Next Article in Journal
Carbon Nanotube/Poly(dimethylsiloxane) Composite Materials to Reduce Bacterial Adhesion
Next Article in Special Issue
From Orphan Phage to a Proposed New Family–The Diversity of N4-Like Viruses
Previous Article in Journal
Microbial Association with Genus Actinomyces in Primary and Secondary Endodontic Lesions, Review
Previous Article in Special Issue
Application of Bacteriophages to Control Vibrio alginolyticus Contamination in Oyster (Saccostrea glomerata) Larvae
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Antibiotics
Volume 9
Issue 8
10.3390/antibiotics9080435
antibiotics-logo
Submit to this Journal Review for this Journal Propose a Special Issue
Article Menu

Article Menu

share Share announcement Help format_quote Cite question_answer Discuss in SciProfiles thumb_up
...
Endorse textsms
...
Comment
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Opinion

Prophage in Phage Manufacturing: Is the Risk Overrated Compared to Other Therapies or Food?

by
Gabard Jérôme
BioMaje SAS, 5, Chemin du Vercors, 49124 Sant Barthélemy d’Anjou, France
Antibiotics 2020, 9(8), 435; https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics9080435
Submission received: 10 June 2020 / Revised: 8 July 2020 / Accepted: 17 July 2020 / Published: 22 July 2020
(This article belongs to the Special Issue Phage Diversity for Research and Application)
Review Reports Versions Notes

Abstract

:
The rehabilitation of lytic bacteriophages, as living and replicative biological therapeutic agents, is only 2 decades old in western countries, compared to other therapeutic approaches using chemicals and inactivated or alive biologicals. This paper attempts to provide arguments to address prophage content issues in phage pharmaceutical preparations from a regulatory perspective. The author rebalances the risk associated with the presence of prophages in their pharmaceutical preparations in comparison (i) to lysogenic phages and prophages contained in various therapeutic anti-infective treatments, as well as in food or probiotics, (ii) to adventitious whole retroviruses or fragments contained in vaccines, and (iii) to the massive release of lysogenic phages and prophages induced by antibiotics usage.

1. Introduction

Phage therapy started [1,2] in 2017 within the western modern pharmaceutical industry. As the 20th century saw pharmaceutical chemistry rise, the concept of treating with a single, pure, and well-characterized chemical active ingredient became the trend [3]. Bacteriophage suffered from production quality issues [4], and the controversies about their true reality placed them in the category of strange, unpredictable, and inexplicable treatment, until electronic microscopy revealed their true biological nature [5] in 1940. Meanwhile, as antibiotics were discovered from biological organisms and chemically and properly characterized drugs, at reproducible concentration, standardized purity levels and contaminant traces started to rule the world of curative treatments [6].
The emergence of inactive biological drugs started to change the trend in the 1980s through the development of complex, but inert, molecules (recombinant proteins, therapeutic monoclonal antibodies, peptides, DNA, etc., often synthesized by microorganisms [7]. Although the active ingredient is a fixed molecule, the production tool is often a living factory more prone to variability than chemical synthesis. Regulatory agencies had to adapt guidelines and rules to these new treatments [8].
A third revolution occurred in the late 1990s with the arrival of curative therapies, using alive organisms on both production and treatment sides, as described in Table 1.
Biological variability now encompasses both production material and therapeutic treatment. The regulation adapted to fixed, chemical, or biological antibiotic molecules cannot apply anymore. Product variability from batch to batch is almost inevitable [9].
As part of it, the presence of prophages in a manufacturing strain, which accidently contaminates a bacteriophage drug batch, is identified as an issue for phage therapy [4]. Regulatory agencies are hampering the approval of phage therapy by insisting on the absence of prophages from phage preparations used to treat patients. This insistence sets a double standard, because many other approved therapies allows for far greater levels of viral release or contamination without greater evidence of safety.

2. Opinion

Prophages in bacteriophage manufacturing: Phage therapy uses lytic phages, which multiply cleanly in their production strain [4]. In other words, they do not leave any DNA from their own genome or embark DNA from their host during their replication cycle.
Contrary to lytic phages, temperate phages can integrate into the chromosome of a bacterial host upon infection, where they can reside as quiescent genetic material [10]. When the strain is stressed, such prophages may start replication. During that cycle, they may embark DNA from their host and transfer it to other bacterial strains. These host DNA fragments may carry virulence, toxins, antibiotic resistance, stress tolerance, and novel metabolic pathway genes, which provide significant adaptation advantages to their hosts [10]. In a way, prophages infecting prokaryote bacteria are comparable to retroviruses infecting eukaryote cells: each of them target a specific cell organism, remain dormant in their hosts, and are expressed when the host is stressed by various chemical, physical, or biological factors. For instance, when bacteria are stressed by Ciprofloxacin or Trimethoprim antibiotics [11], prophages are released, in a similar manner to herpes simplex virus type-2, which is via UV radiation [12].
Comparative genomics demonstrated that bacteria and bacteriophages are coevolving. This process is most evident for pathogenic bacteria, where the vast majority contain lysogenic prophages in their DNA. Therefore, the bacterial strains that are used to produce bacteriophages are likely to contain prophages [11]. High yield production in fermenters is a stress for the phage manufacturing strain; therefore, the process may lead to significant prophage release into the culture media [4]. Consequently, prophages may then be found in a phage therapy suspension batch used to treat patients.
Bacteriophages used to combat antibiotic resistance were classified as drugs in 2013 [13]; therefore, their manufacturing procedures must comply with pharmaceutical good manufacturing practices (GMPs), including stringent quality controls (QCs), such as detecting and eliminating the risk of prophage contamination introduced by bacteria master cell lines [14].
Vaccines containing retrovirus contaminants: One must notice that for prophylactic medicine, the adoption of biologicals, although inactivated, took place much earlier than that in the alive biological drug world. [15]
Inspired by Edward Jenner in the late eighteenth century and his protection against smallpox through cow vaccinia benign disease, Pasteur stated in 1881 the principle of vaccination: a "weakened viruses with the character of never killing, of giving a benign disease, which preserves from fatal disease". The list of vaccines against pathogenic infections with inactivated or killed microbes started with rabies at the end of the nineteenth century, then diphtheria, tetanus, typhoid, and tuberculosis in the 1920s. Vaccines against epidemic viruses, yellow fever, influenza, and polio rose between the 1930s and 1960s. Since then, with notable thanks to biotechnology, meningitis, hepatitis B, and the papillomavirus were amongst the latest targets [15].
This repeated successes in making efficient and reproductible prophylactic treatments against most major human (and animal) infections made of biological inactivated germs a fully integrated tool of our pharmacopeias.
Nevertheless, although vaccines do not generally bear adventitious contaminants, contamination of cell substrates that are used to produce them have been reported [16]. For instance, in 2010, independent researchers detected DNA fragments of porcinecircovirus (PCV) in Rotarix®, manufactured by GlaxoSmithKline, and in RotaTeq® vaccines produced by Merck.
After thorough investigation and identification of trypsin as the likely source of contamination, the European Medicinal Agency (EMA) Committee for Medicinal Products for Human Use considered that the PCV findings did not present a threat to public health and, consequently, that there was no need to restrict the use of the vaccines [16].
Viral risk monitoring is difficult in living human transplants: Alive biological transplants using tissue graft skin [17], organ transplants, or the newest cell therapy [18] refer to the transfer of body parts or cells from a compatible human donor toward a compatible human recipient.
In homograft, the human material from a patient is used to repair an injury, a failure, a defect, or an anomaly of another injury. Material transfer remains mostly intraspecific, i.e., within human genus, even though non-permanent animal material is sometimes temporarily used, such as pig origin skin graft for severe burn patients. In autograft, the biological material comes from the patient’s own body; therefore, the contamination risk is mostly nosocomial.
Guidelines have been published to mitigate the risk of virus transmission, especially retroviruses through homograft organ transplantation. For the EMA, baseline serology for risk factors for transplantation outcome should include cytomegalovirus (CMV), the hepatitis B virus, hepatitis C virus, EpsteinBarr virus, human immunodeficiency virus, polyoma virus, and Herpes simplex virus [19]. The FDA (Food and Drug Administration) for the USA follows identical recommendations [20].
Hence, serology, microbiology, and detailed questionnaires targeting disease-patient history support the choice of the donor. Sometimes, molecular techniques are added to evaluate the presence of retroviruses in the transplants, although such technical approaches are not generalized. Even so, the molecular tools used are not powerful enough to alleviate the risk of recipient contamination. The major hurdles include the worldwide epidemiology shift of infections, for instance with COVID-19, increasing antimicrobial resistance, suboptimal assays for microbiology screening of organ donors, and difficulties in detecting viruses [21].
Nevertheless, regulatory authorities consider that the benefit of organ transplantation for an expecting recipient makes the risk of viral contamination, introduced by the transplant, bearable and manageable using long lasting antiviral treatments, although patients are severely immunosuppressed to avoid graft rejection [22].
The black hole of fecal matter transfer: When it comes to interspecific alive biological medicines, the panoply of non-human living organisms used for treating human pathologies is still narrower. A fecal microbiota transplant (FMT) would be classified as hazardous by the fundamentalist preachers of zero safety risk, according to our current level of analytical tools and possibility of risk evaluation.
The millennium old Chinese therapeutic arsenal (the yellow soup) FMT was only tested in 1958 by Western Medicine, leading to the first randomized controlled and successful trial against Clostridium difficile in 2013 [23]. With FMT, tens of thousands of unknown bacterial species are transferred from a qualified donor to an ill patient, including yeast, fungi, viruses, and trillions of bacteriophages. Phages may play a major role in C. difficile (CDI) patients. Indeed, CDI patient enteric virome dysbiosis seems characterized by an increased Caudovirales phage abundance, opposing their decreased diversity, richness, and evenness [24]. In addition to C. difficile eradication, randomized controlled studies have shown FMT to be somewhat effective in treating ulcerative colitis, irritable bowel syndrome, and hepatic encephalopathy and have shown FMT to be beneficial for the eradication of multidrug-resistant organisms and graft-versus-host diseases [25].
Although putative donors are qualified through health, social, and travel questionnaires, clinical assessments, and microbiological testing [26], the quality of feces for FMT is far from being a 100% controlled process. Even current metagenomic tools, which may be used to qualify the microbial population of a donor, are ineffective for identifying the molecular details of each stool inhabitant [24]. They certainly skip plasmids, viruses, or prophages carrying antibiotic resistant genes, lysogenic phages, or poorly represented unknown pathogenic bacteria, leaving the door open to a transfer of them and/or their genetic material to the donor.
The recent bacteremia of two patients following FMT and leading to the death of one of the patients [27] by an ESBL (Enlarged Spectrum Betalactamase) Escherichia coli is the proof that a bullet-proof screening process is not implemented yet. However, clinical trials continue, as FMT seems full of promises.
Where probiotics and pharmabiotics join the scenario: Probiotics and prebiotics [28] have been used for decades to support human health and the food industry. Most current probiotic bacterial species are lactic strains, Bifidobacteria, or, to a lesser extent, Bacillus or Streptococcus thermophilus.
Dairy products are a reservoir of antibiotic resistance [29]. Following standard fermentation processes via lactic ferments, genes conferring resistance to tetracycline, erythromycin, and vancomycin have been detected and characterized in Lactococcus lactis, Enterococci, and Lactobacillus species isolated from fermented meat and milk products. Commensal bacteria, including lactic acid bacteria (LAB), may act as reservoirs of antibiotic resistance genes, such as those found in human pathogens [29]. Millions of lysogenic bacteriophages are released by lactic bacteria during fermentation, accumulate into a tank [30], and become a source of antibiotic resistance gene transfer. In addition, prophages have been shown to be released from Lactococcus lactis by antimicrobial peptide application [31].
In the case of diet pills and other food complements, such as cheese, yogurt (including fermented foods, such as aban, lassi, kefir, skyr, and other buttermilk), plain milk, and other fermented foods, no authority imposes monitoring of the presence or absence of intact or fragmented phage or prophage material in these products. Whether pasteurized or raw, taken altogether, a great diversity of phages is naturally present in the raw milk ecosystem, thus the absence of phages in dairies is unreachable [30]. An averaged human being eats billions of phages in their daily dairy supply [32].
Pharmabiotics, a new class of bacteria with medicinal properties, have been developed in the last 15 years. Compared to bacteria probiotics that can barely advertise a health claim, pharmabiotics are true drugs with medicinal revendications. For instance, RBX2660 (the first mix of beneficial Clostridium bacteria targeting microbiota) has been granted approval by the FDA for clinical testing in C. difficile intestinal infection [33]. The product has been classified as a drug instead of a diet probiotic.
One can assume that the manufacturing of pharmabiotics will be similar to those of probiotics, even though pharmaceutical good manufacturing practices (GMPs) will have to be truly applied. After more than 70 years of manufacturing optimization, probiotics production processes and quality controls are aspiring toward pharmabiotics production. Today, there is no request to check the presence of prophages in the millions of probiotics pills sold daily in the world. But what is the position of health regulatory authorities toward the latest pharmabiotics?
Antibiotics are potent inducers of prophage release: Antibiotic resistance emergence risk needs to be documented when filing for market authorization of a new antibiotic. The 2019 European Medicine Agency (EMA) guideline “on the evaluation of medicinal products indicated for treatment of bacterial infections, Rev.3” says that, “for test antibacterial agents of a new class, in vitro susceptibility studies should assess the potential for cross-resistance to occur between the test agents and licensed agents of other classes” [34]. In addition, clinical trials of antibiotic drug candidates must address their impact on the control of major antibiotic resistance forms [35].
Various studies have shown that antibiotics induce or boost lytic phage and prophage release upon treatments. A non-exhaustive list of publications is given below:
  • For Staphylococcus aureus under strong antibiotic selection [36];
  • For multidrug-resistant Stenotrophomonas maltophilia in response to ciprofloxacin stress [37];
  • For Clostridium difficile under pressure of profloxacin, moxifloxacin, levofloxacin, or mitomycin C [38];
  • For enterohemorrhagic Escherichia coli O157:H7 by [39];
  • For four isolates of fibrosis epidemic strain of Pseudomonas aeruginosa in cystic fibrosis induced by norfloxacin, tobramycin, colistin, ceftazidime, meropenem, or ciprofloxacin [40] at various levels depending on the antibiotic.
When it comes to antibiotic small molecules or peptides, no data regarding their potential effect on the release of lysogenic bacteriophages or prophages from patient bacterial microbiotas in reaction to treatment is requested by regulatory agencies toward filing for market authorization [41].

3. Discussion

In bacteriophage manufacturing for human therapy, the growing regulatory trend is to recommend that strains used to make master and working bacterial lines be exempt of lysogenic bacteriophages or of prophages. The reason is that they may carry antibiotic, virulence, and/or toxin genes and can be horizontally transferred to other the bacterial strains of a patient. The French Regulatory Agency (ANSM) tries to elaborate a pragmatic approach to rank prophage risk in five classes, as described in Table 2.
In addition, when the bacterial strain comes straight from a patient (as in the case of salvage therapy), although it should be characterized as much as possible (due to the presence of toxins and virulence genes, etc.), ANSM is more flexible when using it because it already expresses toxins or virulence factors in the sick patient.
Nevertheless, the comparison with other medicinal and health application fields makes it difficult today to display such different risk evaluation criteria when it comes to vaccines, FMT, probiotics, antibiotics, or fermented food.
Thousands of years of consumption of cheese or yogurts containing many kinds of pro/lysogenic phages without unusual or visible secondary effects on consumers is a green light for leaving things as they are. Logically, new probiotics and diet supplements containing lactic ferment and phages are not considered a danger for consumers. This is fair because their benefit toward alimentation is far greater than exposing human populations to the risk of eating prophage DNA.
Since the earliest days of vaccine manufacture, there have been cases where laboratory studies provided evidence for the presence of adventitious agents in a marketed product. For instance: (a) SV40 in polio vaccines; (b) bacteriophage in measles and polio vaccines; (c) reverse transcriptase in measles and mumps vaccines; and (d) entire PCV or DNA sequences in rotavirus vaccines [39]. As science and detection means progress, they may be eliminated [16]. However, in agreement with years of practice and a lack of related safety incidents, some of them, such as the PCV porcine virus, are left inside vaccines because they are considered harmless to humans [42].
Antibiotics, which catalyzes pro and lysogenic phage release [43], gene shuffling between bacterial species, and antibiotic resistance genes horizontal transfer have been in use for over 70 years. During the first decades of use, technologies were not available to detect their effects on microbiota flora. Today, we have ways to measure their impact on prophage release, but regulatory health agencies do not ask for this, because, overall, albeit antibiotic resistance emergence, years of practice have demonstrated their efficacy.
Using FMT for gut pathological indication may be considered less risky than injecting a bacteriophage into the blood stream. This may apply when considering a patient with a healthy and fully operational gastrointestinal tract. However, recipients are far from belonging to this category. Their intestinal barrier is quite deteriorated and permeable to many microorganisms, including bacteriophages, prophages, viruses, bacteria, etc. Microorganisms can cross the intestinal barrier and invade other body tissues or the vascular system, leading to severe pathologies [44]. Should we stop FMT from being used? Certainly not, because clinical studies demonstrate their benefits for curing C. difficile infected patients and other inflammatory bowel diseases.

4. Conclusions

Overall, the ratio between the benefit of phage therapy compared to the risk associated with batch content prophage contamination should be the driver. Do regulators influenced by meticulous research experts raise the bar too high for GMP phage manufacturing to succeed? Are we losing the big picture? After all, phage therapy is 100 years old. Don’t we have some historical experience prior to imposing manufacturing and safety constraints that are not applied to other therapeutic areas?

Funding

This opinion paper received no external funding and expresses only the views of the author.

Acknowledgments

The author acknowledges the indirect support given by the Agence Nationale de Securité du Médicament (ANSM) through a free-for-SMEs regulatory advice meeting, dated 27 January 2020.

Conflicts of Interest

The authors declare no conflict of interest.

References

  1. Twort, F. An Investigation on the nature of the ultra-microscopic Viruses. Lancet 1915, 186, 1241–1243. [Google Scholar] [CrossRef] [Green Version]
  2. D’Hérelle, F. On an invisible microbe antagonistic toward dysenteric bacilli: Brief note by Mr. F. D’Herelle, presented by Mr. Roux. Res. Microbiol. 1917, 158, 553–554. [Google Scholar]
  3. Jones, A.W. Early Drug Discovery and the Rise of Pharmaceutical Chemistry. Drug. Test. Anal. 2011, 3, 337–344. [Google Scholar] [CrossRef] [PubMed]
  4. Regulski, K.; Champion-Arnaud, P.; Gabard, J. Bacteriophage Manufacturing: From Early Twentieth-Century Processes to Current GMP. In Bacteriophages; Harper, D.R., Abedon, S.T., Burrowes, B.J., McConville, M.L., Eds.; Springer: Cham, Switzerland, 2018; pp. 1–31. [Google Scholar]
  5. Wittebole, X.; De Rock, S.; Opal, S.M. A historical overview of bacteriophage therapy as an alternative to antibiotics for the treatment of bacterial pathogens. Virulence 2014, 5, 226–235. [Google Scholar] [CrossRef]
  6. Ribeiro da Cunha, B.; Fonseca, L.P.; Calado, C.R.C. Antibiotic Discovery: Where Have We Come from, Where Do We Go? Antibiotics 2019, 8, 45. [Google Scholar] [CrossRef] [Green Version]
  7. Liu, J.K.H. The history of monoclonal antibody development–Progress, remaining challenges and future innovations. Ann. Med. Surg. 2014, 3, 113–116. [Google Scholar] [CrossRef]
  8. Hill, R.G.; Rang, H.P. Drug Discovery and Development. In Technology in Transition, 2nd ed.; Hill, R.G., Rang, H.P., Eds.; Churchill Livingston Elsevier: London, UK, 2013; pp. 293–297. [Google Scholar]
  9. Vulto, A.G.; Jaquez, O.A. The process defines the product: What really matters in biosimilar design and production? Rheumatology (Oxford) 2017, 56, 14–29. [Google Scholar] [CrossRef] [Green Version]
  10. Howard-Varona, C.; Hargreaves, K.R.; Abedon, S.T.; Sullivan, M.B. Lysogeny in nature: Mechanisms, impact and ecology of temperate phages. The ISME J. 2017, 11, 1511–1520. [Google Scholar] [CrossRef] [Green Version]
  11. Goerke, C.; Köller, J.; Wolz, C. Ciprofloxacin and Trimethoprim Cause Phage Induction and Virulence Modulation in Staphylococcus aureus. Antimicrob. Agents Chemother. 2006, 50, 171–177. [Google Scholar] [CrossRef] [Green Version]
  12. Rooney, J.F.; Straus, S.E.; Mannix, M.L.; Wohlenberg, C.R.; Banks, S.; Jagannath, S.; Brauer, J.E.; Notkins, A.L. UV Light-Induced Reactivation of Herpes Simplex Virus Type 2 and Prevention by Acyclovir. J. Infect. Dis. 1992, 166, 500–506. [Google Scholar] [CrossRef]
  13. Gabard, J.; Jault, P. How to Achieve a Good Phage Therapy Clinical Trial? In Phage Therapy: A Practical Approach; Springer: Berlin, Germany, 2019; pp. 147–168. [Google Scholar]
  14. Pirnay, J.-P.; Blasdel, B.G.; Bretaudeau, L.; Buckling, A.; Chanishvili, N.; Clark, J.R.; Corte-Real, S.; Debarbieux, L.; Dublanchet, A.; Vos, D.D.; et al. Quality and Safety Requirements for Sustainable Phage Therapy Products. Pharm. Res. 2015, 32, 2173–2179. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  15. Lombard, M.; Pastoret, P.P.; Moulin, A.M. A Brief History of Vaccines and Vaccination. Rev. Sci. Tech. 2007, 26, 29–48. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  16. Petricciani, J.; Sheets, R.; Griffiths, E.; Knezevic, I. Adventitious agents in viral vaccines: Lessons learned from 4 case studies. Biologicals. 2014, 42, 223–236. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  17. Markmann, C.F.; Barker, J.F. Historical Overview of Transplantation. Cold Spring Harb. Perspect. Med. 2013, 3, 1–18. [Google Scholar]
  18. Forgionea, G.; Sampognaa, S.Y.; Gurayab, A. Regenerative medicine: Historical roots and potential strategies in modern medicine. J. Microsc. Ultrastruct. 2015, 3, 101–106. [Google Scholar]
  19. EMA. Committee For Medicinal Products For Human Use. Available online: https://www.ema.europa.eu/en/documents/scientific-guideline/draft-guideline-clinical-investigation-immunosuppressants-solid-organ-transplantation_en.pdf. (accessed on 19 July 2007).
  20. Debbie, L.; Seem, R.N.; Ingi, L.; Craig, A.; Umscheid, M.D.; Matthew, J.; Kuehnert, M.D. PHS Guideline for Reducing Human Immunodeficiency Virus, Hepatitis B Virus, and Hepatitis C Virus Transmission Through Organ Transplantation. Public Health Rep. 2013, 128, 247–342. [Google Scholar]
  21. White, S.L.; Rawlinson, W.; Boan, P.; Sheppeard, V.; Wong, G.; Waller, K.; Opdam, H.; Kaldor, J.; Fink, M.; Verran, D.; et al. Infectious disease transmission in solid organ transplantation: Donor evaluation, recipient risk, and outcomes of transmission. Transplant Direct. 2019, 5, e416. [Google Scholar] [CrossRef]
  22. Claeys, E.; Vermeire, K. Immunosuppressive drugs in organ transplantation to prevent allograft rejection: Mode of action and side effects. J. Immunol. Sci. 2019, 3, 14–21. [Google Scholar] [CrossRef]
  23. Lee, C.H.; Steiner, T.; Petrof, E.O.; Smieja, M.; Roscoe, D.; Nematallah, A.; Weese, J.S.; Collins, S.; Moayyedi, P.; Crowther, M.; et al. Frozen vs fresh fecal microbiota transplantation and clinical resolution of diarrhea in patients with Recurrent Clostridium difficile Infection: A Randomized clinical trial. JAMA 2016, 315, 142–149. [Google Scholar]
  24. Fortier, L.C. Bacteriophages contribute to shaping clostridioides (clostridium) difficile species. Front. Microbiol. 2018, 9, 2033. [Google Scholar] [CrossRef] [Green Version]
  25. Ooijevaar, R.E.; Terveer, E.M.; Verspaget, H.W.; Kuijper, E.J.; Keller, J.J. Clinical application and potential of fecal microbiota transplantation. Annu. Rev. Med. 2019, 70, 335–351. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  26. McCune, V.L.; Quraishi, M.N.; Manzoor, S.; Moran, C.E.; Banavathi, K.; Steed, H.; Massey, D.C.O.; Trafford, G.R.; Iqbal, T.H.; Hawkey, P.M. Results from the first English stool bank using faecal microbiotatransplant as a medicinal product for the treatment of Clostridioides difficile infection. EclinicalMedicine 2020, 20, 100301. [Google Scholar] [CrossRef] [PubMed]
  27. DeFilipp, Z.; Bloom, P.P.; Torres Soto, M.; Mansour, M.K.; Sater, M.R.A.; Huntley, M.H.; Turbett, S.; Chung, R.T.; Chen, Y.B.; Hohmann, E.L. Drug-Resistant E. coli Bacteremia Transmitted by Fecal Microbiota Transplant. N. Engl. J. Med. 2019, 381, 2043–2050. [Google Scholar] [CrossRef] [PubMed]
  28. Hill, C.; Guarner, F.; Reid, G.; Gibson, G.R.; Merenstein, D.J.; Pot, B.; Morelli, L.; Canabi, R.B.; Flint, H.J.; Salminen, S.; et al. The International Scientific Association for Probiotics and Prebiotics consensus statement on the scope and appropriate use of the term probiotic. Nature 2014, 11, 506–515. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  29. Mathur, S.; Singh, R. Antibiotic resistance in food lactic acid bacteria—a review. Int. J. Food Microbiol. 2005, 105, 281–295. [Google Scholar] [CrossRef]
  30. Briggiler, M.; Marcó, S.; Moineau, S.; Quiberoni, A. Bacteriophages and dairy fermentations. Bacteriophages. Bacteriophage 2012, 2, 149–158. [Google Scholar]
  31. Madera, C.; García, P.; Rodríguez, A.; Suárez, J.E.; Martínez, B. Prophage Induction in Lactococcus Lactis by the Bacteriocin Lactococcin 972. Int. J. Food Microbiol. 2009, 1, 99–102. [Google Scholar] [CrossRef] [Green Version]
  32. Pujato, S.A.; Quiberoni, A.; Mercanti, D.J. Bacteriophages on dairy foods. J. Appl. Microbiol. 2019, 126, 14–30. [Google Scholar]
  33. Dubberke, E.R.; Lee, C.H.; Orenstein, R.; Khanna, S.; Hecht, G.; Gerding, D.N. Results from a randomized, placebo-controlled clinical trial of a RBX2660—A microbiota-based drug for the prevention of recurrent Clostridium difficile infection. Clin. Infect. Dis. 2018, 67, 1198–1204. [Google Scholar] [CrossRef] [Green Version]
  34. EMA. Committee for Human Medicinal Products. Available online: https://www.ema.europa.eu/en/evaluation-medicinal-products-indicated-treatment-bacterial-infections. (accessed on 14 January 2019).
  35. De Kraker, M.E.A.; Sommer, H.; de Velde, F.; Gravestock, I.; Weiss, E.; McAleenan, A.; Nikolakopoulos, S.; Amit, O.; Ashton, T.; Beyersmann, J.; et al. Optimizing the design and analysis of clinical trials for antibacterials against multidrug-resistant organisms: A white paper from COMBACTE’s STAT-Net. Clin. Infect. Dis. 2018, 67, 1922–1931. [Google Scholar]
  36. Haaber, J.; Leisner, J.J.; Cohn, M.T.; Catalan-Moreno, A.; Nielsen, J.B.; Westh, H.; Penadés, J.R.; Ingmer, H. Bacterial viruses enable their host to acquire antibiotic resistance genes from neighbouring cells. Nat. Commun. 2016, 7, 13333. [Google Scholar] [CrossRef] [PubMed]
  37. Devos, S.; Van Putte, W.; Vitse, J.; Van Driessche, G.; Stremersch, S.; Van Den Broek, W.; Raemdonck, K.; Braeckmans, K.; Stahlberg, H.; Kudryashev, M.; et al. Membrane vesicle secretion and prophage induction in multidrug-resistant Stenotrophomonas Maltophilia in response to ciprofloxacin stress. Environ. Microbiol. 2017, 19, 3930–3937. [Google Scholar]
  38. Meessen-Pinard, M.; Sekulovic, O.; Fortier, L.C. Evidence of in vivo prophage induction during Clostridium difficile infection. Appl. Environ. Microbiol. 2012, 78, 7662–7670. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  39. Matsushiro, A.; Sato, K.; Miyamoto, H.; Yamamura, T.; Honda, T. Induction of prophages of enterohemorrhagic Escherichia coli O157:H7 with norfloxacin. J. Bacteriol. 1999, 181, 2257–2260. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  40. Fothergill, J.L.; Mowat, E.; Walshaw, M.J.; Ledson, M.J.; James, C.E.; Winstanley, C. Effect of antibiotic treatment on bacteriophage production by a cystic fibrosis epidemic strain of Pseudomonas aeruginosa. Antimicrob. Agents Chemother. 2011, 55, 426–428. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  41. EMA. Committee For Medicinal Products For Human Use. Available online: https://www.ema.europa.eu/en/evaluation-medicinal-products-indicated-treatment-bacterial-infections (accessed on 19 December 2018).
  42. Victoria, J.G.; Wang, C.; Jones, M.S.; Jaing, C.; McLoughlin, K.; Gardner, S.; Delwart, E.L. Viral Nucleic Acids in Live-Attenuated Vaccines: Detection of Minority Variants and an Adventitious Virus. J. Virol. 2010, 84, 6033–6040. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  43. Filipiak, M.; Łoś, J.M.; Łoś, M. Efficiency of induction of Shiga-toxin lambdoid prophages in Escherichia coli due to oxidative and antibiotic stress depends on the combination of prophage and the bacterial strain. J. Appl. Genetics 2020, 61, 131–140. [Google Scholar] [CrossRef] [Green Version]
  44. Ribet, D.; Cossart, P. How bacterial pathogens colonize their hosts and invade deeper tissues. Microbes Infect. 2015, 17, 175–183. [Google Scholar] [CrossRef]
Table
Table 1. Therapies making living treatments from living organisms.
Table 1. Therapies making living treatments from living organisms.
Biological Therapy TypeProductionTreatment
Cell TherapyHuman bodyModified human cells
Fecal Matter Transfer (FMT)Native Feces from donorScreened feces to recipient
Bacteria therapyMicrobiotaIntestinal Microbes
Phage therapybacterial strainBacteriophage
Table
Table 2. Prophage management risk ranking, according to the French Regulatory Agency (ANSM).
Table 2. Prophage management risk ranking, according to the French Regulatory Agency (ANSM).
Case TypeRisk Level
1IdealProphage-free bacterial strain
2IntermediatePresence of prophage(s) carrying gene(s) that do not have code(s) for character(s), having an impact on the efficacy and/or safety of the treatment
3DegradedContains a prophage carrying an impact on gene(s), but which is (are) not (or barely) expressed
4InsufficientContains a prophage carrying an impact gene that is expressed
5UnacceptableContains a non-eliminable lysogenic phage
The cases ranked from 1 to 3 (above the bold black line) are acceptable. The cases below are not.

Share and Cite

MDPI and ACS Style

Jérôme, G. Prophage in Phage Manufacturing: Is the Risk Overrated Compared to Other Therapies or Food? Antibiotics 2020, 9, 435. https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics9080435

AMA Style

Jérôme G. Prophage in Phage Manufacturing: Is the Risk Overrated Compared to Other Therapies or Food? Antibiotics. 2020; 9(8):435. https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics9080435

Chicago/Turabian Style

Jérôme, Gabard. 2020. "Prophage in Phage Manufacturing: Is the Risk Overrated Compared to Other Therapies or Food?" Antibiotics 9, no. 8: 435. https://0-doi-org.brum.beds.ac.uk/10.3390/antibiotics9080435

Note that from the first issue of 2016, this journal uses article numbers instead of page numbers. See further details here.

Article Metrics

Back to TopTop