemistry

Abstract

The proliferation speed of live foodborne pathogens is fast. A small number of pathogens will have a great impact on food and the environment if positive samples are not detected timely. In this study, transparent porous hydrogel stir bars, modified by two different phages (corresponding to two different bacteria ( Escherichia coli and Hafnia sp )), have been developed for rapid detection of foodborne bacteria. A large number of samples can be analyzed simultaneously with a small animal live imager device to screen out the positive samples, while an adenosine triphosphate (ATP) bioluminescence sensor can be used to quantify the number of bacteria in the positive samples. The phage has good specificity and capture ability to bacteria, which makes the method highly sensitive. In addition, the use of multiple phages also enables the method to detect multiple bacteria simultaneously. The three-dimensional structure of the hydrogel allows it to modify more phages, and its transparent nature also allows the inside bioluminescence to be detected. Both can enhance the sensitivity of the detection. Finally, the reagents needed for bioluminescence, such as d-luciferin, can also be preencapsulated in the hydrogel, thus simplifying the detection step. Under the best conditions, the detection range of the method is 10 2 -10 8 CFU·mL -1 , and the limit of detection is 30 CFU·mL -1 within 11 min. The test results of actual samples show that there is no difference between using the method developed through this study and the traditional plate counting method, but the detection time is greatly shortened.

Published

2024

6. The Hydrophobic Stabilization of Pseudomonas aeruginosa Bacteriophage F8 and the Influence of Modified Bacteriophage Preparation on Biofilm Degradation.

Author

Szermer-Olearnik B, Filik-Matyjaszczyk K, Ciekot J, and Czarny A

Subjects

1-Octanol chemistry, Myoviridae physiology, Myoviridae chemistry, Bacteriophages physiology, Bacteriophages chemistry, Pseudomonas aeruginosa virology, Biofilms growth & development, Pseudomonas Phages physiology, Hydrophobic and Hydrophilic Interactions

Abstract

The bacteriophage F8 belongs to the Myoviridae group of phages and is a pathogen of Pseudomonas aeruginosa. Since Pseudomonas aeruginosa is a multidrug-resistant opportunistic bacterium and can cause serious challenges for health services, studying the potential use of phages against them is a promising approach. Pseudomonas aeruginosa can be found on medical devices because bacteria can attach to surfaces and develop biofilms, which are difficult to eradicate because of their high resistance to environmental conditions and antimicrobial therapeutics. Phage therapy is becoming promising as an alternative for the treatment of antibiotic-resistant infections, but there is still a lack of standardized protocols approved by health organizations for possible use in the clinic. In our research, we focused on the potential use of 1-octanol, which was previously used by our team to develop a method for phage purification from bacterial lysate. 1-octanol is a fatty alcohol that is mostly used in the cosmetics industry, and its advantage is that it is approved by the FDA as a food additive. In this paper, we studied the protective properties of the addition of 1-octanol for storing phage liquid preparations. We demonstrated the stabilization effect of 1-octanol addition on F8 bacteriophage preparation during storage under various conditions. Interestingly, more effective biofilm reduction was observed after treatment with the purified bacteriophage and with 1-octanol addition compared to crude lysate., (© 2024. The Author(s).)

Published

2024

7. Engineering the bacteriophage 80 alpha endolysin as a fast and ultrasensitive detection toolbox against Staphylococcus aureus.

Author

Zhao F, Yang Y, Zhan W, Li Z, Yin H, Deng J, Li W, Li R, Zhao Q, and Li J

Subjects

Bacteriophages chemistry, Bacteriophages genetics, Bacteriophages isolation & purification, Humans, Staphylococcus Phages genetics, Staphylococcus Phages chemistry, Staphylococcus Phages isolation & purification, Animals, Nucleic Acid Amplification Techniques methods, Staphylococcal Infections microbiology, DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Micrococcal Nuclease chemistry, Micrococcal Nuclease metabolism, Micrococcal Nuclease genetics, Viral Proteins chemistry, Viral Proteins metabolism, Staphylococcus aureus isolation & purification, Staphylococcus aureus virology, Biosensing Techniques methods, Endopeptidases chemistry, Endopeptidases isolation & purification, Endopeptidases genetics

Abstract

The isolation and identification of pathogenic bacteria from a variety of samples are critical for controlling bacterial infection-related health problems. The conventional methods, such as plate counting and polymerase chain reaction-based approaches, tend to be time-consuming and reliant on specific instruments, severely limiting the effective identification of these pathogens. In this study, we employed the specificity of the cell wall-binding (CBD) domain of the Staphylococcus aureus bacteriophage 80 alpha (80α) endolysin towards the host bacteria for isolation. Amidase 3-CBD conjugated magnetic beads successfully isolated as few as 1 × 10 2  CFU/mL of S. aureus cells from milk, blood, and saliva. The cell wall hydrolyzing activity of 80α endolysin promoted the genomic DNA extraction efficiency by 12.7 folds on average, compared to the commercial bacterial genomic DNA extraction kit. Then, recombinase polymerase amplification (RPA) was exploited to amplify the nuc gene of S. aureus from the extracted DNA at 37 °C for 30 min. The RPA product activated Cas12a endonuclease activity to cleave fluorescently labeled ssDNA probes. We then converted the generated signal into a fluorescent readout, detectable by either the naked eye or a portable, self-assembled instrument with ultrasensitivity. The entire procedure, from isolation to identification, can be completed within 2 h. The simplicity and sensitivity of the method developed in this study make it of great application value in S. aureus detection, especially in areas with limited resource supply., Competing Interests: Declaration of competing interest The authors 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

8. An electrochemical biosensor for sensitive detection of live Salmonella in food via MXene amplified methylene blue signals and electrostatic immobilization of bacteriophages.

Author

Deng T, Wu W, Zhou J, Zeng Q, Wang H, and Deng C

Subjects

Bacteriophages chemistry, Electrodes, Food Contamination analysis, Nanostructures chemistry, Biosensing Techniques methods, Electrochemical Techniques methods, Limit of Detection, Salmonella isolation & purification, Salmonella virology, Food Microbiology methods, Static Electricity, Methylene Blue chemistry

Abstract

A novel bacteriophage-targeted electrochemical biosensor designed for accurate and quantitative detection of live Salmonella in food samples is presented. The biosensor is simply constructed by electrostatic immobilizing bacteriophages on MXene-nanostructured electrodes. MXene, renowned for its high surface area, biocompatibility, and conductivity, serves as an ideal platform for bacteriophage immobilization. This allows for a high-density immobilization of bacteriophage particles, achieving approximately 71 pcs μm -2 . Remarkably, the bacteriophages immobilized MXene nanostructured electrodes still maintain their viability and functionality, ensuring their effectiveness in pathogen detection. Therefore, the proposed biosensor exhibited enhanced sensitivity with a low limit of detection (LOD) of 5 CFU mL -1 . Notably, the biosensor shows excellent specificity in the presence of other bacteria that commonly contaminate food and can distinguish live Salmonella from a mixed population. Furthermore, it is applicable in detecting live Salmonella in food samples, which highlights its potential in food safety monitoring. This biosensor offers simplicity, convenience, and suitability for resource-limited environments, making it a promising tool for on-site monitoring of foodborne pathogenic bacteria., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Austria, part of Springer Nature.)

Published

2024

9. Structural basis of phage transcriptional regulation.

Author

He C, He G, and Feng Y

Subjects

Crystallography, X-Ray, Gene Expression Regulation, Viral, Models, Molecular, Protein Binding, Bacteriophages metabolism, Bacteriophages genetics, Bacteriophages chemistry, Transcription, Genetic, Cryoelectron Microscopy, Viral Proteins metabolism, Viral Proteins chemistry, Viral Proteins genetics, DNA-Directed RNA Polymerases metabolism, DNA-Directed RNA Polymerases chemistry

Abstract

Phages are the most prevalent and diverse entities in the biosphere and represent the simplest systems that are capable of self-replication. Many fundamental concepts of transcriptional regulation were revealed through phage studies. The replication of phages within bacteria entails the hijacking of the host transcription machinery. Typically, this is accomplished through proteins and RNAs encoded by the phage genome that bind to the host RNA polymerase and modify its characteristics. Understanding these processes offers valuable insights into the mechanisms of bacterial transcription itself. Historically, X-ray crystallography has been the major tool for elucidating the structural basis of phage transcriptional regulation. In recent years, the application of cryoelectron microscopy has not only allowed the exploration of protein-protein and protein-nucleic acid interactions at near-atomic resolution but also captured transient intermediate states, further expanding our mechanistic understanding of phage transcriptional regulation., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2024 Elsevier Inc. All rights reserved.)

Published

2024

10. Capsid structure of bacteriophage ΦKZ provides insights into assembly and stabilization of jumbo phages.

Author

Yang Y, Shao Q, Guo M, Han L, Zhao X, Wang A, Li X, Wang B, Pan JA, Chen Z, Fokine A, Sun L, and Fang Q

Subjects

Virus Assembly, Pseudomonas Phages ultrastructure, Pseudomonas Phages chemistry, Bacteriophages physiology, Bacteriophages chemistry, Bacteriophages ultrastructure, Models, Molecular, Genome, Viral, Capsid ultrastructure, Capsid chemistry, Capsid metabolism, Cryoelectron Microscopy, Capsid Proteins chemistry, Capsid Proteins metabolism, Pseudomonas aeruginosa virology

Abstract

Jumbo phages are a group of tailed bacteriophages with large genomes and capsids. As a prototype of jumbo phage, ΦKZ infects Pseudomonas aeruginosa, a multi-drug-resistant (MDR) opportunistic pathogen leading to acute or chronic infection in immunocompromised individuals. It holds potential to be used as an antimicrobial agent and as a model for uncovering basic phage biology. Although previous low-resolution structural studies have indicated that jumbo phages may have more complicated capsid structures than smaller phages such as HK97, the detailed structures and the assembly mechanism of their capsids remain largely unknown. Here, we report a 3.5-Å-resolution cryo-EM structure of the ΦKZ capsid. The structure unveiled ten minor capsid proteins, with some decorating the outer surface of the capsid and the others forming a complex network attached to the capsid's inner surface. This network seems to play roles in driving capsid assembly and capsid stabilization. Similar mechanisms of capsid assembly and stabilization are probably employed by many other jumbo viruses., (© 2024. The Author(s).)

Published

2024

11. A microfluidic chip platform based on Pt nanozyme and magnetized phage composite probes for dual-mode detecting and imaging pathogenic bacteria viability.

Author

Liu B, Cao J, Hong B, You H, Li T, Yu Z, Li D, Liang B, and Gan N

Subjects

Hydrogen Peroxide chemistry, Hydrogen Peroxide analysis, Microbial Viability, Benzidines chemistry, Bacteriophages chemistry, Colorimetry methods, Metal Nanoparticles chemistry, Platinum chemistry, Salmonella typhimurium isolation & purification, Lab-On-A-Chip Devices

Abstract

The detection of pathogen viability is critically important to evaluate its infectivity. In the study, an integrated microfluidic chip based on dual-mode analytical strategy was developed to rapidly realize detection of bacteria activity (with Salmonella typhimurium, S.T, as a model analyte). Firstly, the composite probes, including deactivated phage modified magnetic beads and nano Pt-antimicrobial peptide (AMP) which can specifically recognize Gram-negative bacteria as nanozyme were prepared. When the composite probes are introduced into the chip together with target bacteria, after enrichment, oscillating and magnetic separation, they will conjugate with S.T and produce a magnetic sandwich complex. The complex can catalyze tetramethylbenzidine (TMB)-H 2 O 2 to produce visible colorimetric signals which is correspondent to the total S.T content. Simultaneously, PtNPs in the complex can produce hydroxyl radical oxidation (∙OH) by decomposing H 2 O 2 . Under the synergistic action of ∙OH and AMP, the captured live S.T can be lysed to release ATP and emit bioluminescence signals which corresponds to the live S.T concentration. Therefore, the chip can simultaneously detect and image S.T at different viability in one test. The dual-mode assay demonstrated high sensitivity (≤33 CFU/mL), high specificity (identifying strain), signal amplification (5 folds) and short time (≤40min). The chip array can detect four samples in one test and exhibited advantages of high-integration, -sensitivity, -specificity and miniaturization, which are suitable to rapidly detect and image pathogen's viability in trace level. The replacement of phage probes can detect other bacteria. It has a wide prospect in pathogens screening., Competing Interests: Declaration of competing interest The authors 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

12. Magnetically modified bacteriophage-triggered ATP release activated EXPAR-CRISPR/Cas14a system for visual detection of Burkholderia pseudomallei.

Author

Yao J, Zhang Z, Pei H, Zhang T, Ruan Y, Liu C, Guo Y, Gu S, and Xia Q

Subjects

Melioidosis microbiology, Limit of Detection, Humans, Magnetite Nanoparticles chemistry, Burkholderia pseudomallei virology, Biosensing Techniques methods, Bacteriophages chemistry, Bacteriophages isolation & purification, Adenosine Triphosphate metabolism, Adenosine Triphosphate analysis, CRISPR-Cas Systems

Abstract

Burkholderia pseudomallei, widely distributed in tropical and subtropical ecosystems, is capable of causing the fatal zoonotic disease melioidosis and exhibiting a global trend of dissemination. Rapid and sensitive detection of B. pseudomallei is essential for environmental monitoring as well as infection control. Here, we developed an innovative biosensor for quantitatively detecting B. pseudomallei relies on ATP released triggered by bacteriophage-induced bacteria lysis. The lytic bacteriophage vB_BpP_HN01, with high specificity, is employed alongside magnetic nanoparticles assembly to create a biological receptor, facilitating the capture and enrichment of viable target bacteria. Following a brief extraction and incubation process, the captured target undergoes rapid lysis to release contents including ATP. The EXPAR-CRISPR cascade reaction provides an efficient signal transduction and dual amplification module that allowing the generated ATP to guide the signal output as an activator, ultimately converting the target bacterial amount into a detectable fluorescence signal. The proposed bacteriophage affinity strategy exhibited superior performance for B. pseudomallei detection with a dynamic range from 10^2 to 10^7 CFU mL -1 , and a LOD of 45 CFU mL -1 within 80 min. Moreover, with the output signal compatible across various monitoring methods, this work offers a robust assurance for rapid diagnosis and on-site environmental monitoring of B. pseudomallei., Competing Interests: Declaration of competing interest The authors 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

13. Inhalable Polymeric Microparticles for Phage and Photothermal Synergistic Therapy of Methicillin-Resistant Staphylococcus aureus Pneumonia.

Author

Liu MY, Liu X, Wang CY, Wan QQ, Tian YF, Liu SL, Pang DW, and Wang ZG

Subjects

Animals, Mice, Microspheres, Photothermal Therapy, Pneumonia, Staphylococcal therapy, Phage Therapy methods, Indocyanine Green chemistry, Indocyanine Green pharmacology, Indocyanine Green therapeutic use, Indocyanine Green administration & dosage, Anti-Bacterial Agents chemistry, Anti-Bacterial Agents pharmacology, Anti-Bacterial Agents administration & dosage, Anti-Bacterial Agents therapeutic use, Administration, Inhalation, Humans, Bacteriophages chemistry, Methicillin-Resistant Staphylococcus aureus drug effects, Polylactic Acid-Polyglycolic Acid Copolymer chemistry

Abstract

Acute methicillin-resistant Staphylococcus aureus (MRSA) pneumonia is a common and serious lung infection with high morbidity and mortality rates. Due to the increasing antibiotic resistance, toxicity, and pathogenicity of MRSA, there is an urgent need to explore effective antibacterial strategies. In this study, we developed a dry powder inhalable formulation which is composed of porous microspheres prepared from poly(lactic- co -glycolic acid) (PLGA), internally loaded with indocyanine green (ICG)-modified, heat-resistant phages that we screened for their high efficacy against MRSA. This formulation can deliver therapeutic doses of ICG-modified active phages to the deep lung tissue infection sites, avoiding rapid clearance by alveolar macrophages. Combined with the synergistic treatment of phage therapy and photothermal therapy, the formulation demonstrates potent bactericidal effects in acute MRSA pneumonia. With its long-term stability at room temperature and inhalable characteristics, this formulation has the potential to be a promising drug for the clinical treatment of MRSA pneumonia.

Published

2024

14. The Structure of Spiroplasma Virus 4 : Exploring the Capsid Diversity of the Microviridae .

Author

Mietzsch M, Kailasan S, Bennett A, Chipman P, Fane B, Huiskonen JT, Clarke IN, and McKenna R

Subjects

Bacteriophages ultrastructure, Bacteriophages genetics, Bacteriophages classification, Bacteriophages chemistry, Bacteriophages physiology, Models, Molecular, Capsid ultrastructure, Capsid metabolism, Capsid chemistry, Cryoelectron Microscopy, Capsid Proteins chemistry, Capsid Proteins metabolism, Capsid Proteins genetics, Spiroplasma ultrastructure, Microviridae genetics, Microviridae ultrastructure, Microviridae chemistry, Virion ultrastructure

Abstract

Spiroplasma virus 4 (SpV4) is a bacteriophage of the Microviridae , which packages circular ssDNA within non-enveloped T = 1 icosahedral capsids. It infects spiroplasmas, which are known pathogens of honeybees. Here, the structure of the SpV4 virion is determined using cryo-electron microscopy to a resolution of 2.5 Å. A striking feature of the SpV4 capsid is the mushroom-like protrusions at the 3-fold axes, which is common among all members of the subfamily Gokushovirinae. While the function of the protrusion is currently unknown, this feature varies widely in this subfamily and is therefore possibly an adaptation for host recognition. Furthermore, on the interior of the SpV4 capsid, the location of DNA-binding protein VP8 was identified and shown to have low structural conservation to the capsids of other viruses in the family. The structural characterization of SpV4 will aid future studies analyzing the virus-host interaction, to understand disease mechanisms at a molecular level. Furthermore, the structural comparisons in this study, including a low-resolution structure of the chlamydia phage 2, provide an overview of the structural repertoire of the viruses in this family that infect various bacterial hosts, which in turn infect a wide range of animals and plants.

Published

2024

15. You get what you test for: The killing effect of phage lysins is highly dependent on buffer tonicity and ionic strength.

Author

Vázquez R, Gutiérrez D, Dezutter Z, Criel B, de Groote P, and Briers Y

Subjects

Osmolar Concentration, Microbial Viability drug effects, Buffers, Humans, Viral Proteins genetics, Viral Proteins metabolism, Viral Proteins chemistry, Endopeptidases metabolism, Endopeptidases chemistry, Bacteriophages chemistry, Bacteriophages physiology, Bacteriophages genetics, Acinetobacter baumannii drug effects, Acinetobacter baumannii virology

Abstract

The phage lysin field has done nothing but grow in the last decades. As a result, many different research groups around the world are contributing to the field, often with certain methodological differences that pose a challenge to the interpretation and comparison of results. In this work, we present the case study of three Acinetobacter baumannii-targeting phage lysins (wild-type endolysin LysMK34 plus engineered lysins eLysMK34 and 1D10) plus one lysin with broad activity against Gram-positive bacteria (PlySs2) to provide exemplary evidence on the risks of generalization when using one of the most common lysin evaluation assays: the killing assay with resting cells. To that end, we performed killing assays with the aforementioned lysins using hypo-, iso- and hypertonic buffers plus human serum either as the reaction or the dilution medium in a systematic manner. Our findings stress the perils of creating hypotonic conditions or a hypotonic shock during a killing assay, suggesting that hypotonic buffers should be avoided as a test environment or as diluents before plating to avoid overestimation of the killing effect in the assayed conditions. As a conclusion, we suggest that the nature of both the incubation and the dilution buffers should be always clearly identified when reporting killing activity data, and that for experimental consistency the same incubation buffer should be used as a diluent for posterior serial dilution and plating unless explicitly required by the experimental design. In addition, the most appropriate buffer mimicking the final application must be chosen to obtain relevant results., (© 2024 The Author(s). Microbial Biotechnology published by John Wiley & Sons Ltd.)

Published

2024

16. Bacteria conjugate ubiquitin-like proteins to interfere with phage assembly.

Author

Hör J, Wolf SG, and Sorek R

Subjects

Ubiquitin-Activating Enzymes metabolism, Viral Tail Proteins metabolism, Viral Tail Proteins chemistry, Evolution, Molecular, Conserved Sequence, Bacteriophages chemistry, Bacteriophages metabolism, Bacteriophages pathogenicity, Bacteriophages physiology, Deubiquitinating Enzymes metabolism, Escherichia coli enzymology, Escherichia coli metabolism, Escherichia coli virology, Ubiquitin-Conjugating Enzymes metabolism, Ubiquitins metabolism, Bacterial Proteins metabolism, Virus Assembly

Abstract

Several immune pathways in humans conjugate ubiquitin-like proteins to virus and host molecules as a means of antiviral defence 1-5 . Here we studied an antiphage defence system in bacteria, comprising a ubiquitin-like protein, ubiquitin-conjugating enzymes E1 and E2, and a deubiquitinase. We show that during phage infection, this system specifically conjugates the ubiquitin-like protein to the phage central tail fibre, a protein at the tip of the tail that is essential for tail assembly as well as for recognition of the target host receptor. Following infection, cells encoding this defence system release a mixture of partially assembled, tailless phage particles and fully assembled phages in which the central tail fibre is obstructed by the covalently attached ubiquitin-like protein. These phages show severely impaired infectivity, explaining how the defence system protects the bacterial population from the spread of phage infection. Our findings demonstrate that conjugation of ubiquitin-like proteins is an antiviral strategy conserved across the tree of life., (© 2024. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2024

17. Phage anti-CRISPR control by an RNA- and DNA-binding helix-turn-helix protein.

Author

Birkholz N, Kamata K, Feussner M, Wilkinson ME, Cuba Samaniego C, Migur A, Kimanius D, Ceelen M, Went SC, Usher B, Blower TR, Brown CM, Beisel CL, Weinberg Z, Fagerlund RD, Jackson SA, and Fineran PC

Subjects

Binding Sites, Clustered Regularly Interspaced Short Palindromic Repeats genetics, CRISPR-Associated Proteins metabolism, Cryoelectron Microscopy, Genes, Viral, Models, Molecular, Nucleic Acid Conformation, Pectobacterium carotovorum virology, Protein Biosynthesis genetics, Protein Domains, Ribosomes metabolism, RNA, Messenger chemistry, RNA, Messenger genetics, RNA, Messenger metabolism, RNA, Messenger ultrastructure, RNA, Viral chemistry, RNA, Viral genetics, RNA, Viral metabolism, RNA, Viral ultrastructure, Substrate Specificity, Transcription, Genetic, Bacteriophages chemistry, Bacteriophages genetics, Bacteriophages metabolism, Bacteriophages ultrastructure, CRISPR-Cas Systems, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, DNA-Binding Proteins ultrastructure, Gene Expression Regulation, Viral, Helix-Turn-Helix Motifs, RNA-Binding Proteins chemistry, RNA-Binding Proteins genetics, RNA-Binding Proteins metabolism, RNA-Binding Proteins ultrastructure, Viral Proteins chemistry, Viral Proteins genetics, Viral Proteins metabolism, Viral Proteins ultrastructure

Abstract

In all organisms, regulation of gene expression must be adjusted to meet cellular requirements and frequently involves helix-turn-helix (HTH) domain proteins 1 . For instance, in the arms race between bacteria and bacteriophages, rapid expression of phage anti-CRISPR (acr) genes upon infection enables evasion from CRISPR-Cas defence; transcription is then repressed by an HTH-domain-containing anti-CRISPR-associated (Aca) protein, probably to reduce fitness costs from excessive expression 2-5 . However, how a single HTH regulator adjusts anti-CRISPR production to cope with increasing phage genome copies and accumulating acr mRNA is unknown. Here we show that the HTH domain of the regulator Aca2, in addition to repressing Acr synthesis transcriptionally through DNA binding, inhibits translation of mRNAs by binding conserved RNA stem-loops and blocking ribosome access. The cryo-electron microscopy structure of the approximately 40 kDa Aca2-RNA complex demonstrates how the versatile HTH domain specifically discriminates RNA from DNA binding sites. These combined regulatory modes are widespread in the Aca2 family and facilitate CRISPR-Cas inhibition in the face of rapid phage DNA replication without toxic acr overexpression. Given the ubiquity of HTH-domain-containing proteins, it is anticipated that many more of them elicit regulatory control by dual DNA and RNA binding., (© 2024. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2024

18. Bacteriophage-Based Bioanalysis.

Author

Parker DR and Nugen SR

Subjects

Bacteria virology, Genetic Engineering, Bacteriophages chemistry, Biosensing Techniques methods

Abstract

Bacteriophages, which are viral predators of bacteria, have evolved to efficiently recognize, bind, infect, and lyse their host, resulting in the release of tens to hundreds of propagated viruses. These abilities have attracted biosensor developers who have developed new methods to detect bacteria. Recently, several comprehensive reviews have covered many of the advances made regarding the performance of phage-based biosensors. Therefore, in this review, we first describe the landscape of phage-based biosensors and then cover advances in other aspects of phage biology and engineering that can be used to make high-impact contributions to biosensor development. Many of these advances are in fields adjacent to analytical chemistry such as synthetic biology, machine learning, and genetic engineering and will allow those looking to develop phage-based biosensors to start taking alternative approaches, such as a bottom-up design and synthesis of custom phages with the singular task of detecting their host.

Published

2024

19. A eukaryotic-like ubiquitination system in bacterial antiviral defence.

Author

Chambers LR, Ye Q, Cai J, Gong M, Ledvina HE, Zhou H, Whiteley AT, Suhandynata RT, and Corbett KD

Subjects

Catalytic Domain, Crystallography, X-Ray, Cysteine chemistry, Cysteine metabolism, Deubiquitinating Enzymes chemistry, Deubiquitinating Enzymes metabolism, Evolution, Molecular, Lysine chemistry, Lysine metabolism, Models, Molecular, Operon genetics, Protein Domains, Eukaryota enzymology, Eukaryota metabolism, Bacterial Proteins metabolism, Bacterial Proteins chemistry, Bacteriophages chemistry, Bacteriophages immunology, Bacteriophages metabolism, Escherichia chemistry, Escherichia enzymology, Escherichia immunology, Escherichia virology, Ubiquitin-Activating Enzymes metabolism, Ubiquitin-Activating Enzymes chemistry, Ubiquitin-Conjugating Enzymes metabolism, Ubiquitin-Conjugating Enzymes chemistry, Ubiquitination, Ubiquitins metabolism, Ubiquitins chemistry

Abstract

Ubiquitination pathways have crucial roles in protein homeostasis, signalling and innate immunity 1-3 . In these pathways, an enzymatic cascade of E1, E2 and E3 proteins conjugates ubiquitin or a ubiquitin-like protein (Ubl) to target-protein lysine residues 4 . Bacteria encode ancient relatives of E1 and Ubl proteins involved in sulfur metabolism 5,6 , but these proteins do not mediate Ubl-target conjugation, leaving open the question of whether bacteria can perform ubiquitination-like protein conjugation. Here we demonstrate that a bacterial operon associated with phage defence islands encodes a complete ubiquitination pathway. Two structures of a bacterial E1-E2-Ubl complex reveal striking architectural parallels with canonical eukaryotic ubiquitination machinery. The bacterial E1 possesses an amino-terminal inactive adenylation domain and a carboxy-terminal active adenylation domain with a mobile α-helical insertion containing the catalytic cysteine (CYS domain). One structure reveals a pre-reaction state with the bacterial Ubl C terminus positioned for adenylation, and a second structure mimics an E1-to-E2 transthioesterification state with the E1 CYS domain adjacent to the bound E2. We show that a deubiquitinase in the same pathway preprocesses the bacterial Ubl, exposing its C-terminal glycine for adenylation. Finally, we show that the bacterial E1 and E2 collaborate to conjugate Ubl to target-protein lysine residues. Together, these data reveal that bacteria possess bona fide ubiquitination systems with strong mechanistic and architectural parallels to canonical eukaryotic ubiquitination pathways, suggesting that these pathways arose first in bacteria., (© 2024. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2024

20. Versatile Platinum Nanoparticles-Decorated Phage Nanozyme Integrating Recognition, Bacteriolysis, and Catalysis Capabilities for On-Site Detection of Foodborne Pathogenic Strains Vitality Based on Bioluminescence/Pressure Dual-Mode Bioassay.

Author

You H, Ma N, Li T, Yu Z, and Gan N

Subjects

Catalysis, Food Microbiology, Biological Assay methods, Biosensing Techniques methods, Pressure, Hydrogen Peroxide chemistry, Platinum chemistry, Metal Nanoparticles chemistry, Salmonella typhimurium isolation & purification, Salmonella typhimurium virology, Salmonella typhimurium chemistry, Luminescent Measurements, Bacteriophages chemistry

Abstract

Sensitive and on-site discrimination of live and dead foodborne pathogenic strains remains a significant challenge due to the lack of appropriate assay and signal probes. In this work, a versatile platinum nanoparticle-decorated phage nanozyme (P2@PtNPs) that integrated recognition, bacteriolysis, and catalysis was designed to establish the bioluminescence/pressure dual-mode bioassay for on-site determination of the vitality of foodborne pathogenic strains. Benefiting from the bacterial strain-level specificity of phage, the target Salmonella typhimurium (S.T) was specially captured to form sandwich complexes with P2@PtNPs on another phage-modified glass microbead (GM@P1). As the other part of the P2@PtNPs nanozyme, the introduced PtNPs could not only catalyze the decomposition of hydrogen peroxide to generate a significant oxygen pressure signal but also produce hydroxyl radicals around the target bacteria to enhance the bacteriolysis of phage and adenosine triphosphate release. It significantly improved the bioluminescence signal. The two signals corresponded to the total and live target bacteria counts, so the dead target could be easily calculated from the difference between the total and live target bacteria counts. Meanwhile, the vitality of S.T was realized according to the ratio of live and total S.T. Under optimal conditions, the application range of this proposed bioassay for bacterial vitality was 10 2 -10 7 CFU/mL, with a limit of detections for total and live S.T of 30 CFU/mL and 40 CFU/mL, respectively. This work provides an innovative and versatile nanozyme signal probe for the on-site determination of bacterial vitality for food safety.

Published

2024

21. Structural mechanisms of Tad pilus assembly and its interaction with an RNA virus.

Author

Wang Y, Theodore M, Xing Z, Narsaria U, Yu Z, Zeng L, and Zhang J

Subjects

Cryoelectron Microscopy, Fimbriae Proteins, Escherichia coli, Viral Proteins chemistry, Viral Proteins metabolism, Caulobacter crescentus cytology, Caulobacter crescentus metabolism, Caulobacter crescentus virology, Fimbriae, Bacterial metabolism, Fimbriae, Bacterial ultrastructure, Bacteriophages chemistry, Bacteriophages metabolism

Abstract

Caulobacter crescentus Tad (tight adherence) pili, part of the type IV pili family, are crucial for mechanosensing, surface adherence, bacteriophage (phage) adsorption, and cell-cycle regulation. Unlike other type IV pilins, Tad pilins lack the typical globular β sheet domain responsible for pilus assembly and phage binding. The mechanisms of Tad pilus assembly and its interaction with phage ΦCb5 have been elusive. Using cryo-electron microscopy, we unveiled the Tad pilus assembly mechanism, featuring a unique network of hydrogen bonds at its core. We then identified the Tad pilus binding to the ΦCb5 maturation protein (Mat) through its β region. Notably, the amino terminus of ΦCb5 Mat is exposed outside the capsid and phage/pilus interface, enabling the attachment of fluorescent and affinity tags. These engineered ΦCb5 virions can be efficiently assembled and purified in Escherichia coli , maintaining infectivity against C. crescentus , which presents promising applications, including RNA delivery and phage display.

Published

2024

22. The structure and physical properties of a packaged bacteriophage particle.

Author

Coshic K, Maffeo C, Winogradoff D, and Aksimentiev A

Subjects

Capsid Proteins chemistry, Capsid Proteins metabolism, Diffusion, Ions analysis, Ions chemistry, Ions metabolism, Static Electricity, Water analysis, Water chemistry, Water metabolism, Bacteriophages chemistry, Bacteriophages genetics, Bacteriophages growth & development, Bacteriophages metabolism, Capsid chemistry, Capsid metabolism, DNA, Viral chemistry, DNA, Viral genetics, DNA, Viral metabolism, Genome, Viral, Virion chemistry, Virion genetics, Virion metabolism, Virus Assembly genetics

Abstract

A string of nucleotides confined within a protein capsid contains all the instructions necessary to make a functional virus particle, a virion. Although the structure of the protein capsid is known for many virus species 1,2 , the three-dimensional organization of viral genomes has mostly eluded experimental probes 3,4 . Here we report all-atom structural models of an HK97 virion 5 , including its entire 39,732 base pair genome, obtained through multiresolution simulations. Mimicking the action of a packaging motor 6 , the genome was gradually loaded into the capsid. The structure of the packaged capsid was then refined through simulations of increasing resolution, which produced a 26 million atom model of the complete virion, including water and ions confined within the capsid. DNA packaging occurs through a loop extrusion mechanism 7 that produces globally different configurations of the packaged genome and gives each viral particle individual traits. Multiple microsecond-long all-atom simulations characterized the effect of the packaged genome on capsid structure, internal pressure, electrostatics and diffusion of water, ions and DNA, and revealed the structural imprints of the capsid onto the genome. Our approach can be generalized to obtain complete all-atom structural models of other virus species, thereby potentially revealing new drug targets at the genome-capsid interface., (© 2024. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2024

23. Activation of Thoeris antiviral system via SIR2 effector filament assembly.

Author

Tamulaitiene G, Sabonis D, Sasnauskas G, Ruksenaite A, Silanskas A, Avraham C, Ofir G, Sorek R, Zaremba M, and Siksnys V

Subjects

Adenosine Diphosphate Ribose analogs & derivatives, Adenosine Diphosphate Ribose biosynthesis, Adenosine Diphosphate Ribose chemistry, Adenosine Diphosphate Ribose metabolism, Cryoelectron Microscopy, Hydrolysis, NAD metabolism, Protein Domains, Protein Multimerization, Protein Stability, Bacteria metabolism, Bacteria virology, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Bacterial Proteins ultrastructure, Bacteriophages chemistry, Bacteriophages metabolism, Bacteriophages ultrastructure

Abstract

To survive bacteriophage (phage) infections, bacteria developed numerous anti-phage defence systems 1-7 . Some of them (for example, type III CRISPR-Cas, CBASS, Pycsar and Thoeris) consist of two modules: a sensor responsible for infection recognition and an effector that stops viral replication by destroying key cellular components 8-12 . In the Thoeris system, a Toll/interleukin-1 receptor (TIR)-domain protein, ThsB, acts as a sensor that synthesizes an isomer of cyclic ADP ribose, 1''-3' glycocyclic ADP ribose (gcADPR), which is bound in the Smf/DprA-LOG (SLOG) domain of the ThsA effector and activates the silent information regulator 2 (SIR2)-domain-mediated hydrolysis of a key cell metabolite, NAD + (refs.  12-14 ). Although the structure of ThsA has been solved 15 , the ThsA activation mechanism remained incompletely understood. Here we show that 1''-3' gcADPR, synthesized in vitro by the dimeric ThsB' protein, binds to the ThsA SLOG domain, thereby activating ThsA by triggering helical filament assembly of ThsA tetramers. The cryogenic electron microscopy (cryo-EM) structure of activated ThsA revealed that filament assembly stabilizes the active conformation of the ThsA SIR2 domain, enabling rapid NAD + depletion. Furthermore, we demonstrate that filament formation enables a switch-like response of ThsA to the 1''-3' gcADPR signal., (© 2024. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2024

24. Cryo-EM structure of a Shigella podophage reveals a hybrid tail and novel decoration proteins.

Author

Subramanian S, Bergland Drarvik SM, Tinney KR, and Parent KN

Subjects

Humans, Cryoelectron Microscopy, Capsid Proteins metabolism, Capsid chemistry, Viral Tail Proteins chemistry, Bacteriophages chemistry, Shigella metabolism

Abstract

There is a paucity of high-resolution structures of phages infecting Shigella, a human pathogen and a serious threat to global health. HRP29 is a Shigella podophage belonging to the Autographivirinae family, and has very low sequence identity to other known phages. Here, we resolved the structure of the entire HRP29 virion by cryo-EM. Phage HRP29 has a highly unusual tail that is a fusion of a T7-like tail tube and P22-like tailspikes mediated by interactions from a novel tailspike adaptor protein. Understanding phage tail structures is critical as they mediate hosts interactions. Furthermore, we show that the HRP29 capsid is stabilized by two novel, and essential decoration proteins, gp47 and gp48. Only one high resolution structure is currently available for Shigella podophages. The presence of a hybrid tail and an adapter protein suggests that it may be a product of horizontal gene transfer, and may be prevalent in other phages., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2023 Elsevier Ltd. All rights reserved.)

Published

2024

25. Design and Purification of Tag/Catcher AP205-Based Capsid Virus-Like Particle Vaccines.

Author

Aves KL and Sander AF

Subjects

Capsid Proteins genetics, Capsid, Vaccines, Virus-Like Particle genetics, Bacteriophages chemistry

Abstract

Capsid virus-like particles (cVLPs), assembled from viral coat proteins, are used as therapeutic cargo delivery vehicles as well as molecular scaffolds for display of vaccine antigens. A versatile vaccine platform has been developed based on the Acinetobacter phage AP205 cVLP, which has been shown to significantly improve antigen-specific antibody responses. This modular cVLP platform exploits a split-protein (Tag/Catcher) conjugation system to enable high-density, unidirectional antigen display. Accordingly, protein antigens can be independently expressed and quality-checked prior to conjugation to pre-assembled cVLPs. Here, we describe considerations for the design of vaccine antigens with genetically fused split-protein (Tag or Catcher) binding partners and provide protocols for the expression and purification of corresponding Tag- or Catcher-AP205 cVLPs from E.coli. Finally, we describe a generic protocol for the formulation and quality assessment of experimental/pre-clinical AP205 cVLP-based vaccines., (© 2024. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

26. Structure of the Borrelia Bacteriophage φBB1 Procapsid.

Author

Rūmnieks J, Füzik T, and Tārs K

Subjects

Capsid Proteins metabolism, Cryoelectron Microscopy, Virus Assembly, Bacteriophages chemistry, Bacteriophages genetics, Borrelia virology, Capsid chemistry

Abstract

Bacteriophages of Borrelia burgdorferi are a biologically important but under-investigated feature of the Lyme disease-causing spirochete. No virulent borrelial viruses have been identified, but all B. burgdorferi isolates carry a prophage φBB1 as resident circular plasmids. Like its host, the φBB1 phage is quite distinctive and shares little sequence similarity with other known bacteriophages. We expressed φBB1 head morphogenesis proteins in Escherichia coli which resulted in assembly of homogeneous prolate procapsid structures and used cryo-electron microscopy to determine the three-dimensional structure of these particles. The φBB1 procapsids consist of 415 copies of the major capsid protein and an equal combined number of three homologous capsid decoration proteins that form trimeric knobs on the outside of the particle. One of the end vertices of the particle is occupied by a portal assembled from twelve copies of the portal protein. The φBB1 scaffolding protein is entirely α-helical and has an elongated shape with a small globular domain in the middle. Within the tubular section of the procapsid, the internal scaffold is built of stacked rings, each composed of 32 scaffolding protein molecules, which run in opposite directions from both caps with a heterogeneous part in the middle. Inside the portal-containing cap, the scaffold is organized asymmetrically with ten scaffolding protein molecules bound to the portal. The φBB1 procapsid structure provides better insight into the vast structural diversity of bacteriophages and presents clues of how elongated bacteriophage particles might be assembled., Competing Interests: Declaration of Competing Interest The authors 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 © 2023 The Authors. Published by Elsevier Ltd.. All rights reserved.)

Published

2023

27. New role of bacteriophages in medical oncology.

Author

Moradi M, Ghaleh HEG, Bolandian M, and Dorostkar R

Subjects

Animals, Humans, Drug Delivery Systems methods, Pharmaceutical Preparations, Medical Oncology, Mammals, Bacteriophages genetics, Bacteriophages chemistry, Vaccines, Neoplasms therapy

Abstract

Targeted treatment of cancer is one of the most paramount approaches in cancer treatment. Despite significant advances in cancer diagnosis and treatment methods, there are still significant limitations and disadvantages in the field, including high costs, toxicity, and unwanted damage to healthy cells. The phage display technique is an innovative method for designing carriers containing exogenic peptides with cancer diagnostic and therapeutic properties. Bacteriophages possess unique properties making them effective in cancer treatment. These characteristics include the small size enabling them to penetrate vessels; having no pathogenicity to mammals; easy manipulation of their genetic information and surface proteins to introduce vaccines and drugs to cancer tissues; lower cost of large-scale production; and greater stimulation of the immune system. Bacteriophages will certainly play a more effective role in the future of medical oncology; however, studies are in the early stages of conception and require more extensive research. We aimed in this review to provide some related examples and bring insights into the potential of phages as targeted vectors for use in cancer diagnosis and treatment, especially regarding their capability in gene and drug delivery to cancer target cells, determination of tumor markers, and vaccine design to stimulate anticancer immunity., (© 2023 International Union of Biochemistry and Molecular Biology, Inc.)

Published

2023

28. Identification of Structural and Morphogenesis Genes of Sulfitobacter Phage ΦGT1 and Placement within the Evolutionary History of the Podoviruses.

Author

Hardies SC, Cho BC, Jang GI, Wang Z, and Hwang CY

Subjects

Prospective Studies, Genome, Viral, Prophages genetics, Bacteriophages genetics, Bacteriophages chemistry, Podoviridae genetics

Abstract

ΦGT1 is a lytic podovirus of an alphaproteobacterial Sulfitobacter species, with few closely matching sequences among characterized phages, thus defying a useful description by simple sequence clustering methods. The history of the ΦGT1 core structure module was reconstructed using timetrees, including numerous related prospective prophages, to flesh out the evolutionary lineages spanning from the origin of the ejectosomal podovirus >3.2 Gya to the present genes of ΦGT1 and its closest relatives. A peculiarity of the ΦGT1 structural proteome is that it contains two paralogous tubular tail A (tubeA) proteins. The origin of the dual tubeA arrangement was traced to a recombination between two more ancient podoviral lineages occurring ~0.7 Gya in the alphaproteobacterial order Rhizobiales . Descendants of the ancestral dual A recombinant were tracked forward forming both temperate and lytic phage clusters and exhibiting both vertical transmission with patchy persistence and horizontal transfer with respect to host taxonomy. The two ancestral lineages were traced backward, making junctions with a major metagenomic podoviral family, the LUZ24-like gammaproteobacterial phages, and Myxococcal phage Mx8, and finally joining near the origin of podoviruses with P22. With these most conservative among phage genes, deviations from uncomplicated vertical and nonrecombinant descent are numerous but countable. The use of timetrees allowed conceptualization of the phage's evolution in the context of a sequence of ancestors spanning the time of life on Earth.

Published

2023

29. Structure and proposed DNA delivery mechanism of a marine roseophage.

Author

Huang Y, Sun H, Wei S, Cai L, Liu L, Jiang Y, Xin J, Chen Z, Que Y, Kong Z, Li T, Yu H, Zhang J, Gu Y, Zheng Q, Li S, Zhang R, and Xia N

Subjects

Genome, Viral, Genes, Viral, Capsid Proteins genetics, DNA, DNA, Viral genetics, Bacteriophages genetics, Bacteriophages chemistry, Caudovirales genetics

Abstract

Tailed bacteriophages (order, Caudovirales) account for the majority of all phages. However, the long flexible tail of siphophages hinders comprehensive investigation of the mechanism of viral gene delivery. Here, we report the atomic capsid and in-situ structures of the tail machine of the marine siphophage, vB_DshS-R4C (R4C), which infects Roseobacter. The R4C virion, comprising 12 distinct structural protein components, has a unique five-fold vertex of the icosahedral capsid that allows genome delivery. The specific position and interaction pattern of the tail tube proteins determine the atypical long rigid tail of R4C, and further provide negative charge distribution within the tail tube. A ratchet mechanism assists in DNA transmission, which is initiated by an absorption device that structurally resembles the phage-like particle, RcGTA. Overall, these results provide in-depth knowledge into the intact structure and underlining DNA delivery mechanism for the ecologically important siphophages., (© 2023. The Author(s).)

Published

2023

30. Crystal structure of the engineered endolysin mtEC340M.

Author

Wang JM, Seok SH, Yoon WS, Kim JH, and Seo MD

Subjects

Crystallography, X-Ray, Endopeptidases, Anti-Bacterial Agents chemistry, Escherichia coli genetics, Peptidoglycan, Bacteriophages chemistry

Abstract

Endolysins produced by bacteriophages play essential roles in the release of phage progeny by degrading the peptidoglycan layers of the bacterial cell wall. Bacteriophage-encoded endolysins have emerged as a new class of antibacterial agents to combat surging antibiotic resistance. The crystal structure of mtEC340M, an engineered endolysin EC340 from the PBEC131 phage that infects Escherichia coli, was determined. The crystal structure of mtEC340M at 2.4 Å resolution consists of eight α-helices and two loops. The three active residues of mtEC340M were predicted by structural comparison with peptidoglycan-degrading lysozyme.

Published

2023

31. Deciphering Bacteriophage T5 Host Recognition Mechanism and Infection Trigger.

Author

Degroux S, Effantin G, Linares R, Schoehn G, and Breyton C

Subjects

Bacterial Outer Membrane Proteins chemistry, Bacterial Outer Membrane Proteins metabolism, Bacterial Outer Membrane Proteins ultrastructure, Escherichia coli virology, Protein Binding, Cryoelectron Microscopy, Viral Proteins chemistry, Viral Proteins metabolism, Viral Proteins ultrastructure, Bacteriophages chemistry, Bacteriophages metabolism, Escherichia coli Proteins chemistry

Abstract

Bacteriophages, viruses infecting bacteria, recognize their host with high specificity, binding to either saccharide motifs or proteins of the cell wall of their host. In the majority of bacteriophages, this host recognition is performed by receptor binding proteins (RBPs) located at the extremity of a tail. Interaction between the RBPs and the host is the trigger for bacteriophage infection, but the molecular details of the mechanisms are unknown for most bacteriophages. Here, we present the electron cryomicroscopy (cryo-EM) structure of bacteriophage T5 RBP pb5 in complex with its Escherichia coli receptor, the iron ferrichrome transporter FhuA. Monomeric RBP pb5 is located at the extremity of T5's long flexible tail, and its irreversible binding to FhuA commits T5 to infection. Analysis of the structure of RBP pb5 within the complex, comparison with its AlphaFold2-predicted structure, and its fit into a previously determined map of the T5 tail tip in complex with FhuA allow us to propose a mechanism of transmission of the RBP pb5 receptor binding to the straight fiber, initiating the cascade of events that commits T5 to DNA ejection. IMPORTANCE Tailed bacteriophages specifically recognize their bacterial host by interaction of their receptor binding protein(s) (RBPs) with saccharides and/or proteins located at the surface of their prey. This crucial interaction commits the virus to infection, but the molecular details of this mechanism are unknown for the majority of bacteriophages. We determined the structure of bacteriophage T5 RBP pb5 in complex with its E. coli receptor, FhuA, by cryo-EM. This first structure of an RBP bound to its protein receptor allowed us to propose a mechanism of transmission of host recognition to the rest of the phage, ultimately opening the capsid and perforating the cell wall and, thus, allowing safe channeling of the DNA into the host cytoplasm.

Published

2023

32. Bacteriophage endolysin powders for inhaled delivery against pulmonary infections.

Author

Wang Y, Khanal D, Alreja AB, Yang H, Yk Chang R, Tai W, Li M, Nelson DC, Britton WJ, and Chan HK

Subjects

Humans, Powders chemistry, Chemistry, Pharmaceutical methods, Lactose chemistry, Leucine chemistry, Trehalose chemistry, Respiratory Aerosols and Droplets, Particle Size, Administration, Inhalation, Bacteriophages chemistry, Pneumonia

Abstract

Endolysins are bacteriophage-encoded enzymatic proteins that have great potential to treat multidrug-resistant bacterial infections. Bacteriophage endolysins Cpl-1 and ClyJ-3 have shown promising antimicrobial activity against Streptococcus pneumoniae, which causes pneumonia in humans. This is the first study to investigate the feasibility of spray-dried endolysins Cpl-1 and ClyJ-3 with excipients to produce inhalable powders. The two endolysins were individually tested with leucine and sugar (lactose or trehalose) for spray drying method followed by characterization of biological and physico-chemical properties. A complete loss of ClyJ-3 bioactivity was observed after atomization of the liquid feed solution（before the drying process）, while Cpl-1 maintained its bioactivity in the spray-dried powders. Cpl-1 formulations containing leucine with lactose or trehalose showed promising physico-chemical properties (particle size, crystallinity, hygroscopicity, etc.) and aerosol performances (fine particle fraction values above 65%). The results indicated that endolysin Cpl-1 can be formulated as spray dried powders suitable for inhaled delivery to the lungs for the potential treatment of pulmonary infections., Competing Interests: Declaration of Competing Interest The authors 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 © 2023 Elsevier B.V. All rights reserved.)

Published

2023

33. An easy-to-use high-throughput selection system for the discovery of recombinant protein binders from alternative scaffold libraries.

Author

Möller M, Jönsson M, Lundqvist M, Hedin B, Larsson L, Larsson E, Rockberg J, Uhlén M, Lindbo S, Tegel H, and Hober S

Subjects

Recombinant Proteins genetics, Recombinant Proteins metabolism, Cell Surface Display Techniques, Escherichia coli genetics, Escherichia coli metabolism, Peptide Library, Bacteriophages chemistry, Bacteriophages genetics, Bacteriophages metabolism

Abstract

Selection by phage display is a popular and widely used technique for the discovery of recombinant protein binders from large protein libraries for therapeutic use. The protein library is displayed on the surface of bacteriophages which are amplified using bacteria, preferably Escherichia coli, to enrich binders in several selection rounds. Traditionally, the so-called panning procedure during which the phages are incubated with the target protein, washed and eluted is done manually, limiting the throughput. High-throughput systems with automated panning already in use often require high-priced equipment. Moreover, the bottleneck of the selection process is usually the screening and characterization. Therefore, having a high-throughput panning procedure without a scaled screening platform does not necessarily increase the discovery rate. Here, we present an easy-to-use high-throughput selection system with automated panning using cost-efficient equipment integrated into a workflow with high-throughput sequencing and a tailored screening step using biolayer-interferometry. The workflow has been developed for selections using two recombinant libraries, ADAPT (Albumin-binding domain-derived affinity proteins) and CaRA (Calcium-regulated affinity) and has been evaluated for three new targets. The newly established semi-automated system drastically reduced the hands-on time and increased robustness while the selection outcome, when compared to manual handling, was very similar in deep sequencing analysis and generated binders in the nanomolar affinity range. The developed selection system has shown to be highly versatile and has the potential to be applied to other binding domains for the discovery of new protein binders., (© The Author(s) 2023. Published by Oxford University Press. All rights reserved. For Permissions, please e-mail: journals.permissions@oup.com.)

Published

2023

34. Viruses inhibit TIR gcADPR signalling to overcome bacterial defence.

Author

Leavitt A, Yirmiya E, Amitai G, Lu A, Garb J, Herbst E, Morehouse BR, Hobbs SJ, Antine SP, Sun ZJ, Kranzusch PJ, and Sorek R

Subjects

Bacterial Proteins antagonists & inhibitors, Bacterial Proteins chemistry, Bacterial Proteins immunology, Bacterial Proteins metabolism, Plant Proteins antagonists & inhibitors, Plant Proteins chemistry, Plant Proteins immunology, Plant Proteins metabolism, Crystallography, X-Ray, Bacteria immunology, Bacteria metabolism, Bacteria virology, Receptors, Interleukin-1 chemistry, Signal Transduction immunology, Protein Domains, Bacteriophages chemistry, Bacteriophages immunology, Bacteriophages metabolism, Viral Proteins chemistry, Viral Proteins immunology, Viral Proteins metabolism, Toll-Like Receptors chemistry

Abstract

The Toll/interleukin-1 receptor (TIR) domain is a key component of immune receptors that identify pathogen invasion in bacteria, plants and animals 1-3 . In the bacterial antiphage system Thoeris, as well as in plants, recognition of infection stimulates TIR domains to produce an immune signalling molecule whose molecular structure remains elusive. This molecule binds and activates the Thoeris immune effector, which then executes the immune function 1 . We identified a large family of phage-encoded proteins, denoted here as Thoeris anti-defence 1 (Tad1), that inhibit Thoeris immunity. We found that Tad1 proteins are 'sponges' that bind and sequester the immune signalling molecule produced by TIR-domain proteins, thus decoupling phage sensing from immune effector activation and rendering Thoeris inactive. Tad1 can also efficiently sequester molecules derived from a plant TIR-domain protein, and a high-resolution crystal structure of Tad1 bound to a plant-derived molecule showed a unique chemical structure of 1 ''-2' glycocyclic ADPR (gcADPR). Our data furthermore suggest that Thoeris TIR proteins produce a closely related molecule, 1''-3' gcADPR, which activates ThsA an order of magnitude more efficiently than the plant-derived 1''-2' gcADPR. Our results define the chemical structure of a central immune signalling molecule and show a new mode of action by which pathogens can suppress host immunity., (© 2022. The Author(s), under exclusive licence to Springer Nature Limited.)

Published

2022

35. Viral Small Terminase: A Divergent Structural Framework for a Conserved Biological Function.

Author

Lokareddy RK, Hou CD, Li F, Yang R, and Cingolani G

Subjects

Cryoelectron Microscopy, Viral Proteins genetics, DNA, Viral chemistry, DNA Packaging, Endodeoxyribonucleases genetics, Adenosine Triphosphate, Virus Assembly genetics, Bacteriophages genetics, Bacteriophages chemistry

Abstract

The genome packaging motor of bacteriophages and herpesviruses is built by two terminase subunits, known as large (TerL) and small (TerS), both essential for viral genome packaging. TerL structure, composition, and assembly to an empty capsid, as well as the mechanisms of ATP-dependent DNA packaging, have been studied in depth, shedding light on the chemo-mechanical coupling between ATP hydrolysis and DNA translocation. Instead, significantly less is known about the small terminase subunit, TerS, which is dispensable or even inhibitory in vitro, but essential in vivo. By taking advantage of the recent revolution in cryo-electron microscopy (cryo-EM) and building upon a wealth of crystallographic structures of phage TerSs, in this review, we take an inventory of known TerSs studied to date. Our analysis suggests that TerS evolved and diversified into a flexible molecular framework that can conserve biological function with minimal sequence and quaternary structure conservation to fit different packaging strategies and environmental conditions.

Published

2022

36. Expansion of the Plaquing Host Range and Improvement of the Absorption Rate of a T5-like Salmonella Phage by Altering the Long Tail Fibers.

Author

Zhang J, Ning H, Lin H, She J, Wang L, Jing Y, and Wang J

Subjects

Genome, Viral, Host Specificity, Myoviridae genetics, Bacteriophages chemistry, Salmonella Phages genetics

Abstract

The high host specificity of phages is a real challenge in the therapy applications of the individual phages. This study aimed to edit the long tail fiber proteins ( pb1 ) of a T5-like phage to obtain the engineered phages with expanded plaquing host range. Two T5-like Salmonella phages with high genome sequence homology but different plaquing host ranges, narrow-host range phage vB STyj5-1 (STyj5-1) and wide-host range phage vB BD13 (BD13), were isolated and characterized. The pb1 parts of STyj5-1 were replaced by the corresponding part of BD13 using homologous recombination method to obtain the engineered phages. The alterations of the whole pb1 part or the N-terminal amino acids 1-400 of pb1 of STyj5-1 could expand their plaquing host ranges (from 20 strains to 30 strains) and improve their absorption rates (from 0.28-28.84% to 28.10-99.49%). Besides, the one-step growth curves of these engineered phages with modified pb1 parts were more similar to that of STyj5-1. The burst sizes of phages BD13, STyj5-1 and the engineered phages were 250, 236, 166, and 223 PFU per cell, respectively. The expanded plaquing host range and improved absorption rates of these engineered phages revealed that the pb1 part might be the primary determinant of the host specificities of some T5-like phages. IMPORTANCE Genetic editing can be used to change or expand the host range of phages and have been successfully applied in T2, T4 and other phages to obtain engineered phages. However, there are hardly any similar reports on T5-like phages due to that the determinant regions related to their host ranges have not been completely clarified and the editing of T5-like phages is more difficult compared to other phages. This study attempted and successfully expanded the host range of a narrow-host range T5-like phage (STyj5-1) by exchanging its whole pb1 part or the N-terminal 1-400aa of that part by a broad-host range phage (BD13). These demonstrated the pb1 part might be the primary determinant of the host specificities for some T5-like phages and provided an effective method of extension plaquing host range of these phages.

Published

2022

37. Architecture and self-assembly of the jumbo bacteriophage nuclear shell.

Author

Laughlin TG, Deep A, Prichard AM, Seitz C, Gu Y, Enustun E, Suslov S, Khanna K, Birkholz EA, Armbruster E, McCammon JA, Amaro RE, Pogliano J, Corbett KD, and Villa E

Subjects

Cryoelectron Microscopy, Bacteria cytology, Bacteria immunology, Bacteria metabolism, Bacteria virology, Bacteriophages chemistry, Bacteriophages immunology, Bacteriophages physiology, Bacteriophages ultrastructure, Cell Compartmentation, Viral Proteins chemistry, Viral Proteins metabolism, Viral Proteins ultrastructure, Virus Assembly

Abstract

Bacteria encode myriad defences that target the genomes of infecting bacteriophage, including restriction-modification and CRISPR-Cas systems 1 . In response, one family of large bacteriophages uses a nucleus-like compartment to protect its replicating genomes by excluding host defence factors 2-4 . However, the principal composition and structure of this compartment remain unknown. Here we find that the bacteriophage nuclear shell assembles primarily from one protein, which we name chimallin (ChmA). Combining cryo-electron tomography of nuclear shells in bacteriophage-infected cells and cryo-electron microscopy of a minimal chimallin compartment in vitro, we show that chimallin self-assembles as a flexible sheet into closed micrometre-scale compartments. The architecture and assembly dynamics of the chimallin shell suggest mechanisms for its nucleation and growth, and its role as a scaffold for phage-encoded factors mediating macromolecular transport, cytoskeletal interactions, and viral maturation., (© 2022. The Author(s).)

Published

2022

38. Capsule-Targeting Depolymerases Derived from Acinetobacter baumannii Prophage Regions.

Author

Drobiazko AY, Kasimova AA, Evseev PV, Shneider MM, Klimuk EI, Shashkov AS, Dmitrenok AS, Chizhov AO, Slukin PV, Skryabin YP, Volozhantsev NV, Miroshnikov KA, Knirel YA, and Popova AV

Subjects

Bacterial Capsules genetics, Bacterial Capsules metabolism, Glycoside Hydrolases metabolism, Polysaccharides metabolism, Polysaccharides, Bacterial metabolism, Prophages genetics, Prophages metabolism, Acinetobacter baumannii chemistry, Acinetobacter baumannii genetics, Acinetobacter baumannii metabolism, Bacteriophages chemistry, Bacteriophages metabolism

Abstract

In this study, several different depolymerases encoded in the prophage regions of Acinetobacter baumannii genomes have been bioinformatically predicted and recombinantly produced. The identified depolymerases possessed multi-domain structures and were identical or closely homologous to various proteins encoded in other A. baumannii genomes. This means that prophage-derived depolymerases are widespread, and different bacterial genomes can be the source of proteins with polysaccharide-degrading activities. For two depolymerases, the specificity to capsular polysaccharides (CPSs) of A. baumannii belonging to K1 and K92 capsular types (K types) was determined. The data obtained showed that the prophage-derived depolymerases were glycosidases that cleaved the A. baumannii CPSs by the hydrolytic mechanism to yield monomers and oligomers of the K units. The recombinant proteins with established enzymatic activity significantly reduced the mortality of Galleria mellonella larvae infected with A. baumannii of K1 and K92 capsular types. Therefore, these enzymes can be considered as suitable candidates for the development of new antibacterials against corresponding A. baumannii K types.

Published

2022

39. The DNA polymerase of bacteriophage YerA41 replicates its T-modified DNA in a primer-independent manner.

Author

Gomez-Raya-Vilanova MV, Leskinen K, Bhattacharjee A, Virta P, Rosenqvist P, Smith JLR, Bayfield OW, Homberger C, Kerrinnes T, Vogel J, Pajunen MI, and Skurnik M

Subjects

Capsid, Cryoelectron Microscopy, DNA, Viral genetics, DNA-Directed DNA Polymerase genetics, Genome, Viral genetics, Thymidine, Bacteriophages chemistry, Bacteriophages genetics

Abstract

Yersinia phage YerA41 is morphologically similar to jumbo bacteriophages. The isolated genomic material of YerA41 could not be digested by restriction enzymes, and used as a template by conventional DNA polymerases. Nucleoside analysis of the YerA41 genomic material, carried out to find out whether this was due to modified nucleotides, revealed the presence of a ca 1 kDa substitution of thymidine with apparent oligosaccharide character. We identified and purified the phage DNA polymerase (DNAP) that could replicate the YerA41 genomic DNA even without added primers. Cryo-electron microscopy (EM) was used to characterize structural details of the phage particle. The storage capacity of the 131 nm diameter head was calculated to accommodate a significantly longer genome than that of the 145 577 bp genomic DNA of YerA41 determined here. Indeed, cryo-EM revealed, in contrast to the 25 Å in other phages, spacings of 33-36 Å between shells of the genomic material inside YerA41 heads suggesting that the heavily substituted thymidine increases significantly the spacing of the DNA packaged inside the capsid. In conclusion, YerA41 appears to be an unconventional phage that packages thymidine-modified genomic DNA into its capsids along with its own DNAP that has the ability to replicate the genome., (© The Author(s) 2022. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2022

40. New method to quantify hydrophobicity of non-enveloped virions in aqueous media by capillary zone electrophoresis.

Author

Bastin G, Gantzer C, and Sautrey G

Subjects

Algorithms, Amino Acid Sequence, Bacteriophages chemistry, Humans, Models, Theoretical, Sodium Dodecyl Sulfate, Viral Proteins chemistry, Virion isolation & purification, Virion ultrastructure, Electrophoresis, Capillary, Hydrophobic and Hydrophilic Interactions, Virion chemistry

Abstract

The hydrophobicity of virions is a major physicochemical parameter regulating their dissemination in humans and the environment. But knowledge about potential factors modulating virion hydrophobicity is limited due to the lack of suitable quantifying methods. It has been recently shown that sodium dodecyl-sulfate (SDS) labels capsid hydrophobic domains in capillary zone electrophoresis of non-enveloped virions, altering their electrophoretic mobility (μ) in proportion to their hydrophobicity. This was exploited here to quantify the hydrophobicity of GA, Qβ and MS2 phages as a function of pH. By subtracting the native from the SDS-modified μ of phages, measured in the absence and presence of SDS, respectively, we defined a "hydrophobic index" increasing with virion hydrophobicity. Using this approach, we found that the virion hydrophobicity changes at a virion-specific pivotal pH. This procedure may be applied under various physicochemical conditions and to diverse non-enveloped virus families of significance to human health and the environment., (Copyright © 2022 Elsevier Inc. All rights reserved.)

Published

2022

41. Structure and assembly pattern of a freshwater short-tailed cyanophage Pam1.

Author

Zhang JT, Yang F, Du K, Li WF, Chen Y, Jiang YL, Li Q, and Zhou CZ

Subjects

Cryoelectron Microscopy, Crystallography, X-Ray, Genome Size, Genome, Viral, Models, Molecular, Molecular Conformation, Virus Assembly, Bacteriophages chemistry, Capsid chemistry, Cyanobacteria virology, Whole Genome Sequencing methods

Abstract

Despite previous structural analyses of bacteriophages, quite little is known about the structures and assembly patterns of cyanophages. Using cryo-EM combined with crystallography, we solve the near-atomic-resolution structure of a freshwater short-tailed cyanophage, Pam1, which comprises a 400-Å-long tail and an icosahedral capsid of 650 Å in diameter. The outer capsid surface is reinforced by trimeric cement proteins with a β-sandwich fold, which structurally resemble the distal motif of Pam1's tailspike, suggesting its potential role in host recognition. At the portal vertex, the dodecameric portal and connected adaptor, followed by a hexameric needle head, form a DNA ejection channel, which is sealed by a trimeric needle. Moreover, we identify a right-handed rifling pattern that might help DNA to revolve along the wall of the ejection channel. Our study reveals the precise assembly pattern of a cyanophage and lays the foundation to support its practical biotechnological and environmental applications., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2021 Elsevier Ltd. All rights reserved.)

Published

2022

42. Acid-stable capsid structure of Helicobacter pylori bacteriophage KHP30 by single-particle cryoelectron microscopy.

Author

Kamiya R, Uchiyama J, Matsuzaki S, Murata K, Iwasaki K, and Miyazaki N

Subjects

Cryoelectron Microscopy, DNA, Viral chemistry, Models, Molecular, Protein Conformation, Protein Domains, Protein Stability, Single Molecule Imaging, Bacteriophages chemistry, Capsid chemistry, Capsid Proteins chemistry, Helicobacter pylori virology

Abstract

The acid-stable capsid structures of Helicobacter pylori phages KHP30 and KHP40 are solved at 2.7 and 3.0 Å resolutions by cryoelectron microscopy, respectively. The capsids have icosahedral T = 9 symmetry and consist of each 540 copies of 2 structural proteins, a major capsid protein, and a cement protein. The major capsid proteins form 12 pentagonal capsomeres occupying icosahedral vertexes and 80 hexagonal capsomeres located at icosahedral faces and edges. The major capsid protein has a unique protruding loop extending to the neighboring subunit that stabilizes hexagonal capsomeres. Furthermore, the capsid is decorated with trimeric cement proteins with a jelly roll motif. The cement protein trimer sits on the quasi-three-fold axis formed by three major capsid protein capsomeres, thereby enhancing the particle stability by connecting these capsomeres. Sequence and structure comparisons between the related Helicobacter pylori phages suggest a possible mechanism of phage adaptation to the human gastric environment., Competing Interests: Declaration of interests The authors declare no competing interests., (Copyright © 2021 Elsevier Ltd. All rights reserved.)

Published

2022

43. Structural Assembly of Qβ Virion and Its Diverse Forms of Virus-like Particles.

Author

Chang JY, Gorzelnik KV, Thongchol J, and Zhang J

Subjects

Bacteriophages chemistry, Bacteriophages genetics, Bacteriophages ultrastructure, Capsid metabolism, Capsid ultrastructure, Capsid Proteins chemistry, Capsid Proteins genetics, Capsid Proteins metabolism, Cryoelectron Microscopy, Models, Molecular, RNA, Viral chemistry, RNA, Viral genetics, RNA, Viral metabolism, Virion chemistry, Virion genetics, Virion ultrastructure, Bacteriophages physiology, Virion physiology, Virus Assembly

Abstract

The coat proteins (CPs) of single-stranded RNA bacteriophages (ssRNA phages) directly assemble around the genomic RNA (gRNA) to form a near-icosahedral capsid with a single maturation protein (Mat) that binds the gRNA and interacts with the retractile pilus during infection of the host. Understanding the assembly of ssRNA phages is essential for their use in biotechnology, such as RNA protection and delivery. Here, we present the complete gRNA model of the ssRNA phage Qβ, revealing that the 3' untranslated region binds to the Mat and the 4127 nucleotides fold domain-by-domain, and is connected through long-range RNA-RNA interactions, such as kissing loops. Thirty-three operator-like RNA stem-loops are located and primarily interact with the asymmetric A/B CP-dimers, suggesting a pathway for the assembly of the virions. Additionally, we have discovered various forms of the virus-like particles (VLPs), including the canonical T = 3 icosahedral, larger T = 4 icosahedral, prolate, oblate forms, and a small prolate form elongated along the 3-fold axis. These particles are all produced during a normal infection, as well as when overexpressing the CPs. When overexpressing the shorter RNA fragments encoding only the CPs, we observed an increased percentage of the smaller VLPs, which may be sufficient to encapsidate a shorter RNA.

Published

2022

44. Viability, Stability and Biocontrol Activity in Planta of Specific Ralstonia solanacearum Bacteriophages after Their Conservation Prior to Commercialization and Use.

Author

Álvarez B, Gadea-Pallás L, Rodríguez A, Vicedo B, Figàs-Segura À, and Biosca EG

Subjects

Food Preservation economics, Freeze Drying, Fruit economics, Fruit microbiology, Solanum lycopersicum economics, Plant Diseases microbiology, Ralstonia solanacearum physiology, Bacteriophages chemistry, Bacteriophages growth & development, Biological Control Agents chemistry, Food Preservation methods, Solanum lycopersicum microbiology, Plant Diseases prevention & control, Ralstonia solanacearum virology

Abstract

Ralstonia solanacearum is a pathogen that causes bacterial wilt producing severe damage in staple solanaceous crops. Traditional control has low efficacy and/or environmental impact. Recently, the bases of a new biotechnological method by lytic bacteriophages vRsoP-WF2, vRsoP-WM2 and vRsoP-WR2 with specific activity against R. solanacearum were established. However, some aspects remain unknown, such as the survival and maintenance of the lytic activity after submission to a preservation method as the lyophilization. To this end, viability and stability of lyophilized vRsoP-WF2, vRsoP-WM2 and vRsoP-WR2 and their capacity for bacterial wilt biocontrol have been determined against one pathogenic Spanish reference strain of R. solanacearum in susceptible tomato plants in different conditions and making use of various cryoprotectants. The assays carried out have shown satisfactory results with respect to the viability and stability of the bacteriophages after the lyophilization process, maintaining high titers throughout the experimental period, and with respect to the capacity of the bacteriophages for the biological control of bacterial wilt, controlling this disease in more than 50% of the plants. The results offer good prospects for the use of lyophilization as a conservation method for the lytic bacteriophages of R. solanacearum in view of their commercialization as biocontrol agents.

Published

2022

45. Phage display-derived immunorecognition elements LSPR nanobiosensor for peptide hormone glycine-extended gastrin 17 detection.

Author

Fattahi Z, Tohidkia MR, and Yari Khosroushahi A

Subjects

Gold chemistry, Metal Nanoparticles chemistry, Bacteriophages chemistry, Biosensing Techniques, Gastrins analysis, Surface Plasmon Resonance

Abstract

The current study intended to evaluate two types of biorecognition element (BRE), namely recombinant antibody fragments and M13 bacteriophage-displayed antibody fragments, where protein L and electrostatic interactions were used to respectively conjugated antibodies and bacteriophages on AuNPs. The functionalization process was examined by DLS to monitor the changes in the size and zeta potential. The formation of the BRE-G17-Gly immunological complexes was manifested by aggregation (confirmed by FE-SEM) and color change from red to dark blue visible to the naked eye. Local refractive index variations of functionalized AuNPs were monitored by a UV - vis spectrophotometer, showing increasing size and decreasing zeta potential in all stages. The calibration plot was developed in the concentration range 1-5 µg/mL and the limit of detection (LOD) was 1 µg/mL. The LSRP nanobiosensor in combination with the phage-based BRE was an affordable and simple approach, as it was able to eliminate the time-consuming and costly step of extracting antibodies. Contrary to the traditional immunoassays, this method does not require additional amplification, e.g., enzymatic, to read the result. The proposed LSPR nanobiosensor model can be adapted to detect a wide range of pathogens, viruses, and biomarkers in the shortest possible time., (© 2022. The Author(s), under exclusive licence to Springer-Verlag GmbH Austria, part of Springer Nature.)

Published

2022

46. Major tail proteins of bacteriophages of the order Caudovirales.

Author

Zinke M, Schröder GF, and Lange A

Subjects

Capsid chemistry, Capsid metabolism, Cryoelectron Microscopy, Protein Conformation, Virion metabolism, Bacteriophages chemistry, Bacteriophages metabolism, Capsid Proteins metabolism, Caudovirales chemistry, Caudovirales metabolism

Abstract

Technological advances in cryo-EM in recent years have given rise to detailed atomic structures of bacteriophage tail tubes-a class of filamentous protein assemblies that could previously only be studied on the atomic scale in either their monomeric form or when packed within a crystal lattice. These hollow elongated protein structures, present in most bacteriophages of the order Caudovirales, connect the DNA-containing capsid with a receptor function at the distal end of the tail and consist of helical and polymerized major tail proteins. However, the resolution of cryo-EM data for these systems differs enormously between different tail tube types, partly inhibiting the building of high-fidelity models and barring a combination with further structural biology methods. Here, we review the structural biology efforts within this field and highlight the role of integrative structural biology approaches that have proved successful for some of these systems. Finally, we summarize the structural elements of major tail proteins and conceptualize how different amounts of tail tube flexibility confer heterogeneity within cryo-EM maps and, thus, limit high-resolution reconstructions., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2022

47. Cryo-EM Structures of Two Bacteriophage Portal Proteins Provide Insights for Antimicrobial Phage Engineering.

Author

Javed A, Villanueva H, Shataer S, Vasciaveo S, Savva R, and Orlova EV

Subjects

Bacteriophages chemistry, Caudovirales chemistry, Host Specificity, Phylogeny, Protein Domains, Protein Engineering, Synthetic Biology, Bacillus pumilus virology, Bacteriophages genetics, Capsid Proteins chemistry, Clostridium perfringens virology, Cryoelectron Microscopy methods, Genetic Engineering

Abstract

Widespread antibiotic resistance has returned attention to bacteriophages as a means of managing bacterial pathogenesis. Synthetic biology approaches to engineer phages have demonstrated genomic editing to broaden natural host ranges, or to optimise microbicidal action. Gram positive pathogens cause serious pastoral animal and human infections that are especially lethal in newborns. Such pathogens are targeted by the obligate lytic phages of the Salasmaviridae and Guelinviridae families. These phages have relatively small ~20 kb linear protein-capped genomes and their compact organisation, relatively few structural elements, and broad host range, are appealing from a phage-engineering standpoint. In this study, we focus on portal proteins, which are core elements for the assembly of such tailed phages. The structures of dodecameric portal complexes from Salasmaviridae phage GA1, which targets Bacillus pumilus , and Guelinviridae phage phiCPV4 that infects Clostridium perfringens , were determined at resolutions of 3.3 Å and 2.9 Å, respectively. Both are found to closely resemble the related phi29 portal protein fold. However, the portal protein of phiCPV4 exhibits interesting differences in the clip domain. These structures provide new insights on structural diversity in Caudovirales portal proteins and will be essential for considerations in phage structural engineering.

Published

2021

48. Biochemical characterization of LysVpKK5 endolysin from a marine vibriophage.

Author

Melo-López FN, Zermeño-Cervantes LA, Barraza A, Loera-Muro A, and Cardona-Félix CS

Subjects

Amino Acid Sequence, Aquatic Organisms, Bacteriophages classification, Bacteriophages genetics, Bacteriophages metabolism, Binding Sites, Calcium chemistry, Calcium pharmacology, Cations, Divalent, Endopeptidases chemistry, Endopeptidases genetics, Hydrogen-Ion Concentration, Kinetics, Models, Molecular, N-Acetylmuramoyl-L-alanine Amidase chemistry, N-Acetylmuramoyl-L-alanine Amidase genetics, Phylogeny, Protein Binding drug effects, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Interaction Domains and Motifs, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sequence Homology, Amino Acid, Sodium Chloride chemistry, Sodium Chloride pharmacology, Substrate Specificity, Viral Proteins chemistry, Viral Proteins genetics, Zinc chemistry, Zinc pharmacology, Bacteriophages chemistry, Endopeptidases metabolism, N-Acetylmuramoyl-L-alanine Amidase metabolism, Peptidoglycan metabolism, Vibrio parahaemolyticus virology, Viral Proteins metabolism

Abstract

Endolysins have been proposed as a potential antibacterial alternative for aquaculture, especially against Vibrio; the bacterial-agents that most frequently cause disease. Although multiple marine vibriophages have been characterized to date, research on vibriophage endolysins is recent. In this study, biochemical characterization of LysVpKK5 endolysin encoded by Vibrio parahaemolyticus-infecting VpKK5 phage was performed. In silico analysis revealed that LysVpKK5 possesses a conserved amidase_2 domain with a zinc-binding motif of high structural similarity to T7 lysozyme (RMSD = 0.107 Å). Contrary to expectations, the activity was inhibited with Zn 2+ and was improved with other divalent cations, especially Ca 2+ . It showed optimal muralytic activity at pH 10, and curiously, no lytic activity at pH ≤ 7 was recorded. As for the thermal stability test, the optimal activity was recorded at 30 °C; the higher residual activity was recorded at 4 °C, and was lost at ≥ 50 °C. On the other hand, increasing NaCl concentrations reduced the activity gradually; the optimal activity was recorded at 50 mM NaCl. On the other hand, the enzymatic activity at 0.5 M NaCl was approx 30% and of approx 50% in seawater. LysVpKK5 endolysin exhibited a higher activity on V. parahaemolyticus ATCC-17802 strain, in comparison with AHPND + strains., (Copyright © 2021 Elsevier Inc. All rights reserved.)

Published

2021

49. Pinholin S 21 mutations induce structural topology and conformational changes.

Author

Ahammad T, Khan RH, Sahu ID, Drew DL Jr, Faul E, Li T, McCarrick RM, and Lorigan GA

Subjects

Bacteriophages chemistry, Biological Transport, Cell Death genetics, Endopeptidases chemistry, Membrane Proteins chemistry, Mutation genetics, Viral Proteins chemistry, Virion chemistry, Bacteriophages genetics, Endopeptidases genetics, Membrane Proteins genetics, Viral Proteins genetics, Virion genetics

Abstract

The bacteriophage infection cycle is terminated at a predefined time to release the progeny virions via a robust lytic system composed of holin, endolysin, and spanin proteins. Holin is the timekeeper of this process. Pinholin S 21 is a prototype holin of phage Φ21, which determines the timing of host cell lysis through the coordinated efforts of pinholin and antipinholin. However, mutations in pinholin and antipinholin play a significant role in modulating the timing of lysis depending on adverse or favorable growth conditions. Earlier studies have shown that single point mutations of pinholin S 21 alter the cell lysis timing, a proxy for pinholin function as lysis is also dependent on other lytic proteins. In this study, continuous wave electron paramagnetic resonance (CW-EPR) power saturation and double electron-electron resonance (DEER) spectroscopic techniques were used to directly probe the effects of mutations on the structure and conformational changes of pinholin S 21 that correlate with pinholin function. DEER and CW-EPR power saturation data clearly demonstrate that increased hydrophilicity induced by residue mutations accelerate the externalization of antipinholin transmembrane domain 1 (TMD1), while increased hydrophobicity prevents the externalization of TMD1. This altered hydrophobicity is potentially accelerating or delaying the activation of pinholin S 21 . It was also found that mutations can influence intra- or intermolecular interactions in this system, which contribute to the activation of pinholin and modulate the cell lysis timing. This could be a novel approach to analyze the mutational effects on other holin systems, as well as any other membrane protein in which mutation directly leads to structural and conformational changes., (Copyright © 2021 Elsevier B.V. All rights reserved.)

Published

2021

50. Structural basis for anti-CRISPR repression mediated by bacterial operon proteins Aca1 and Aca2.

Author

Liu Y, Zhang L, Guo M, Chen L, Wu B, and Huang H

Subjects

Bacteriophages chemistry, Bacteriophages genetics, Models, Molecular, Pectobacterium carotovorum genetics, Pectobacterium carotovorum metabolism, Protein Conformation, Protein Multimerization, Pseudomonas Phages chemistry, Pseudomonas Phages genetics, Pseudomonas Phages metabolism, Pseudomonas aeruginosa genetics, Pseudomonas aeruginosa metabolism, Viral Proteins chemistry, Viral Proteins genetics, Bacteriophages metabolism, Clustered Regularly Interspaced Short Palindromic Repeats, Operon, Pectobacterium carotovorum virology, Pseudomonas aeruginosa virology, Viral Proteins metabolism

Abstract

It has been shown that phages have evolved anti-CRISPR (Acr) proteins to inhibit host CRISPR-Cas systems. Most acr genes are located upstream of anti-CRISPR-associated (aca) genes, which is instrumental for identifying these acr genes. Thus far, eight Aca families (Aca1-Aca8) have been identified, all proteins of which share low sequence homology and bind to different target DNA sequences. Recently, Aca1 and Aca2 proteins were discovered to function as repressors by binding to acr-aca promoters, thus implying a potential anti-anti-CRISPR mechanism. However, the structural basis for the repression roles of Aca proteins is still unknown. Here, we elucidated apo-structures of Aca1 and Aca2 proteins and their complex structures with their cognate operator DNA in two model systems, the Pseudomonas phage JBD30 and the Pectobacterium carotovorum template phage ZF40. In combination with biochemical and cellular assays, our study unveils dimerization and DNA-recognition mechanisms of Aca1 and Aca2 family proteins, thus revealing the molecular basis for Aca1-and Aca2-mediated anti-CRISPR repression. Our results also shed light on understanding the repression roles of other Aca family proteins and autoregulation roles of acr-aca operons., Competing Interests: Conflict of interest The authors declare that they have no conflicts of interest with the contents of this article., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2021