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A comprehensive literature scoping review of infection prevention and control methods for viral-mediated gene therapies

Published online by Cambridge University Press:  31 January 2024

Jill E. Blind Open the ORCID record for Jill E. Blind [Opens in a new window] ,
Sumit Ghosh ,
Taylor D. Niese ,
Julia C. Gardner Open the ORCID record for Julia C. Gardner [Opens in a new window] ,
Stephanie Stack-Simone ,
Abigail Dean  and
Matthew Washam
Jill E. Blind*
Affiliation:
Department of Pharmacy, Nationwide Children’s Hospital, Columbus, OH, USA
Sumit Ghosh
Affiliation:
Department of Research Safety, Abigail Wexner Research Institute at Nationwide Children’s Hospital, Columbus, OH, USA
Taylor D. Niese
Affiliation:
Department of Pharmacy, Nationwide Children’s Hospital, Columbus, OH, USA
Julia C. Gardner
Affiliation:
Department of Pharmacy, Cincinnati Children’s Hospital Medical Center, Cincinnati, OH, USA
Stephanie Stack-Simone
Affiliation:
Center for Clinical Excellence, Department of Epidemiology, Nationwide Children’s Hospital, Columbus, OH, USA
Abigail Dean
Affiliation:
Department of Pharmacy, Nationwide Children’s Hospital, Columbus, OH, USA
Matthew Washam
Affiliation:
Center for Clinical Excellence, Department of Epidemiology, Nationwide Children’s Hospital, Columbus, OH, USA
*
Corresponding author: Jill Blind; Email: jill.blind@nationwidechildrens.org

Abstract

Objective:

This comprehensive literature scoping review outlines available infection prevention and control (IPC) methods for viral-mediated gene therapies and provides one IPC strategy for the healthcare setting based on a single-center recommendation.

Methods:

A team of experts in pharmacy, healthcare epidemiology, and biosafety with experience in viral-mediated gene therapy was assembled within a pediatric hospital to conduct a comprehensive literature scoping review. The comprehensive review included abstracts and full-text articles published since 2009 and utilized prespecified search terms of the five viral vectors of interest: adenovirus (AV), retrovirus (RV), adeno-associated virus (AAV), lentivirus (LV), and herpes simplex virus (HSV). Case reports, randomized controlled trials, and bench research studies were all included, while systematic reviews were excluded.

Results:

A total of 4473 case reports, randomized control trials, and benchtop research studies were identified using the defined search criteria. Chlorine compounds were found to inactivate AAV and AV, while alcohol-based disinfectants were ineffective. There was a relative paucity of studies investigating surface-based disinfection for HSV, however, alcohol-based disinfectants were effective in one study. Ultraviolent irradiation was also found to inactivate HSV in numerous studies. No studies investigated disinfection for LV and RV vectors.

Conclusions:

The need to define IPC methods is high due to the rapid emergence of viral-mediated gene therapies to treat rare diseases, but published clinical guidance remains scarce. In the absence of these data, our center recommends a 1:10 sodium hypochlorite solution in clinical and academic environments to ensure complete germicidal activity of viral-mediated gene therapies.

Type
Original Article
Information
Antimicrobial Stewardship & Healthcare Epidemiology , Volume 4 , Issue 1 , 2024 , e15
Creative Commons
Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution and reproduction, provided the original article is properly cited.
Copyright
© The Author(s), 2024. Published by Cambridge University Press on behalf of The Society for Healthcare Epidemiology of America

Introduction

Over the last 10 years, novel biological therapies have rapidly emerged as revolutionary treatment options for rare diseases. Reference Eisenman and Swindle1,Reference Ginn, Amaya and Alexander2 According to the American Society for Gene and Cell Therapy, over 3,900 gene, cell, and RNA therapies are currently in development across the globe. Reference Eisenman, Debold and Riddle3,Reference Ghosh, Brown and Jenkins4 Within the gene therapy landscape, many of the in vivo genetically modified therapies are formulated with a viral-mediated backbone. Viral vector-mediated gene therapies use modified viruses as drug-delivery vehicles to introduce specific DNA sequences, regulatory RNAs, or other therapeutic substrates into cells Reference Eisenman and Swindle5,Reference Lundstrom6 Commercial gene therapy agents, such as onasemnogene abeparvovec and voretigene neparvovec, are comprised of an adeno-associated virus (AAV) vector, whereas the oncolytic virus, talimogene laherparepvec, is comprised of a modified herpes simplex virus. Reference Hernandez7 Nearly all gene therapies commercially available use one of three vector types: AAV, adenovirus (AV), or lentivirus (LV). Reference Ghosh, Brown and Jenkins4,Reference Bulcha, Wang and Hong8 Adeno-associated virus and AV vectors are typically used in gene therapies directly administered to patients by infusion or local administration, with AAV being the most popular vector for areas outside of oncology and vaccines. Reference Ghosh, Brown and Jenkins4,Reference Bulcha, Wang and Hong8 Lentivirus vectors are typically used for ex vivo therapies, in which cells harvested from a patient are modified in the lab before transplantation. Reference Ghosh, Brown and Jenkins4,Reference Bulcha, Wang and Hong8

Although these viral-mediated gene therapies are genetically modified to not cause human disease, they all possess the unique property of being biologically active and carry potential biohazardous risks to the healthcare workers who handle them directly—a characteristic not typically seen with traditional pharmaceutical drug formulations. Reference Blind, McLeod and Campbell9,Reference Eisenman10 In addition, viral shedding post-infusion may present the possibility of viral transmission to healthcare workers caring for these patients. While the viability for long-term gene expression and the adverse effects of these drugs within their respective patient populations will continue to be monitored in late-phase clinical trials and through post-marketing surveillance, occupational safety data will lag. Further, the limited shedding data reported in early clinical trials and the lack of regulatory guidance describing infection prevention and control (IPC) methods for these therapies ultimately prevent biosafety and healthcare epidemiology professionals from clearly defining post-infusion infection control standards. Reference Eisenman and Swindle1

With many novel biologic therapies being pushed through fast-track approval pathways, health systems will consequently be challenged to develop on-demand IPC guidance, using limited knowledge and occupational safety data to match both the unique viral vector systems and the quick pace of gene and cell therapy development. Reference Eisenman, Debold and Riddle3 Contact times for kill rates on commercial disinfecting agents could be utilized to provide baseline guidance for defining IPC practices within the institutional setting; however, emerging therapies utilize novel viral vector systems or genetically modified organisms that are not found in the environment and, therefore, do not have corresponding published kill rate data. The current literature scoping review provides a comprehensive analysis of available IPC methods reported for viral-mediated therapeutics. Additionally, we provide one possible strategy for the development of best-practice IPC recommendations for the healthcare setting based on our extensive, single-center experience working in a large pediatric hospital with an associated research institute.

Methods

A team of pharmacy, healthcare epidemiology, and biosafety experts was identified within the institution and assembled to initiate the project. The viral vectors chosen for the comprehensive literature scoping review included AV, retrovirus (RV), AAV, LV, and herpes simplex virus (HSV). These 5 viruses account for over 56% of all vector systems utilized in clinical trials. Reference Eisenman, Debold and Riddle3 In addition, modified versions of 3 of these viruses are found in commercially approved drugs within the United States (AV, AAV, HSV); the remaining 2 (RV, LV) are frequently utilized for genetic modifications in cellular-based gene therapy but continue to be researched in a variety of clinical applications. Reference Lundstrom6,Reference Chen, Keiser and Davidson11Reference Petrich, Marchese and Jenkins14 Three bibliographic databases were chosen for review: Cumulative Index to Nursing and Allied Health Literature; MEDLINE from the National Library of Medicine; and PubMed from the National Library of Medicine. The Laboratory-Acquired Infections (LAI) database from the American Biological Safety Association was also used to acquire research case reports of occupational or environmental infections in research.

Search terms were identified using medical subject headings from the National Library of Medicine. To obtain articles on infection control, the following search terms were defined by the team: disinfect; environmental exposure; occupational exposure; biosafety; infection control; and inactivation. Viral vector search terms were expanded to include various alliterations and included: adenoviridae; adenoviridae vector; AV; AV vector; retroviridae; retroviridae vector; RV; RV vector; adeno-associated virus vector; AAV vector; LV; LV vector; simplex virus; and simplex virus vector. Each viral vector term was individually paired with each infection control term, requiring 70 different search combinations to complete the literature scoping review within the bibliographic databases (Table 1). Viral vector terms alone were utilized to search the LAI database. Search filters were applied to limit results to those published since 2009 and published in English. Both abstracts and full articles were permitted for inclusion.

Table 1. Search strategy for comprehensive literature review a , b

a Search method for Cumulative Index to Nursing and Allied Health Literature (CINAHL), MEDLINE from the National Library of Medicine, and PubMed from the National Library of Medicine included “[Vector Term] AND [Cleaning Term].”

b Search method for Laboratory-Acquired Infections database included “[Vector Term].”

Case reports, randomized controlled trials, and bench research studies that met the search criteria were all included for evaluation and data abstraction, while systematic reviews were excluded. Following article collection, an independent abstractor evaluated each publication for inclusion and manual data abstraction into a spreadsheet containing the following data points: virus/vector, viral family, study interventions based on the Centers for Disease Control and Prevention Guideline for Disinfection and Sterilization in Healthcare Facilities (2008), other non-chemical interventions, affected party and reaction (if case report), duration of intervention, assessment of intervention, and study conclusions. Duplicate articles within the same viral family, case reports with no interventions, and publications on in vivo treatment options for clinical patients were removed. Two independent reviewers then validated the data points for accuracy and relevance to the primary research aim.

Results

The comprehensive literature scoping review resulted in 4473 total publications and case reports related to the five designated viral-mediated vectors and associated disinfection terms (Table 2). Inclusion of taxonomic viral family and genus classifications in the search terminology resulted in publications related to clinical manifestations of the wild-type virus and in vivo treatment methods for patients. Therefore, 98.1% (n = 4390) of the total publications reviewed were deemed to be irrelevant to the primary research question of viral vector-mediated IPC methods. A subset of publications was further excluded (n = 59, 1.3%) due to the various alliterations of IPC methods utilized as search terms, which resulted in duplicate publications within the same viral vector category. The remaining 24 publications were represented within 20 unique journals, with 19 of the journals describing a peer-review process as part of manuscript submission.

Table 2. Comprehensive literature review results

Table 3 provides a comprehensive overview of IPC methods for viral vector-based gene therapy products. Chlorine compounds were found to inactivate AAV and AV, while alcohol-based disinfectants were ineffective. There was a relative paucity of studies investigating surface-based disinfection for HSV, however alcohol-based disinfectants were effective in one study. Ultraviolent (UV) irradiation was also found to inactivate HSV in numerous studies. No studies investigated disinfection for LV and retrovirus vectors.

Table 3. Infection prevention and control methods for common viruses utilized in viral-mediated gene therapy

Abbreviations: AAV, Adeno-associated Virus; Adv, Adenovirus; CAGE, Choline and Geranate; EtOH, Ethyl Alcohol; HSV, Herpes Simplex Virus; HPV, Hydrogen Peroxide Vapor; LV, Lentivirus; MB, Methylene Blue; PAA, Peracetic Acid; PHMB, Polyhexamethylene Biguanide; Recombinant rAAV, adeno-associated virus; RV, Retrovirus; TCID, Tissue Culture Infectious Dose; UV, Ultraviolet; UV-C, Ultraviolet-C.

a No peer-review process is described within journal acceptance policies.

Key: ✓ partial or complete inactivation; X no inactivation; — not studied.

Discussion

Novel gene therapies represent a significant breakthrough in the care of many medical conditions. Gene therapies utilizing viral vectors to deliver the genetic material present unique IPC considerations not present with traditional pharmaceutical formulations in the clinical setting, specifically concerning environmental disinfection and personal protective equipment. The NIH Recombinant DNA Guidelines, United States Pharmacopeia Chapters 800, and the sixth edition of Biosafety in Microbiological and Biomedical Laboratories (BMBL) offer the general framework of working with viral vectors, and they are often used as a reference for risk assessment for human gene transfer research. Reference Blind, McLeod and Campbell9 However, no single guidance document has comprehensive information about disinfection practices, shedding, and risk assessment when using these vector systems in a healthcare setting. Additionally, limited data on shedding requires organizations to work with their Institutional Biosafety Committee (IBC) and healthcare epidemiology teams to develop policies specific to their centers. Reference Eisenman, Debold and Riddle3,Reference Ghosh, Brown and Jenkins4 In the last few years, several local IBCs have been requiring study teams to collect shedding data during the early phase of clinical trials. Hopefully, as there is growth in the field of human gene transfer in the coming few years more information related to shedding will be available. In general, most healthcare facilities recommend universal/standard precautions with patient material between 14 and 30 days after administration for both healthcare staff and direct family members. Reference Blind, McLeod and Campbell9

A hierarchy originally designed by Earle H Spaulding defines common disinfectants as either high-, intermediate-, or low level, based on their ability to kill various microorganisms. Disinfection protocols in the patient setting are extrapolated from this rational approach provided by Spaulding and from data generated from wild-type viruses in basic research studies. When placed on untreated plastic, recombinant AAV and adenoviral vectors were recoverable by cell culture for 3 and 14 days, respectively. Reference Reuter, Fang and Ly39 Common oxidative disinfectants include peroxides, peroxygen-persulfate types, peroxide-peracetic acid, and chlorine-based disinfectants. These disinfectants have been found to successfully eliminate adenoviral vectors in research studies. These disinfectants have an appropriate spectrum of activity against some of the most common viruses in a research facility, given that any organism of equal or greater sensitivity than that of AVs likely also will be inactivated by these products. Reference McDonnell and Burke40

Similarly, the Environmental Protection Agency has a list of disinfectants for emerging viral pathogens that provides endorsement and kill claims based on active ingredient, virus type, and surfaces which are utilized for risk assessment during clinical trials by organizations. 41 Based on this information, most therapies utilizing AV, AAV, or plasmid DNA vectors require disinfection with 1% sodium hypochlorite solution, with the need for prolonged contact times causing concern for damage to surfaces with repetitive long-term use. Reference Ghosh, Brown and Jenkins4,41 Similarly, center-wise policies related to disinfection are developed in consultation with local IBCs and infection prevention teams based on data gathered related to shedding. Herpesvirus can be inactivated with 70% alcohol solutions as well, presenting fewer material surface incompatibility concerns. Reference Dickinson, Marsh and Shao37 Non-surface-based disinfectant options including hydrogen peroxide vapor and UV irradiation may also play a role in viral gene vector therapy disinfection protocols, however, effectiveness is dependent upon multiple factors including burden of organic matter which limits their usage as a primary disinfection agent.

Duration and extent of viral shedding varies with individual therapeutics, though data are limited. Reference Eisenman and Swindle1,Reference Eisenman, Debold and Riddle3,Reference Ghosh, Brown and Jenkins4 Standard precautions, including covering site of inoculation, should be utilized in patients treated with viral vector gene therapies. Additional transmission-based precautions with contact, droplet, and eye precautions should be employed when viral vectors are administered via aerosol. Immunocompromised healthcare workers or household contacts should avoid contact with patients treated with attenuated, replication-competent herpes viral vectors during the shedding period. Reference Bulcha, Wang and Hong8,Reference Blind, McLeod and Campbell9,42 When working with viral vector gene therapies, clinical staff should wear appropriate personal protective equipment, including gowns, gloves, and eye or respiratory protection, and should further be educated on the potential risks of percutaneous exposure through accidental needlestick. Reference Hernandez7,Reference Blind, McLeod and Campbell9

Commercially approved agents may provide healthcare teams with some product-specific disinfection and spill-related recommendations within their package inserts. Nadofaragene firadenovec, an AV-mediated therapy, recommends sodium hypocholorite with 0.5% active chlorine or 6% hydrogen preroxide solution with a contact time of 15 minutes to treat any local spill. 43 Talimogene laherparepvec notes that any surface that comes in contact with the product should be treated with a virucidal agent, such as 1% sodium hypochlorite or 70% isopropyl alcohol. 42 In the absence of clinical regulatory recommendations to support broad IPC methods for all commercial and clinical research therapies, institutions must develop local policies and procedures to cover a variety of operational scenarios.

Standardized, consistent, and easily interpreted recommendations must be established to ensure the safety of healthcare workers handling these products. Current handling recommendations for viral-based gene therapies should be derived from the United States Pharmacopeia Chapters 800, commercially available gene therapy package inserts, the Center for Disease Control and Prevention’s Biosafety in Microbiological and Biomedical Laboratories (BMBL, 6 th Edition), and the NIH Guidelines for Research Involving Recombinant or Synthetic Nucleic Acid Molecules. Reference Blind, McLeod and Campbell9 Table 4 provides institutional recommendations for infection control methods when handling or preparing viral-based gene therapies in a healthcare system.

Table 4. An infection prevention and control strategy based on single-center experience

In this review, we highlight some of the challenges pharmacy and healthcare staff face regarding the use of virus-based gene therapies. The heterogeneity of methodology in studies included in this review precludes definitive recommendations of a single best infection control approach to these gene therapies, and further study will be needed as new products become available for patient use. Current advancements in gene therapy have opened the door to cures at a molecular level for many genetic diseases. The design of new experimental viral vectors with emerging technologies and the rate at which gene therapies are approved highlight the critical role of pharmacists, healthcare epidemiologists, infection preventionists, and biosafety professionals in identifying overall risk and operationalizing acceptable policies, predominantly in the absence of a consensus framework for the risk assessment process.

Data availability statement

The authors confirm that the data supporting the findings of this review are available within the article and supplementary material.

Acknowledgments

The authors have no additional acknowledgments for this article.

Financial support

No funding was secured for this review.

Competing interests

None of the authors have conflicts of interest relevant to this article.

Footnotes

Previous presentation: These data or findings have not been presented previously in any other preliminary report or abstract.

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Figure 0

Table 1. Search strategy for comprehensive literature reviewa,b

Figure 1

Table 2. Comprehensive literature review results

Figure 2

Table 3. Infection prevention and control methods for common viruses utilized in viral-mediated gene therapy

Figure 3

Table 4. An infection prevention and control strategy based on single-center experience