A tripartite strategy for controlling Clostridioides difficile
Lead Research Organisation:
University of Hertfordshire
Department Name: School of Life and Medical Sciences
Abstract
Gut bacteria can exchange DNA in many ways to resist antibiotics and cause untreatable infections. Our research on understanding how and when antibiotic resistance genes (ARGs) are exchanged with other bacteria, and finding new treatment agents should ultimately reduce these occurrences and make infections more easily treated.
This research is focused on Clostridioides difficile, an important human pathogen that causes infection with high illness and death rates. C. difficile found in animals and the environment are capable of causing human disease. Antibiotic therapy that disrupts the balance of microbes in the gut is a major risk factor for C. difficile infection (CDI), hence antibiotic treatment of CDI often fails. Also C. difficile is constantly evolving to be antibiotic-resistant because of gene exchange events that involve contact with other cells, bacterial viruses (known as phages), and external DNA such as transposons. Some of these events occur more frequently than others probably because of environmental factors, and understanding these is important for controlling ARG exchange events. For this, we examine C. difficile cells in contact with other bacteria, phages, and external DNA under different environmental conditions that mimic gut conditions such as presence of antibiotics and changing pH, and measure differences in ARG being exchanged between cells.
We are investigating new agents that kill or enhance antibiotic-killing of C. difficile as possible treatments for infection. Two such agents we investigate are phages and cationic peptides. Phages are natural enemies of bacteria, and many phages found so far can be genetically altered to efficiently kill C. difficile. We do this by removing phage genes that prevent efficient killing of bacteria, forcing the phage to replicate and break apart its bacterial host cell after infection. Cationic peptides are short pieces of positively-charged proteins that disrupt the cell wall or DNA of bacteria. In this research we will be testing a synthetic cationic peptide for its ability to enhance the activity of antibiotics against C. difficile by mixing them together and adding them to actively growing cells.
We also look for agents that protect patients from recurrent CDI, which is a serious problem in about 20% of CDI patients. Probiotics are harmless bacteria that help our gut resist colonisation by pathogens. We are testing the ability of different types of probiotics to stop C. difficile from colonising a human gut model that mimics the natural microbial environment in humans suffering from CDI. This is done by growing bacteria from faecal samples of healthy humans in three flasks of pH, nutrient, and oxygen-free conditions similar to a human large intestine. Antibiotics and C. difficile are then added to the flasks to establish "infection", more antibiotics are added to remove C. difficile and simulate a recurring infection. Probiotics are then added to the system and checked to see if the probiotic prevents C. difficile. We also investigate the ability of harmless C. difficile (which lack the ability to produce toxins) to compete with toxin-producing C. difficile strains and prevent infection. So far we have found a harmless strain that prevents growth and toxin production by a superbug strain of C. difficile under a wide range of experimental conditions and this has not been shown before.
This three-pronged approach to control C. difficile in acquiring ARG, growth, and re-colonisation will open new avenues for developing treatments for CDI.
This research is focused on Clostridioides difficile, an important human pathogen that causes infection with high illness and death rates. C. difficile found in animals and the environment are capable of causing human disease. Antibiotic therapy that disrupts the balance of microbes in the gut is a major risk factor for C. difficile infection (CDI), hence antibiotic treatment of CDI often fails. Also C. difficile is constantly evolving to be antibiotic-resistant because of gene exchange events that involve contact with other cells, bacterial viruses (known as phages), and external DNA such as transposons. Some of these events occur more frequently than others probably because of environmental factors, and understanding these is important for controlling ARG exchange events. For this, we examine C. difficile cells in contact with other bacteria, phages, and external DNA under different environmental conditions that mimic gut conditions such as presence of antibiotics and changing pH, and measure differences in ARG being exchanged between cells.
We are investigating new agents that kill or enhance antibiotic-killing of C. difficile as possible treatments for infection. Two such agents we investigate are phages and cationic peptides. Phages are natural enemies of bacteria, and many phages found so far can be genetically altered to efficiently kill C. difficile. We do this by removing phage genes that prevent efficient killing of bacteria, forcing the phage to replicate and break apart its bacterial host cell after infection. Cationic peptides are short pieces of positively-charged proteins that disrupt the cell wall or DNA of bacteria. In this research we will be testing a synthetic cationic peptide for its ability to enhance the activity of antibiotics against C. difficile by mixing them together and adding them to actively growing cells.
We also look for agents that protect patients from recurrent CDI, which is a serious problem in about 20% of CDI patients. Probiotics are harmless bacteria that help our gut resist colonisation by pathogens. We are testing the ability of different types of probiotics to stop C. difficile from colonising a human gut model that mimics the natural microbial environment in humans suffering from CDI. This is done by growing bacteria from faecal samples of healthy humans in three flasks of pH, nutrient, and oxygen-free conditions similar to a human large intestine. Antibiotics and C. difficile are then added to the flasks to establish "infection", more antibiotics are added to remove C. difficile and simulate a recurring infection. Probiotics are then added to the system and checked to see if the probiotic prevents C. difficile. We also investigate the ability of harmless C. difficile (which lack the ability to produce toxins) to compete with toxin-producing C. difficile strains and prevent infection. So far we have found a harmless strain that prevents growth and toxin production by a superbug strain of C. difficile under a wide range of experimental conditions and this has not been shown before.
This three-pronged approach to control C. difficile in acquiring ARG, growth, and re-colonisation will open new avenues for developing treatments for CDI.
Technical Summary
Clostridioides difficile is an anaerobic gut pathogen and recurring infections are difficult to treat. C. difficile infection (CDI) is facilitated by gut microflora dysbiosis, commonly caused by antibiotic therapy. C. difficile genomes are diverse with a core-/pan-genomic split of 29/71%, and mobile genetic elements can be transmitted by conjugation, transduction, and transformation, but it is unknown which mechanism is optimal. Our research aims to control C. difficile by targeting three areas - antimicrobial resistance acquisition, cell viability, and gut colonisation through three objectives: i) examine environmental factors of resistance gene dissemination, ii) develop phage and cationic peptides active against C. difficile, iii) develop probiotics as CDI prophylactic/treatment intervention agents. To examine gene transmission, newly isolated C. difficile in UK farms and public spaces will be conditionally induced for phage (e.g. exposure to various antimicrobials and pH) and tested for transduction of resistance genes in batch cultures and a CDI gut model. Conjugation and transformation will also be assayed in batch culture. C. difficile membrane vesicles (MV) are relatively unstudied; we will examine MV for gene transfer to bacterial cells, with and without phage. To develop C. difficile-specific phage and cationic peptides, CRISPR-based deletion of lysogeny genes will convert known temperate phages to virulent, while spontaneous lytic phage mutants will be selected by chelating agents. Phage host range, lysogeny, and resistance will be examined in batch culture and a gut model. A cationic polymer will be tested for potentiation of antibiotics and antisense PNA in vitro. To develop probiotics against colonising C. difficile, various species will be tested for preventing primary or secondary CDI and microbial interactions will be mapped. Research outcomes will lead to greater understanding of resistance transmission and intervention agents.
Publications
Goh S
(2024)
Membrane Vesicles of Clostridioides difficile and Other Clostridial Species.
in Advances in experimental medicine and biology
| Description | This equipment grant has enabled us to determine the prevalence of Clostridioides difficile, a pathogen normally associated with hospital settings, in environmental samples (soil and water), farms, animals and food in Great Britain. Characterisation of these isolates and comparisons to those of human origin will allow us to understand whether anthropogenic activities may be contributing to the evolution and spread of this bacterium, including its ability to swap antimicrobial resistance genes with other bacterial species, and how we can avoid or reduce C. difficile spread. We genetically modified a hypervirulent C. difficile strain to be rid of an infecting virus (phage) and found the mutant appears more able to grow in a low nutrient environment compared to the wild type. More experiments are on-going to investigate in the ways which the infecting phage may be influencing the physiology of its bacterial host. |
| Exploitation Route | The collection of C. difficile isolates derived from animals, food and the environment can be used to study C. difficile and antimicrobial resistance genes transmission within and between human, animals, and the environment to control its spread. This impacts on farming practices, food policies, environment protection and biosurveillance (e.g. screening for community-acquired infections) nationally and internationally. The C. difficile phage isogenic mutant could be used to investigate the contribution of phages to bacterial fitness, pathogenicity and persistence when compared to the hypervirulent wild-type. Our strategy employed to delete phage could be used by others to create other phage mutants for wider studies, and methods we developed for isolating C. difficile membrane vesicles could be used for developing phage therapy or vaccines, and will eventually impact healthcare and medical biotechnology. |
| Sectors | Agriculture Food and Drink Environment Healthcare Pharmaceuticals and Medical Biotechnology |
| Description | Pig health |
| Geographic Reach | National |
| Policy Influence Type | Participation in a guidance/advisory committee |
| Impact | No changes on policy or practice have arisen yet, since this project only started last 5 months ago. But I anticipate changes in farm practice and food policy in the future (perhaps 5 years from now). |
| Description | Problem based learning assignment |
| Geographic Reach | National |
| Policy Influence Type | Influenced training of practitioners or researchers |
| Description | PhD studentship |
| Amount | £56,000 (GBP) |
| Funding ID | Clostridioides difficile in UK pigs and risks to the food chain |
| Organisation | Perry Foundation |
| Sector | Charity/Non Profit |
| Country | United Kingdom |
| Start | 08/2023 |
| End | 08/2027 |
| Title | Membrane vesicle purification and assays |
| Description | The anaerobic workstations purchased with this grant has enabled anaerobic culture of C. difficile in larger volumes for membrane vesicle (MV) purification at different time points. We have developed a purification method that uses ultrafiltration and ultracentrifugation, and a semi-quantitative method for MVs using a lipid-specific fluorescence dye assay. We have also developed a more complex MV-phage co-culture method which previously was not possible with the old equipment. |
| Type Of Material | Biological samples |
| Year Produced | 2023 |
| Provided To Others? | No |
| Impact | PhD student presented findings at the UK Extracellular Vesicle Society meeting in December 2023. |
| Title | Non-clinical C. difficile isolates |
| Description | A collection of non-clinical C. difficile isolates derived from pigs, soil, and water has been created. The isolates will be used to investigate whether C. difficile is a risk to the food chain, and transmission pathways between animals, human and the environment (One Health). The equipment award has enabled my research in C. difficile to continue and expand. Notably, I was able to accept grants from Food Safety Research Network, and Perry Foundation on C. difficile as a risk to the food chain. This project involves sampling pig farms and abattoirs for isolation of C. difficile, hence processing a large number of samples which would not have been possible in our old equipment. |
| Type Of Material | Database/Collection of data |
| Year Produced | 2023 |
| Provided To Others? | No |
| Impact | None as yet |
| Description | Collaborative Action for Pork Safety (CAPS) |
| Organisation | Agricultural and Horticulture Development Board |
| Country | United Kingdom |
| Sector | Charity/Non Profit |
| PI Contribution | I am leading the collaboration with AHDB and Animal and Plant Health Agency (APHA). My team work on isolating C. difficile from pig farms and slaughtered pigs in abattoirs. We will then characterise the isolates and compare genomic phylogeny to human isolates, and investigate the mobilome and resistome. |
| Collaborator Contribution | AHDB help with advertising the study to recruit farmers, sampling of abattoirs for a national pig tissue bank, developing educational material for pork producers on engaging in research for the benefit of the pork sector. AHDB are also undertaking a study on the behaviour of farmers to biosecurity. APHA is undertaking a study on hepatitis E virus in the same pig farms sampled for C. difficile and hosting the national pig tissue bank for disease surveillance. Both AHDB and APHA staff have trained UH staff on pig behaviour and sampling. |
| Impact | Through this partnership we have preliminary data on C. difficile prevalence in GB pigs and pork, results of which were presented at the Combatting CDI conference in Cardiff, 27-18/2. However this project only started last September hence it is too early for other outputs. |
| Start Year | 2023 |
| Description | Collaborative Action for Pork Safety (CAPS) |
| Organisation | Animal and Plant Health Agency |
| Country | United Kingdom |
| Sector | Public |
| PI Contribution | I am leading the collaboration with AHDB and Animal and Plant Health Agency (APHA). My team work on isolating C. difficile from pig farms and slaughtered pigs in abattoirs. We will then characterise the isolates and compare genomic phylogeny to human isolates, and investigate the mobilome and resistome. |
| Collaborator Contribution | AHDB help with advertising the study to recruit farmers, sampling of abattoirs for a national pig tissue bank, developing educational material for pork producers on engaging in research for the benefit of the pork sector. AHDB are also undertaking a study on the behaviour of farmers to biosecurity. APHA is undertaking a study on hepatitis E virus in the same pig farms sampled for C. difficile and hosting the national pig tissue bank for disease surveillance. Both AHDB and APHA staff have trained UH staff on pig behaviour and sampling. |
| Impact | Through this partnership we have preliminary data on C. difficile prevalence in GB pigs and pork, results of which were presented at the Combatting CDI conference in Cardiff, 27-18/2. However this project only started last September hence it is too early for other outputs. |
| Start Year | 2023 |
| Description | PATH-SAFE meeting Nov 2023 |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | National |
| Primary Audience | Study participants or study members |
| Results and Impact | I was invited to attend this PATH-SAFE meeting by Food Safety Research Network because of the relevance of m CAPS project. It was a very late invitation after the programme was fixed, but I was invited to present a poster of my project plans (which at that point was only 2 months old). I spoke to many people from academia, industry, trade associations, and government about my project and contributed to discussions on biosurveillance and data sharing. Most people had never heard of University of Hertfordshire. |
| Year(s) Of Engagement Activity | 2023 |
| URL | https://www.food.gov.uk/our-work/pathogen-surveillance-in-agriculture-food-and-environment-path-safe... |
| Description | UK Extracellular Vesicle Society meeting Dec 2023 |
| Form Of Engagement Activity | A talk or presentation |
| Part Of Official Scheme? | No |
| Geographic Reach | National |
| Primary Audience | Postgraduate students |
| Results and Impact | My PhD student presented a poster at the meeting. The topic was on membrane vesicles of C. difficile. She had many useful discussions on membrane vesicles with other PhD students and academics. |
| Year(s) Of Engagement Activity | 2023 |
| URL | https://www.ukev.org.uk/ukev-forum-2023/ |