Next Article in Journal
Human T-Lymphotropic Virus (HTLV): Epidemiology, Genetic, Pathogenesis, and Future Challenges
Previous Article in Journal
HPV-Driven Head and Neck Cancer: The European Perspective
Previous Article in Special Issue
Seroprevalence and Risk Factors of Crimean–Congo Hemorrhagic Fever Exposure in Wild and Domestic Animals in Benin
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Viruses
Volume 17
Issue 5
10.3390/v17050663
viruses-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
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Review

Virucidal Approaches for Hemorrhagic Fever Viruses

by
Raymond W. Nims
1 and
M. Khalid Ijaz
2,*
1
Syner-G BioPharma, Boulder, CO 80503, USA
2
Global Research and Development for Lysol and Dettol, Reckitt Benckiser LLC, Montvale, NJ 07645, USA
*
Author to whom correspondence should be addressed.
Viruses 2025, 17(5), 663; https://doi.org/10.3390/v17050663
Submission received: 27 February 2025 / Revised: 11 April 2025 / Accepted: 19 April 2025 / Published: 30 April 2025
(This article belongs to the Special Issue Viral Hemorrhagic Disease)
Versions Notes

Abstract

We have reviewed the primary literature on the virucidal efficacy of microbicidal active ingredients, formulated microbicides, and physical inactivation approaches (heat, irradiation) for hemorrhagic fever viruses (HFVs) (arenaviruses, filoviruses, flaviviruses, hantaviruses, nairoviruses, and phenuiviruses), and for two non-typical HFV paramyxoviruses. As each of these HFVs are large, lipid-enveloped RNA viruses, their susceptibilities to virucidal agents are informed by the so-called hierarchy of susceptibility of pathogens to microbicides. The unique susceptibility of lipid-enveloped viruses to most classes of microbicides is based on the common mechanisms of action of envelope-disrupting microbicides. Despite this, due to the relatively great lethality of these viruses, it is prudent (where possible) to confirm the expected efficacies of inactivation approaches in testing involving the HFVs themselves (as opposed to less lethal surrogate viruses) using field-relevant methods. Empirical data for virucidal activities of microbicidal active ingredients, formulated microbicides, and physical inactivation approaches, such as heat, ultraviolet light, and gamma irradiation, that were collected specifically for HFVs have been reviewed and summarized in this paper. These empirical data for surface and hand hygiene approaches, liquid inactivation approaches, and approaches for rendering diagnostic samples safe to handle inform non-pharmaceutical interventions intended to mitigate transmission risk associated with these HFVs.

1. Introduction

The hemorrhagic fever viruses (HFVs) are members of a group of virus families, including the Arenaviridae, Filoviridae, Flaviviridae, Hantaviridae, Nairoviridae, and Phenuiviridae. These, and two non-typical HFVs from the Paramyxoviridae family share the following commonalities [1]: they are relatively large, enveloped viruses with positive- or negative-sense single-stranded RNA genomes; they are arboviruses (insect-borne) or are carried in rodent or mammalian vectors; and they are uniquely lethal in terms of case mortality rates in humans. The U.S. Centers for Disease Prevention and Control (CDC) describes viral hemorrhagic fever as “a condition where many of the body’s organ systems are affected, the overall cardiovascular system is damaged, and the body’s ability to function on its own is reduced. In addition to VHFs, there are serious infectious diseases like Nipah and Hendra diseases that also require a specialized laboratory, are highly pathogenic, and have no, or limited, vaccine or treatment currently available. VHFs, Nipah, and Hendra disease can cause relatively mild illness or more life-threatening disease. Symptoms can vary but may include bleeding or hemorrhaging” [2]. Examples of specific HFVs include the arenaviruses Lassa virus, Junin virus, Machupo virus, Sabiá virus, Lujo virus, and Guanarito virus; the filoviruses Ebola virus and Marburg virus; the flaviviruses Kyasanur Forest disease virus, Alkhurma hemorrhagic fever virus, Omsk hemorrhagic fever virus, dengue virus, and yellow fever virus; the nairovirus Crimean–Congo hemorrhagic fever; the hantavirus Hantaan virus; and the phenuiviruses Rift Valley fever virus, heartland virus, and severe fever with thrombocytopenia syndrome virus [2,3,4]. The non-typical HFVs include the Nipah virus and Hendra virus [2]. Certain of the diseases associated with the HFVs to be discussed (including Crimean–Congo hemorrhagic fever, Ebola virus disease and Marburg virus disease, Lassa fever, Nipah disease and henipaviral disease, and Rift Valley fever) have been included in past World Health Organization (WHO) Priority Disease lists [5]. This inclusion signifies that these “diseases pose the greatest public health risk due to their epidemic potential and/or whether there is no or insufficient countermeasures” [5].
Due to the relative lethality of HFVs, manipulation of cell cultures infected with these viruses and handling of virus stocks for efficacy studies on inactivation approaches are typically restricted to BSL-4 laboratories. This has resulted in a slower accumulation of suspension- and surface-inactivation efficacy data for microbicides and efficacy data for hand/skin hygiene products for these viruses relative to viruses which are able to be handled safely in BSL-2 or BSL-3 laboratories. Fortunately, in the absence of such empirical data, one may predict the efficacy of microbicides for use against HFVs on the basis of the so-called hierarchy of susceptibility of pathogens to microbicides [1] (developed originally from the Spaulding Classification [6]). In a U.S. Environmental Protection Agency (EPA) guidance [7], viruses have been classified into three categories, ranked from lesser to greater susceptibility to microbicides: small, non-enveloped viruses; large, non-enveloped viruses; and enveloped viruses. The generally accepted hierarchy of susceptibility of pathogens to microbicides provides to the public health communities a starting point for infection prevention and control (IPAC) measures to be used for emerging pathogens (including HFVs), per the EPA [8] and European Health authorities [9].
It is prudent, whenever possible, to confirm the efficacies of inactivation approaches predicted for emerging HFVs on the basis of the hierarchy of pathogen susceptibility by conducting empirical efficacy studies on the specific viruses. While the mechanisms of action of microbicides for viruses should apply similarly to different members of a given virus family, certain intrafamily exceptions in susceptibility are known to exist [10,11].
In the present review, we have assembled the primary literature concerning the virucidal efficacy of microbicidal active ingredients, formulated microbicidal products, hand/skin hygiene formulations, laboratory reagents, and physical inactivation approaches for inactivating HFVs. This review represents a refocusing and update of our previous review on the efficacy of microbicides against WHO Priority Disease List viruses [1] and is intended to complement recent reviews focusing primarily on inactivation methods for emerging viruses to be used for diagnostic samples or for vaccine development purposes [12,13].

2. Materials and Methods

The approach that we have taken for this review consisted of searching the literature (Google Scholar, PubMed) up to January 2025 for articles pertaining to virucidal efficacies of microbicidal active ingredients, microbicidal formulations, hand sanitizers, laboratory reagents, and physical inactivation approaches evaluated specifically against HFVs. Our goal was to attempt to identify and consider all the primary literature on these topics and to supplement this with the secondary literature only where the primary literature was not able to be identified.

3. Results

3.1. General Considerations

The hierarchy of pathogen susceptibility to microbicides [1,7] suggests that certain classes of microbicidal agents should display virucidal efficacy against lipid-enveloped viruses in general and therefore against the HFVs under consideration here. These include lipid-disrupting agents (alcohols, quaternary ammonium compounds such as benzalkonium chloride, phenolics such as para-chloro-meta-xylenol, detergents such as soap and nonionic surfactants, and organic acids such as citric, lactic, and salicylic acids) [14]. Protein-denaturing agents (alcohols, phenolics, oxidizers, and organic acids) inactivate enveloped viruses by degrading the spike proteins required for infection of host cells and by degrading capsid proteins [14]. Genome-degrading agents, such as alcohols and oxidizing agents, are expected to inactivate both enveloped and non-enveloped viruses [14]. Those microbicides displaying virucidal efficacy against less susceptible pathogens (such as mycobacteria, large and small non-enveloped viruses, bacterial spores/protozoan oocysts, and prions) are expected to display virucidal efficacy against HFVs as well. In the remainder of this review, we have identified the empirical testing data available to confirm the above expectations.
Physical inactivation approaches display virucidal efficacies that are less dependent upon the envelope status of the virus but rather on genome or particle size (gamma irradiation, electron beam irradiation), capsid protein make-up and spike proteins in enveloped viruses (heat), or nucleotide composition or size of the genome (ultraviolet light) [15]. The physical inactivation approaches are more typically used to render laboratory specimens safe to handle (gamma irradiation, X-ray irradiation, electron beam irradiation, heat) or for surface disinfection (ultraviolet light in the C range, UV-C) [15]. The literature addressing the empirically determined efficacies of these physical inactivation approaches for HFVs has been reviewed, and the data have been summarized along with the microbicidal inactivation data.
Virucidal activities (efficacies) of microbicidal active ingredients, formulated microbicides and hand/skin hygiene products, and physical inactivation approaches may be assessed using a variety of experimental approaches. For instance, one approach involves the examination of the efficacy for inactivating viruses intentionally deposited on model environmental surfaces (e.g., glass, plastic, or stainless-steel carriers). Such studies ideally are performed according to international standards (such as the American Society for Testing and Materials [ASTM] method ASTM E1053-20 [16]). Alternatively, the efficacy of microbicides may be tested by the addition of the active ingredients or formulations at typical use concentrations to viruses suspended in liquid matrices (suspension testing), ideally according to international standards (ASTM E1052-20 [17] or EN 14476:2013 + A2:2019 [18]). The efficacy of hand/skin hygiene agents is typically performed according to the suspension testing standards. Inactivation of viruses aerosolized into aerobiology chambers by air sanitizing sprays or devices may be evaluated according to U.S. Environmental Protection Agency guidelines and standardized protocols [19,20,21]. In each of the experimental approaches described above, the inclusion of an organic load (a mixture of organic and inorganic substances intended to mimic human pathophysiological enteric or respiratory body fluids such as mucus, saliva, or fecal matter) into the inactivation matrix is often included as a field-appropriate challenge to the inactivation approach [22]. In fact, requirements for the inclusion of such an organic load in the inactivation matrix are articulated within the international standards [16,17,18,20]. The final category of virucidal efficacy testing that has been addressed within this review pertains to inactivation approaches (chemical and physical) intended to render hemorrhagic fever virus-contaminated diagnostic samples and other laboratory specimens safe for handling within non-BSL-4 facilities. These approaches have included gamma irradiation, heat, nucleic acid extraction reagents, lysis buffers, tissue fixatives, and various types of microbicidal active ingredients and formulations.
In the sections that follow, the tables pertaining to the various families of HFVs are intended to provide only a high-level description of the inactivation efficacy results contained within the cited primary literature. That is, not all information from the cited articles has been included in the tables. Readers who are interested in a particular hemorrhagic fever virus or a particular family of HFVs and who desire additional granular detail are encouraged to obtain and review the individual articles cited. In addition, where specific formulated microbicidal or laboratory products were tested for virucidal efficacy against HFVs, the trade names of those products can be obtained by reviewing the individual articles cited.

3.2. Efficacy of Virucidal Approaches for Inactivating Hemorrhagic Fever Arenaviruses

Hemorrhagic fever viruses in the Arenaviridae family include Lassa virus (causing Lassa fever), Junin virus (Argentine hemorrhagic fever), Machupo virus (Bolivian hemorrhagic fever), Sabiá virus (Brazilian hemorrhagic fever), Lujo virus (Lujo hemorrhagic fever), and Guanarito virus (Venezuelan hemorrhagic fever). Each of these viruses is transmitted by a rodent vector [3,4]. The disease Lassa fever may be acquired through touching surfaces (fomites) contaminated with the virus, by eating contaminated food (including the rodent vector), by inhaling air contaminated with the virus (which may contain virus-contaminated urine or feces aerosolized through human activities such as sweeping) or following exposure to bodily fluids of an infected person [23]. Approaches for inactivating arenaviruses in suspension (i.e., within liquids) have been characterized quite recently, while approaches for rendering laboratory specimens safe for handling in diagnostic laboratories have been available for a longer period of time. Included in the latter category are a variety of solvents and detergents for which efficacy against a surrogate low pathogenic arenavirus (Morogor arenavirus) have been reported [24].
The results of this literature review (Table 1) indicate that knowledge gaps exist in the cases of surface hygiene and hand/skin hygiene agent efficacy for the HFVs from the arenavirus family. Until such gaps have been resolved, the efficacies of surface and hand hygiene agents shown to be effective for other enveloped viruses may be extrapolated to these arenaviral HFVs.

3.3. Efficacy of Virucidal Approaches for Inactivating Hemorrhagic Fever Filoviruses

Hemorrhagic fever viruses in the Filoviridae family [37] include the various variants of the Zaire Ebola virus (EBOV, EBOV/Mak, EBOV/May, EBOV/Kik, and EBOV/Yam-Ecr), Reston virus, Sudan virus, and Marburg virus. The filoviruses cause zoonotic infections in wild animals, and the reservoir animal is speculated to be bats [3]. During Ebola outbreaks, it has been noted that human-to-human transmission may occur through ritual handling of corpses, intrafamilial transmission, or nosocomial transmission [3]. Less is known about the transmission of the Marburg virus. A relatively great deal of research into the effectiveness of approaches for inactivating filoviruses on environmental surfaces has been reported (Table 2). Fewer data have been published on the inactivation of filoviruses in suspension (i.e., within liquids). As with the arenaviruses, multiple approaches for rendering laboratory specimens safe for handling in diagnostic laboratories have been characterized. Until the identified knowledge gaps have been resolved, the efficacy of inactivation approaches shown to be effective for other enveloped viruses in suspension testing may be extrapolated to these filoviral HFVs.

3.4. Efficacy of Virucidal Approaches for Inactivating Hemorrhagic Fever Flaviviruses

Hemorrhagic fever viruses in the Flaviviridae family include some well-known viruses that have been prevalent for some time in tropical regions of the globe, such as dengue virus and yellow fever virus, as well as more recently emerging viruses, including Kyasanur Forest disease virus (first identified in Karnataka, India in 1957), Alkhurma hemorrhagic fever virus (first isolated Jeddah, Saudia Arabia in the 1990s), and Omsk hemorrhagic fever virus (first identified around 1945 in Omsk, Russia) [57]. As with other HFVs, the global distribution of these flaviviruses is linked with the ecology of the vectors and reservoir species. In the case of yellow fever virus and dengue virus, outbreaks have occurred in areas (e.g., Brazil) where established mosquito vectors were thought to have been under control as changes in established vector ecology have occurred and the viruses have adapted to additional vector species (e.g., Aedes albopictus) [4]. Vector (tick) migration has also expanded the distribution of the Alkhurma hemorrhagic fever virus from its initial focus in southwestern India [4].
The results of this literature review (Table 3) indicate that some knowledge exists in the cases of surface hygiene, suspension inactivation, hand/skin hygiene agent efficacies and for approaches for rendering laboratory specimens safe for handling in diagnostic laboratories for the HFVs from the Flaviviridae family, although almost exclusively for yellow fever virus and dengue virus.

3.5. Efficacy of Virucidal Approaches for Inactivating Hemorrhagic Fever Hantaviruses

Hemorrhagic fever viruses within the Hantaviridae family include the Hantaan virus, Sin Nombre virus, and Dobrava virus, for which 5–15% of cases are fatal. In contrast, Seoul, Saaremaa, and Puumala virus infections appear to be less severe, with less than 1% of cases dying from the disease. Additional named hantaviruses are listed in references [62,63]. The hantaviruses are transmitted by a variety of rodent vectors, causing in the Americas hantavirus pulmonary syndrome (HPS) and in Europe hemorrhagic fever with renal syndrome (HFRS) [64,65]. The global distributions of the various hantaviruses are determined by the host ranges of their rodent vectors.
The results of this literature review (Table 4) indicate that knowledge gaps exist in the cases of surface hygiene with microbicides and hand/skin hygiene agent efficacies for the HFVs from the Hantaviridae family. Until the identified knowledge gaps have been resolved, the efficacies of agents shown to be effective for other enveloped viruses in surface inactivation and hand/skin hygiene testing may be extrapolated to these hantaviral HFVs.

3.6. Efficacy of Virucidal Approaches for Inactivating Hemorrhagic Fever Nairoviruses

The nairovirus with the greatest public health impact on humans is the ixodid tick-borne Crimean–Congo hemorrhagic fever virus (CCHFV). CCHFV outbreaks have occurred over a geographic area including Western and Central Asia, the Middle East, Africa, and Southern Europe. The virus causes a hemorrhagic fever with a case fatality rate of 10% to 40% [71]. While it is not clear that CCHFV is transmitted during blood transfusions, investigators have proactively characterized the efficacy and fluence requirements of methylene blue and ultraviolet C or visible light inactivation systems (THERAFLEX UV-Platelets and THERAFLEX MB-Plasma, for inactivating the virus in spiked donor blood platelet concentrates or plasma, respectively) [72].
The results of this literature review (Table 5) indicate that extensive knowledge gaps exist in the case of the HFVs from the Nairoviridae family. The secondary literature provides some guidance (e.g., “CCHFV can be inactivated by many disinfectants including 1% hypochlorite, 70% alcohol, hydrogen peroxide, peracetic acid, iodophors, glutaraldehyde, and formalin. It can also be destroyed by UV light or pH < 6. One study found that heating at 56 °C (133 °F) for 30 min inactivated the virus, while another reported that 60 °C (140 °F) for 60 min was more effective” [73]) and similar statements have appeared in the primary literature. In each case, however, there have been no empirical details (i.e., contact times and temperatures for microbicides, strain of challenge virus, methodologies used, etc.) provided and no original references cited to substantiate the efficacy claims. A conference abstract was identified, which provided evidence that a sample inactivant (FA Lysis Buffer) led to >4 log10 inactivation of CCHFV when applied undiluted for 4 min contact time [74]. Efficacy data for other members of the Nairoviridae family, including members that appear to be relatively non-pathogenic for humans and, therefore, could be handled safely in BSL-2 or BSL-3 laboratories, are also sparse. Until the identified knowledge gaps have been resolved, the efficacies of agents shown to be effective for other enveloped viruses may be extrapolated to these nairoviral HFVs.

3.7. Efficacy of Virucidal Approaches for Inactivating Non-Typical Hemorrhagic Fever Paramyxoviruses

The two non-typical HFVs of the Paramyxoviridae family include the Nipah virus and the Hendra virus. These viruses are mentioned in the U.S. Centers for Disease Prevention and Control (CDC) website dedicated to viral hemorrhagic fevers [2], appear in the WHO Priority Disease List [5], and are specified as Priority Pathogens in the 2024 WHO Pathogens Prioritization website [77], yet have not always been included in review articles pertaining to VHF [3,4]. As the list of HFVs is fairly dynamic, and since in severe cases these paramyxoviruses can cause hemorrhage, we have considered these two non-typical HFVs within scope for this review. Both the Nipah and the Hendra viruses are transmitted via various species of Pteropus flying fox bats [2], and spillover animal hosts for the Nipah virus include pigs, dogs, cats, horses, and goats [78,79]. The only known spillover host for the Hendra virus is the horse [80].
While it is not clear that the Nipah virus is transmitted during blood transfusions, investigators have proactively characterized the efficacy and fluence requirements of methylene blue and ultraviolet C or visible light inactivation systems (THERAFLEX UV-Platelets and THERAFLEX MB-Plasma, for inactivating the virus in spiked donor blood platelet concentrates or plasma, respectively) [72].
The results of this literature review (Table 6) indicate that knowledge gaps exist in the cases of surface hygiene with microbicides and hand/skin hygiene agent efficacies for the HFVs from the Paramyxoviridae family. Until the identified knowledge gaps have been resolved, the efficacies of surface and hand/skin hygiene agents shown to be effective for other enveloped viruses may be extrapolated to the paramyxoviral HFVs.

3.8. Efficacy of Virucidal Approaches for Inactivating Hemorrhagic Fever Phenuiviruses

Hemorrhagic fever viruses of the Phenuiviridae family include Rift Valley fever virus (RVFV) in sub-Saharan Africa, the Arabian Peninsula, and certain islands of the Indian Ocean [88]; severe fever with thrombocytopenia syndrome virus (SFTSV) in East and Southeast Asia [89]; and heartland virus (HRTV) in the United States [90]. The vectors for these viruses include various mosquitos (RVFV) and ticks (SFTSV and HRTV) [88,89,90]. Methods for inactivating RVFV in mosquitos during fixation for further assay have been described [88,91].
The results of this literature review (Table 7) indicate that knowledge gaps exist in the cases of surface hygiene with microbicides and hand/skin hygiene agent efficacies for the HFVs from the Phenuiviridae family. In addition, insufficient coverage of the efficacy of microbicides intended for suspension inactivation of phenuiviruses is available. Until the identified knowledge gaps have been resolved, the efficacies of surface and hand/skin hygiene agents and suspension inactivation agents that were shown to be effective for other enveloped viruses may be extrapolated to the phenuiviral HFVs.

4. Discussion

As mentioned in the Introduction, this review of the efficacies of inactivation approaches evaluated specifically for HFVs represents an extension and refocusing of our previous review, assembled in 2021 and published in 2022 [1]. That review was focused on the efficacy of microbicidal approaches for inactivating World Health Organization (WHO) Priority Disease list viruses [5]. While the Priority Disease list in 2022 (and the more current 2024 WHO Pathogens Prioritization website [77]) included a number of diseases associated with HFVs (Crimean–Congo hemorrhagic fever, Ebola virus disease and Marburgvirus disease, Lassa fever, Nipah and henipaviral diseases, and Rift Valley fever) [5,77], these lists also included diseases caused by alphaviruses, coronaviruses, othomyxoviruses, and the flavivirus Zika virus. The latter viruses are not considered HFVs. Diseases caused by certain HFVs of the Flaviviridae family (yellow fever virus, Alkhumra fever virus, dengue virus) and the Hantaviridae family (e.g., Hantaan virus, Sin Nombre virus, and others) have not been included in the WHO Priority Disease lists. These HFVs have, with the exception of yellow fever virus, now been specified as Priority Pathogens in the 2024 WHO Pathogens Prioritization website [77].
In addition to the refocusing of this review exclusively toward HFVs, we have broadened the scope of the review to include not only the efficacies of microbicides but also the efficacies of physical inactivation approaches (such as heat, ultraviolet light in the C range, gamma irradiation, and X-irradiation), which were considered out of scope for the 2022 review [1].
We note that for these HFVs, which typically must be manipulated within BSL-3 or BSL-4 facilities, the chronologically earliest reports of efficacy have pertained to inactivation approaches used in rendering laboratory specimens safe for handling in diagnostic laboratories. This reflects the importance of diagnostic procedures in ascertaining new cases and informing epidemiological inquiries. More recently, studies focusing on inactivation approaches for surface hygiene, liquids, and hand/skin hygiene have been conducted and reported. For example, the amount of data available for these topics for arenaviruses (especially Lassa virus), filoviruses (especially Ebola virus), flaviviruses and paramyxoviruses (especially Nipah virus) has increased considerably in the relatively short time since the writing of our 2022 review [1].
A substantial knowledge base for the inactivation of filoviruses, including various variants of the Ebola virus, Reston virus, Sudan virus, and Marburg virus, is now available in the primary literature. This pertains to each of the different inactivation applications (surface hygiene, suspension inactivation, hand/skin hygiene, and decontamination of laboratory specimens). Of course, as is the case for each of the HFVs considered in this review, data on air sanitization approaches are lacking for the filoviruses. This likely reflects the relative difficulties and dangers associated with the conduct of such aerobiology studies using lethal aerosolized challenge viruses. However, efficacy studies intended to determine the in-air virucidal activity of air sanitizers against experimentally aerosolized surrogate enveloped and non-enveloped viruses have been reported [21,97]. On the basis of the hierarchy of pathogen susceptibility to microbicides, an air sanitizer demonstrating virucidal activity against airborne non-enveloped viruses should also be effective against airborne HFVs in general, as the latter are lipid-enveloped viruses [98,99].
We can rapidly summarize the most significant remaining knowledge gaps for the inactivation of HFVs based on the results of this current review. For instance, in all cases other than the filoviruses, there are limited efficacy data available pertaining to surface and hand/skin hygiene agents. The hemorrhagic fever virus family for which the least amount of inactivation efficacy information is currently available is the Nairoviridae. This suggests that future research should be focused on the Crimean–Congo hemorrhagic fever virus or its less pathogenic family member, the Hazara virus.
Until such data become available, it must be recognized that since each of the HFVs considered in this review are relatively large, lipid-enveloped RNA viruses, inactivation approaches that are shown to be effective for surface hygiene, liquid disinfection, or hand/skin hygiene for the filoviruses are also likely to be effective for the other families of HFVs. This position is summed up nicely by Weber et al. [100]: “However, once the nature of the emerging disease is known (i.e, bacteria, non-enveloped virus, enveloped virus), it is possible to determine the proper antiseptic and disinfectant, even in the absence of studies of the exact infectious agent. For example, an enveloped virus (e.g., Lassa, EVD, MERS-CoV, SARS-CoV, influenza A) would be inactivated by any agent active against vegetative bacteria, non-enveloped viruses, or mycobacteria” [100]. This position is also reflected in the U.S. EPA guidance Disinfectants for Emerging Viral Pathogens (EVPs): List Q [101]. The lipid envelope is an effective target for microbicides because it is a virally modified, host-cell-derived, phospholipid bilayer with associated glycoproteins, which (especially the spike glycoproteins) interact with the cellular receptors required for initiation of viral infection of the host cells [98,99].
It might be questioned by some whether hygiene (sanitization) agents are required for environmental surfaces, hand/skin, or air for HFVs known to be conveyed by insect, rodent, or mammalian vectors. While the proximate sources (reservoirs) of the various HFVs may indeed be the insect or animal vectors, there are indications that human-to-human, environmental surface-to-human, and air-to-human transmission may also be relevant for certain HFVs [102]. For example, Lassa fever may be acquired through touching surfaces (fomites) contaminated with the virus, by eating contaminated food (including the rodent vector), by inhaling air contaminated with the virus (which may contain virus-contaminated urine or feces aerosolized through human activities such as sweeping) or following exposure to bodily fluids of an infected person [23,102,103,104]. At 30% RH and 24–32 °C, the infectivity half-life of aerosolized Lassa virus Josiah strain has been reported to be 10 to 55 min [104]. The time required to reduce the surface (glass) infectious Lassa virus Josiah strain titer by 1 log10 has been reported to be 53 h at 30–40% RH and 20–25 °C in the dark [105]. The times required to reduce the surface infectious Lassa virus Josiah strain and Sauerwald strain titers by 1 log10 at room temperature were 13 h and 24 h, respectively, on high-density polyethylene surfaces and 10 h and 20 h, respectively, on stainless-steel surfaces [27]. The considerations discussed above suggest that targeted surface hygiene may represent a useful non-pharmaceutical intervention for mitigating the exposure risk to the Lassa virus.
In the case of the Ebola virus, while many cases appear to be transmitted directly through contact with the mammalian vector (fruit bats), human-to-human transmission as a result of contact with contaminated body fluids or excretions or exposure to airborne virus may also occur [102,106,107]. Indirect transmission through contact with contaminated fomites has also been considered [107,108]. The time required to reduce the surface (glass) infectious Zaire Ebola virus titer by 1 log10 has been reported to be 35 h at 30–40% RH and 20–25 °C in the dark [105]. Cook et al. reported similar results for EBOV/Mak [38], i.e., the time required to reduce the infectious titer by 1 log10 was found to be 30 h on stainless steel at 21.5 °C and 30% RH. Piercy et al. [109] reported the infectivity half-lives for aerosolized Zaire Ebola virus and Lake Victoria Marburg virus at 50–55% RH and 19–25 °C to be 104 min and 93 min, respectively. The filoviruses represent another case where the use of targeted surface hygiene in the field may help to mitigate transmission risk.
The flaviviral HFVs are transmitted exclusively through insect vectors, and studies on persistence on environmental surfaces or in the air were not identified during the literature search [102]. The hantaviral HFVs are thought to be transmitted both by direct contact with the vectors and indirectly through contact with contaminated fomites [66,102]. The nairovirus Crimean–Congo hemorrhagic fever virus primarily is transmitted directly to humans via the insect vector, although human-to-human transmission via contaminated bodily fluids is also possible, as is transmission through exposure to contaminated aerosols [73]. The persistence of infectious Hantaan virus strain 76–118 and Crimean–Congo hemorrhagic fever virus strain IbAr 10200 on aluminum discs at 20 °C was investigated by Hardestam et al. [67]. The times required to reduce the infectious titers by 1 log10 were found to be ~60 min for the Hantaan virus and ~90 min for the Crimean–Congo hemorrhagic fever virus [67].
Nipah and Hendra viruses are thought to be transmitted to humans through contact with the animal reservoir species or with food or fomites contaminated with excretions from the reservoir species [79,102]. Human-to-human transmission is also thought to occur in the case of the Nipah virus but has not been reported for the Hendra virus [79]. The persistence of these paramyxoviral HFVs on surfaces has not been investigated, to our knowledge. The infectivity half-life of aerosolized Nipah virus Malaysia at 19–21 °C and 42–57% RH in the dark was reported to be 47 min [82]. The phenuivirus Rift Valley fever virus is transmitted to humans via the insect vector and by contact with organs or excretions of infected animals; human-to-human transmission has not been reported [110]. Published data on the persistence of infectious RVFV on surfaces or in air were not identified during the literature search. Nipah virus is of particular concern among HFVs as it displays potential for rapid human-to-human transmission, has a high case fatality rate, and a specific antiviral treatment is lacking [111,112].
The limitations of this review include the following:
  • Since the stated goal of the review was to identify inactivation efficacy information specifically for the HFVs, certain information available for family members not considered to be HFVs (especially of the Flaviviridae and the Paramyxoviridae) have not been included in the tabular summaries;
  • Secondly, the emergence of new HFVs within the various virus families discussed in this review is very dynamic. Not all currently known HFVs within these families may have been mentioned. This is especially true for the arenaviruses and the hantaviruses. On the other hand, our tabular summaries provide information for two paramyxoviruses that may be considered non-typical HFVs as the resulting symptoms—though more neurological in nature—do include hemorrhages [2,113,114];
  • Thirdly, the tabular information assembled represents primary empirical data only. Secondary literature information has been excluded from the tables. In addition, there are some predictive data that have not been included in the tables presented. An example of this type of data is the prediction of the susceptibilities of HFVs to ultraviolet light in the C range (UV-C, 254 nm) by Lytle and Sagripanti [115]. The predicted UV-C susceptibilities were found to be similar for the various HFVs considered (Marburg virus, Ebola virus, Hanta virus, Rift Valley fever virus, Lassa virus, and Junin virus), with decimal reduction (D) values (the fluence of 254 nm radiation required to inactivate 1 log10 of HFVs) ranging from 1.7 to 3.0 mJ/cm2 [115];
  • Fourthly, the efficacies of certain less commonly used inactivation approaches for HFVs, including photodynamic methods (e.g., psoralen + ultraviolet light in the A range [116,117]; methylene blue + visible light [72]) and high-hydrostatic pressure inactivation [118], have not been included within the tables provided in this review as the methods are rather niche approaches for the described applications or require specialized devices that are not widely available in research and diagnostic laboratories globally.
This review represents a snapshot in time as additional inactivation efficacy studies for HFVs are being published on a continuing basis. It is hoped that, despite the various limitations discussed above, the review provides an up-to-date listing of the topical information available as of the beginning of 2025 and that readers and investigators conducting research on HFVs will find this compilation to be useful.

Author Contributions

Conceptualization, R.W.N. and M.K.I.; methodology, R.W.N. and M.K.I.; investigation, R.W.N. and M.K.I.; data curation, R.W.N. and M.K.I.; writing—original draft preparation, R.W.N.; writing—review and editing, R.W.N. and M.K.I. All authors have read and agreed to the published version of the manuscript.

Funding

This research received no external funding.

Data Availability Statement

This is a review article. All original data may be obtained from the literature cited.

Conflicts of Interest

Raymond W. Nims is employed by Syner-G BioPharma, and M. Khalid Ijaz is employed by Reckitt Benckiser LLC. The authors declare no conflicts of interest.

References

  1. Ijaz, M.K.; Nims, R.W.; Cutts, T.A.; McKinney, J.; Gerba, C.P. Predicted and measured virucidal efficacies of microbicides for emerging and reemerging viruses associated with WHO priority diseases. In Disinfection of Viruses; Nims, R.W., Ijaz, M.K., Eds.; Intech Open: London, UK, 2022. [Google Scholar] [CrossRef]
  2. U.S. CDC. About Viral Hemorrhagic Fevers. Fact Sheet. Available online: https://www.cdc.gov/viral-hemorrhagic-fevers/about/index.html (accessed on 10 April 2025).
  3. Pigott, D.C. Hemorrhagic fever viruses. Crit. Care Clin. 2005, 21, 765–783. [Google Scholar] [CrossRef] [PubMed]
  4. Flórez-Álvarez, L.; de Souza, E.E.; Botosso, V.F.; de Oliveira, D.B.L.; Ho, P.L.; Taborda, C.P.; Palmisano, G.; Capurro, M.L.; Pinho, J.R.R.; Ferreira, H.L.; et al. Hemorrhagic fever viruses: Pathogenesis, therapeutics, and emerging and re-emerging potential. Front. Microbiol. 2022, 13, 1040093. [Google Scholar] [CrossRef]
  5. World Health Organization. Prioritizing Diseases for Research and Development in Emergency Contexts. 2021. Available online: https://www.who.int/activities/prioritizing-diseases-for-research-and-development-in-emergency-contexts (accessed on 10 April 2025).
  6. Spaulding, E.H. Chemical disinfection of medical and surgical materials. In Disinfection, Sterilization, & Preservation, 3rd ed.; Block, S., Ed.; Lea & Febiger: Philadelphia, PA, USA, 1968. [Google Scholar]
  7. U.S. Environmental Protection Agency. Guidance to Registrants: Process for Making Claims Against Emerging Viral Pathogens not on EPA-Registered Disinfectant Labels. 2016. Available online: https://www.epa.gov/sites/default/files/2016-09/documents/emerging_viral_pathogen_program_guidance_final_8_19_16_001_0.pdf (accessed on 10 April 2025).
  8. U.S. Environmental Protection Agency. Emerging Viral Pathogen Guidance for Antimicrobial Pesticides. 2021. Available online: https://www.epa.gov/pesticide-registration/emerging-viral-pathogen-guidance-antimicrobial-pesticides (accessed on 10 April 2025).
  9. Eggers, M.; Schwebke, I.; Suchomel, M.; Fotheringham, V.; Gebel, J.; Meyer, B.; Morace, G.; Roedger, H.J.; Roques, C.; Visa, P.; et al. The European tiered approach for virucidal efficacy testing–rationale for rapidly selecting disinfectants against emerging and re-emerging viral diseases. EuroSurveillance 2021, 26, 2000708. [Google Scholar] [CrossRef]
  10. Nims, R.W.; Zhou, S.S. Intra-family differences in efficacy of inactivation of small, non-enveloped viruses. Biologicals 2016, 44, 456–462. [Google Scholar] [CrossRef] [PubMed]
  11. Zhou, S.S. Variation in resistance among enveloped and non-enveloped viruses to chemical treatments. In Disinfection of Viruses; Nims, R.W., Ijaz, M.K., Eds.; Intech Open: London, UK, 2022; Available online: https://www.intechopen.com/chapters/80772 (accessed on 10 April 2025).
  12. Elveborg, S.; Monteil, V.M.; Mirazimi, A. Methods of inactivation of highly pathogenic viruses for molecular, serology or vaccine development purposes. Pathogens 2022, 11, 271. [Google Scholar] [CrossRef]
  13. Hossain, F. Sources, enumerations and inactivation mechanisms of four emerging viruses in aqueous phase. J. Water Health 2022, 20, 396–440. [Google Scholar] [CrossRef]
  14. Gerba, C.P.; Boone, S.; Nims, R.W.; Maillard, J.-Y.; Sattar, S.A.; Rubino, J.R.; McKinney, J.; Ijaz, M.K. Mechanisms of action of microbicides commonly used in infection prevention and control. Microbiol. Mol. Biol. Rev. 2024, 88, e0020522. [Google Scholar] [CrossRef] [PubMed]
  15. Nims, R.W.; Plavsic, M. Physical inactivation of SARS-CoV-2 and other coronaviruses: A review. In Disinfection of Viruses; Nims, R.W., Ijaz, M.K., Eds.; Intech Open: London, UK, 2022; Available online: https://www.intechopen.com/chapters/81019 (accessed on 10 April 2025).
  16. ASTM E1053-20; Standard Practice to Assess Virucidal Activity of Chemicals Intended for Disinfection of Inanimate, Nonporous Environmental Surfaces. ASTM International: West Conshohocken, PA, USA, 2020. Available online: https://store.astm.org/standards/e1053 (accessed on 10 April 2025).
  17. ASTM E1052-20; Standard Practice to Assess the Activity of Microbicides Against Viruses in Suspension. ASTM International: West Conshohocken, PA, USA, 2020. Available online: https://store.astm.org/e1052-20.html (accessed on 10 April 2025).
  18. BS EN 14476:2013+A2:2019; Chemical Disinfectants and Antiseptics. Quantitative Suspension Test for the Evaluation of Virucidal Activity in the Medical Area. Test Method and Requirements (Phase 2/Step 1). British Standards Institute: London, UK, 2019. Available online: https://www.en-standard.eu/bs-en-14476-2013-a2-2019-chemical-disinfectants-and-antiseptics-quantitative-suspension-test-for-the-evaluation-of-virucidal-activity-in-the-medical-area-test-method-and-requirements-phase-2-step-1/ (accessed on 10 April 2025).
  19. U.S. Environmental Protection Agency. OCSPP 810.2500-Air Sanitizers_2012-03-12 [EPA 730-C-11-003]. 2012. Available online: https://www.regulations.gov/document/EPA-HQ-OPPT-2009-0150-0025 (accessed on 10 April 2025).
  20. E3273-21; Standard Practice to Assess Microbial Decontamination of Indoor Air Using an Aerobiology Chamber. ASTM International: West Conshohocken, PA, USA, 2021. [CrossRef]
  21. Ijaz, M.K.; Zargar, B.; Nims, R.W.; McKinney, J.; Sattar, S.A. Rapid virucidal activity of an air sanitizer against airborne bacteriophage Phi6 and MS2 surrogates for non-enveloped and enveloped vertebrate viruses, including SARS-CoV-2. Appl. Environ. Microbiol. 2024, 91, e01426-24. [Google Scholar] [CrossRef]
  22. Springthorpe, V.S.; Sattar, S.A. Application of a quantitative carrier test to evaluate microbicides against mycobacteria. J. AOAC Int. 2007, 90, 817–824. [Google Scholar] [CrossRef]
  23. U.S. CDC. About Lassa Fever. 2024. Available online: https://www.cdc.gov/lassa-fever/about/index.html (accessed on 10 April 2025).
  24. Olschewski, S.; Thielbein, A.; Hoffmann, C.; Blake, O.; Müller, J.; Bockholt, S.; Pallasch, E.; Hinzmann, J.; Wurr, S.; Neddersen, N.; et al. Validation of inactivation methods for arenaviruses. Viruses 2021, 13, 968. [Google Scholar] [CrossRef]
  25. Sagripanti, J.-L.; Lytle, C.D. Sensitivity to ultraviolet radiation of Lassa, vaccinia, and Ebola viruses dried on surfaces. J. Arch. Virol. 2011, 156, 489–494. [Google Scholar] [CrossRef] [PubMed]
  26. Sagripanti, J.-L.; Routson, L.B.; Lytle, C.D. Virus inactivation by copper or iron ions alone and in the presence of peroxide. Appl. Environ. Microbiol. 1993, 59, 4374–4376. [Google Scholar] [CrossRef] [PubMed]
  27. Shaffer, M.; Fischer, R.J.; Gallogly, S.; Ginn, O.; Munster, V.; Bibby, K. Environmental persistence and disinfection of Lassa virus. Emerg. Infect. Dis. 2023, 29, 2285–2291. [Google Scholar] [CrossRef]
  28. Cutts, T.A.; Nims, R.W.; Rubino, J.R.; McKinney, J.; Kuhn, J.; Ijaz, M.K. Efficacy of microbicidal actives and formulations for inactivation of Lassa virus in suspension. Sci. Rep. 2023, 13, 12983. [Google Scholar] [CrossRef] [PubMed]
  29. Elliott, L.H.; McCormick, J.B.; Johnson, K.M. Inactivation of Lassa, Marburg, and Ebola viruses by gamma irradiation. J. Clin. Med. 1982, 16, 704–708. [Google Scholar] [CrossRef]
  30. Mitchell, S.W.; McCormick, J.B. Physicochemical inactivation of Lassa, Ebola, and Marburg viruses and effect on clinical laboratory analyses. J. Clin. Microbiol. 1984, 20, 486–489. [Google Scholar] [CrossRef]
  31. Kochel, T.J.; Kocher, G.A.; Ksiazek, T.G.; Burans, J.P. Evaluation of Trizol LS inactivation of viruses. ABSA Int. 2017, 22, 52–55. [Google Scholar] [CrossRef]
  32. Cutts, T.; Leung, A.; Banadyga, L.; Krishnan, J. Inactivation validation of Ebola, Marburg, and Lassa viruses in AVL and ethanol-treated viral cultures. Viruses 2024, 16, 1354. [Google Scholar] [CrossRef]
  33. Lloyd, G.; Bowen, E.T.W.; Slade, J.H.R. Physical and chemical methods of inactivating Lassa virus. Lancet 1982, 1, 1046–1048. [Google Scholar] [CrossRef]
  34. Retterer, C.; Kenny, T.; Zamani, R.; Altamura, L.A.; Kearney, B.; Jaissle, J.; Coyne, S.; Olschner, S.; Harbourt, D. Strategies for validation of inactivation of viruses with Trizol® LS and formalin solutions. Appl. Biosaf. 2020, 25, 74–82. [Google Scholar] [CrossRef]
  35. Feldmann, F.; Shupert, W.L.; Haddock, E.; Twardoski, B.; Feldmann, H. Gamma irradiation as an effective method for inactivation of emerging viruses. Am. J. Trop. Med. Hyg. 2019, 100, 1275–1277. [Google Scholar] [CrossRef]
  36. Olejnik, J.; Hume, A.J.; Ross, S.J.; Scoon, W.A.; Seitz, S.; White, M.R.; Slutzky, B.; Yun, N.E.; Mühlberger, E. Art of the kill: Designing and testing viral inactivation procedures for highly pathogenic negative sense RNA viruses. Pathogens 2023, 12, 952. [Google Scholar] [CrossRef]
  37. Kuhn, J.H.; Amarasinghe, G.K.; Basler, C.F.; Bavari, S.; Bukreyev, A.; Chandran, K.; Crozier, I.; Dolnick, O.; Dye, J.M.; Formenty, P.B.H.; et al. ICTV virus taxonomy profile: Filoviridae. J. Gen. Virol. 2019, 100, 911–912. [Google Scholar] [CrossRef]
  38. Cook, B.W.M.; Cutts, T.A.; Nikiforuk, A.M.; Poliquin, P.G.; Court, D.A.; Strong, J.E.; Theriault, S.S. Evaluating environmental persistence and disinfection of the Ebola virus Makona variant. Viruses 2015, 7, 1975–1986. [Google Scholar] [CrossRef]
  39. Cook, B.W.M.; Cutts, T.A.; Nikiforuk, A.M.; Leung, A.; Kobasa, D.; Theriault, S.S. The disinfection characteristics of Ebola virus outbreak variants. Sci. Rep. 2016, 6, 38293. [Google Scholar] [CrossRef]
  40. Smither, S.J.; Eastaugh, L.; Filone, C.M.; Freeburger, D.; Herzog, A.; Lever, M.S.; Miller, D.M.; Mitzel, D.; Noah, J.W.; Reddick-Elick, M.S.; et al. Two-center evaluation of disinfectant efficacy against Ebola virus in clinical and laboratory matrices. Emerg. Infect. Dis. 2018, 24, 135–139. [Google Scholar] [CrossRef]
  41. Cutts, T.A.; Robertson, C.; Theriault, S.S.; Nims, R.W.; Kasloff, S.B.; Rubino, J.R.; Ijaz, M.K. Efficacy of microbicides for inactivation of Ebola-Makona virus on a non-porous surface: A targeted hygiene intervention for reducing virus spread. Sci. Rep. 2020, 10, 15247. [Google Scholar] [CrossRef]
  42. Cutts, T.A.; Kasloff, S.B.; Krishnan, J.; Nims, R.W.; Theriault, S.S.; Rubino, J.R.; Ijaz, M.K. Comparison of the efficacy of disinfectant pre-impregnated wipes for decontaminating stainless steel carriers experimentally inoculated with Ebola virus and vesicular stomatitis virus. Front. Publ. Health 2021, 9, 657443. [Google Scholar] [CrossRef]
  43. Smither, S.; Phelps, A.; Eastaugh, L.; Ngugi, S.; O’Brien, L.; Dutch, A.; Lever, M.S. Effectiveness of four disinfectants against Ebola virus on different materials. Viruses 2016, 8, 185. [Google Scholar] [CrossRef]
  44. Bibby, K.; Fischer, R.J.; Casson, L.W.; de Carvalho, N.A.; Haas, C.N.; Munster, V.J. Disinfection of Ebola virus in sterilized municipal wastewater. PLoS Negl. Trop. Dis. 2017, 11, e0005299. [Google Scholar] [CrossRef]
  45. Eggers, M.; Eickmann, M.; Kowalski, K.; Zorn, J.; Reimer, K. Povidone-iodine hand wash and hand rub products demonstrated excellent in vitro virucidal efficacy against Ebola virus and modified vaccinia virus Ankara, the new European test virus for enveloped viruses. BMC Infect. Dis. 2015, 15, 375. [Google Scholar] [CrossRef]
  46. Lupton, H.W. Inactivation of Ebola virus with 60Co irradiation. J. Infect. Dis. 1981, 143, 291. [Google Scholar] [CrossRef]
  47. Cutts, T.A.; Ijaz, M.K.; Nims, R.W.; Rubino, J.R.; Theriault, S.S. Effectiveness of Dettol Antiseptic Liquid for inactivation of Ebola virus in suspension. Sci. Rep. 2019, 9, 6590. [Google Scholar] [CrossRef]
  48. Cutts, T.A.; Nims, R.W.; Theriault, S.S.; Bruning, E.; Rubino, J.R.; Ijaz, M.K. Hand hygiene: Virucidal efficacy of a liquid hand wash product against Ebola virus. Infect. Prev. Pract. 2021, 3, 100122. [Google Scholar] [CrossRef]
  49. Siddharta, A.; Pfaender, S.; Vielle, N.J.; Dijkman, R.; Friesland, M.; Becker, B.; Yang, J.; Engelmann, M.; Todt, D.; Windisch, M.P.; et al. Virucidal activity of World Health Organization-recommended formulations against enveloped viruses, including Zika, Ebola, and emerging coronaviruses. J. Infect. Dis. 2017, 215, 902–906. [Google Scholar] [CrossRef]
  50. Colavita, F.; Quartu, S.; Lalle, E.; Bordi, L.; Lapa, D.; Meschi, S.; Vulcano, A.; Toffoletti, A.; Bordi, E.; Paglia, M.G.; et al. Evaluation of the inactivation effect of Triton X-100 on Ebola virus infectivity. J. Clin. Virol. 2017, 86, 27–30. [Google Scholar] [CrossRef]
  51. van Kampen, J.J.A.; Tintu, A.; Russcher, H.; Fraaij, P.L.A.; Reusken, C.B.E.M.; Rijken, M.; van Hellemond, J.J.; van Genderen, P.J.; Koelewijn, R.; de Jong, M.D.; et al. Ebola virus inactivation by detergents is annulled in serum. J. Infect. Dis. 2017, 216, 859–866. [Google Scholar] [CrossRef]
  52. Boytz, R.; Seitz, S.; Guadiano, E.; Patten, J.J.; Keiser, P.T.; Connor, J.H.; Sharpe, A.H.; Davey, R.A. Inactivation of Ebola virus and SARS-CoV-2 in cell culture supernatants and cell pellets by gamma irradiation. Viruses 2023, 15, 43. [Google Scholar] [CrossRef]
  53. Burton, J.E.; Easterbrook, L.; Pitman, J.; Anderson, D.; Roddy, S.; Bailey, D.; Vipond, R.; Bruce, C.B.; Roberts, A.D. The effect of a non-denaturing detergent and a guanidinium-based inactivation agent on the viability of Ebola virus in mock clinical serum samples. J. Virol. Meth. 2017, 250, 34–40. [Google Scholar] [CrossRef]
  54. Blow, J.A.; Dohm, D.J.; Negley, D.L.; Mores, C.N. Virus inactivation by nucleic acid extraction reagents. J. Virol. Meth. 2004, 119, 195–198. [Google Scholar] [CrossRef]
  55. Alfson, K.J.; Griffiths, A. Development and testing of a method for validating chemical inactivation of Ebola virus. Viruses 2018, 10, 126. [Google Scholar] [CrossRef]
  56. Smither, S.J.; Weller, S.A.; Phelps, A.; Eastaugh, L.; Ngugi, S.; O’Brien, L.M.; Steward, J.; Lonsdale, S.G.; Lever, M.S. Buffer AVL alone does not inactivate Ebola virus in a representative clinical sample type. J. Clin. Microbiol. 2015, 53, 3148–3154. [Google Scholar] [CrossRef]
  57. Bhatia, B.; Feldmann, H.; Marzi, A. Kyasanur Forest disease and Alkhurma hemorrhagic fever virus—Two neglected zoonotic pathogens. Microorganisms 2020, 8, 1406. [Google Scholar] [CrossRef]
  58. Meister, T.L.; Frericks, N.; Kleinert, R.D.V.; Rodriguez, E.; Steinmann, J.; Todt, D.; Brown, R.J.P.; Steinmann, E. Inactivation of yellow fever virus by WHO-recommended hand rub formulations and surface disinfectants. PLoS Negl. Trop. Dis. 2024, 18, e0012264. [Google Scholar] [CrossRef]
  59. Amanna, I.J.; Raué, H.P.; Slifka, M.K. Development of a new hydrogen peroxide-based vaccine platform. Nat. Med. 2012, 18, 974–979. [Google Scholar] [CrossRef]
  60. Gröner, A.; Broumis, C.; Fang, R.; Nowak, T.; Popp, B.; Schäfer, W.; Roth, N.J. Effective inactivation of a wide range of viruses by pasteurization. Transfusion 2018, 58, 41–51. [Google Scholar] [CrossRef]
  61. Madani, T.A.; Abuelzein, E.-T.M.E.; Azhar, E.I.; Al-Bar, H.M.S. Thermal inactivation of Alkhumra hemorrhagic fever virus. Arch. Virol. 2014, 159, 2687–2691. [Google Scholar] [CrossRef]
  62. Loterio, R.K.; Rosevear, K.; Edenborough, K.; Fraser, J.E. Complete inactivation of orthoflavi- and alphaviruses by acetone for safe titering by ELISA. J. Virol. Meth. 2025, 335, 115146. [Google Scholar] [CrossRef]
  63. Idris, F.; Muharram, S.H.; Zaini, Z.; Diah, S. Effectiveness of physical inactivation methods of dengue virus: Heat-versus UV-inactivation. bioRxiv 2018. Available online: https://www.biorxiv.org/content/10.1101/427666v1 (accessed on 10 April 2025).
  64. Jacob, A.T.; Ziegler, B.M.; Farha, S.M.; Vivian, L.R.; Zilinski, C.A.; Armstrong, A.R.; Burdette, A.J.; Beachboard, D.C.; Stobart, C.C. Sin Nombre virus and the emergence of other hantaviruses: A review of the biology, ecology, and disease of a zoonotic pathogen. Biology 2023, 12, 1413. [Google Scholar] [CrossRef]
  65. The Center for Food Security and Public Health, Iowa State University. Hantavirus Disease. 2018. Available online: https://www.cfsph.iastate.edu/Factsheets/pdfs/hantavirus.pdf (accessed on 10 April 2025).
  66. Kallio, E.R.; Klingström, J.; Gustafsson, E.; Manni, T.; Vaheri, A.; Henttonen, H.; Vapalahti, O.; Lundkvist, A. Prolonged survival of Puumala hantavirus outside of the host: Evidence for indirect transmission via the environment. J. Gen. Virol. 2006, 87, 2127–2134. [Google Scholar] [CrossRef]
  67. Hardestam, J.; Simon, M.; Hedlund, K.O.; Vaheri, A.; Klingström, J.; Lundkvist, Å. Ex vivo stability of the rodent-borne Hantaan virus in comparison to that of arthropod-borne members of the Bunyaviridae family. Appl. Environ. Microbiol. 2007, 73, 2547–2551. [Google Scholar] [CrossRef]
  68. Maes, P.; Li, S.; Verbeek, J.; Keyaerts, E.; Clement, J.; Van Ranst, M. Evaluation of the efficacy of disinfectants against Puumala hantavirus by real-time RT-PCR. J. Virol. Meth. 2007, 141, 111–115. [Google Scholar] [CrossRef]
  69. Egorova, M.S.; Kurashova, S.S.; Dzagurova, T.K.; Balovneva, M.V.; Ishmukhametov, A.A.; Tkachenko, E.A. Effect of virus-inactivating agents on the immunogenicity of hantavirus vaccines against hemorrhagic fever with renal syndrome. Appl. Biochem. Microbiol. 2020, 56, 940–947. [Google Scholar] [CrossRef]
  70. Kraus, A.A.; Priemer, C.; Heider, H.; Kruger, D.H.; Ulrich, R. Inactivation of Hantaan virus-containing samples for subsequent investigations outside biosafety level 3 facilities. Intervirology 2005, 48, 255–261. [Google Scholar] [CrossRef]
  71. Mishra, A.K.; Mover, C.L.; Abelson, D.M.; Deer, D.J.; El Omari, K.; Duman, R.; Lobel, L.; Lutwama, J.J.; Dye, J.M.; Wagner, A.; et al. Structure and characterization of Crimean-Congo hemorrhagic fever virus GP38. J. Virol. 2020, 94, e02005-19. [Google Scholar] [CrossRef]
  72. Eickmann, M.; Gravemann, U.; Handke, W.; Tolksdorf, F.; Reichenberg, S.; Müller, T.H.; Seltsam, A. Inactivation of three emerging viruses—Severe acute respiratory syndrome coronavirus, Crimean-Congo haemorrhagic fever virus and Nipah virus—In platelet concentrates by ultraviolet C light, and in plasma by methylene blue plus visible light. Vox Sanguin. 2020, 115, 146–151. [Google Scholar] [CrossRef]
  73. The Center for Food Security and Public Health, Iowa State University, College of Veterinary Medicine. Crimean-Congo Hemorrhagic Fever. 2019. Available online: https://www.cfsph.iastate.edu/Factsheets/pdfs/crimean_congo_hemorrhagic_fever.pdf (accessed on 10 April 2025).
  74. Ferraris, O.; Gay-Andrieu, F.; Moroso, M.; Jarjaval, F.; Miller, M.; Peyrefitte, C.N. Complete hemorrhagic fever virus inactivation during lysis in the FilmArray BioThreat-E assay demonstrates the biosafety of this test. In Proceedings of the 3rd International CBRNE Research & Innovation Conference, Nantes, France, 20–23 May 2019; Available online: https://www.biofiredefense.com/wp-content/uploads/2019/06/20180529_Poster-Biofire_CBRNE-2019.pdf (accessed on 10 April 2025).
  75. Saluzzo, J.F.; Leguenno, B.; Van der Groen, G. Use of heat inactivated viral haemorrhagic fever antigens in serological assays. J. Virol. Meth. 1988, 22, 165–172. [Google Scholar] [CrossRef]
  76. Afrough, B.; Eakins, J.; Durley-White, S.; Dowall, S.; Findlay-Wilson, S.; Graham, V.; Lewandowski, K.; Carter, D.P.; Hewson, R. X-ray inactivation of RNA viruses without loss of biological characteristics. Sci. Rep. 2020, 10, 21431. [Google Scholar] [CrossRef]
  77. World Health Organization. Pathogens Prioritization. 2024. Available online: https://cdn.who.int/media/docs/default-source/consultation-rdb/prioritization-pathogens-v6final.pdf?sfvrsn=c98effa7_7&download=true (accessed on 10 April 2025).
  78. The Center for Food Security and Public Health, Iowa State University, College of Veterinary Medicine. Nipah Virus Infection. 2016. Available online: https://www.cfsph.iastate.edu/Factsheets/pdfs/nipah.pdf (accessed on 10 April 2025).
  79. Branda, F.; Ceccarelli, G.; Giovenetti, M.; Albanese, M.; Binetti, E.; Ciccozzi, M.; Scarpa, F. Nipah virus: A zoonotic threat reemerging in the wake of global public health challenges. Microorganisms 2025, 13, 124. [Google Scholar] [CrossRef]
  80. The Center for Food Security and Public Health, Iowa State University, College of Veterinary Medicine. Hendra Virus Infection. 2024. Available online: https://www.cfsph.iastate.edu/Factsheets/pdfs/hendra.pdf (accessed on 10 April 2025).
  81. Huang, Y.; Xiao, S.; Song, D.; Yuan, Z. Evaluation and comparison of three virucidal agents on inactivation of Nipah virus. Sci. Rep. 2022, 12, 11365. [Google Scholar] [CrossRef]
  82. Smither, S.J.; Eastaugh, L.S.; O’Brien, L.M.; Phelps, A.L.; Lever, M.S. Aerosol survival, disinfection and formalin inactivation of Nipah virus. Viruses 2022, 14, 2057. [Google Scholar] [CrossRef] [PubMed]
  83. Fogarty, R.; Halpin, K.; Hyatt, A.D.; Daszak, P.; Mungall, B.A. Henipavirus susceptibility to environmental variables. Virus Res. 2008, 132, 140–144. [Google Scholar] [CrossRef]
  84. Widerspick, L.; Vázquez, C.A.; Niemetz, L.; Heung, M.; Olal, C.; Bencsik, A.; Henkel, C.; Pfister, A.; Brunetti, J.E.; Kucinskaite-Kodze, I.; et al. Inactivation methods for experimental Nipah virus infection. Viruses 2022, 14, 1052. [Google Scholar] [CrossRef]
  85. Watanabe, S.; Fukushi, S.; Harada, T.; Shimojima, M.; Yoshikawa, T.; Kurosu, T.; Kaku, Y.; Morikawa, S.; Saijo, M. Effective inactivation of Nipah virus in serum samples for safe processing in low-containment laboratories. Virol. J. 2020, 17, 151. [Google Scholar] [CrossRef]
  86. Edwards, S.J.; Caruso, S.; Suen, W.W.; Jackson, S.; Rowe, B.; Marsh, G.A. Evaluation of henipavirus chemical inactivation methods for the safe removal of samples from the high-containment PC4 laboratory. J. Virol. Meth. 2021, 298, 114287. [Google Scholar] [CrossRef]
  87. Hume, A.J.; Olejnik, J.; White, M.R.; Huang, J.; Turcinovic, J.; Heiden, B.; Bawa, P.S.; Williams, C.J.; Gorman, N.G.; Alekseyev, Y.O.; et al. Heat inactivation of Nipah virus for downstream single-cell RNA sequencing does not interfere with sample quality. Pathogens 2024, 13, 62. [Google Scholar] [CrossRef]
  88. Bergren, N.A.; Patterson, E.I.; Blair, H.; Ellis, R.P.; Kading, R.C. Methods for successful inactivation of Rift Valley fever virus in infected mosquitos. J. Virol. Meth. 2020, 276, 113794. [Google Scholar] [CrossRef]
  89. Harada, T.; Fukushi, S.; Kurosu, T.; Yoshikawa, T.; Shimojima, M.; Tanabayashi, K.; Saijo, M. Inactivation of severe fever with thrombocytopenia syndrome virus for improved laboratory safety. J. Biosaf. Biosec. 2020, 2, 31–35. [Google Scholar] [CrossRef]
  90. Dembek, Z.F.; Mothershead, J.L.; Cirimotich, C.M.; Wu, A. Heartland virus disease—An underreported emerging infection. Microorganisms 2024, 12, 286. [Google Scholar] [CrossRef] [PubMed]
  91. Kading, R.; Crabtree, M.; Miller, B. Inactivation of infectious virus and serological detection of virus antigen in Rift Valley fever virus-exposed mosquitos fixed with paraformaldehyde. J. Virol. Meth. 2013, 189, 184–188. [Google Scholar] [CrossRef]
  92. Romeo, M.A.; Specchiarello, E.; Mija, C.; Zulian, V.; Francalancia, M.; Maggi, F.; Garbuglia, A.R.; Lapa, D. Heat treatment as a safe-handling procedure for Rift Valley fever virus. Pathogens 2024, 13, 1089. [Google Scholar] [CrossRef]
  93. Al-Olayan, E.M.; Mohamed, A.F.; El-Khadraqy, M.F.; Shebl, R.I.; Yehia, H.M. An alternative inactivant for Rift Valley fever virus using cobra venom-derived L-amino oxidase, which is related to its immune potential. Braz. Arch. Biol. Technol. 2016, 59, e16160044. [Google Scholar] [CrossRef]
  94. Hartman, A.L.; Cole, K.S.; Homer, L.C. Verification of inactivation methods for removal of biological materials from a biosafety level 3 select agent facility. Appl. Biosaf. 2012, 17, 70–75. [Google Scholar] [CrossRef]
  95. Rangel, M.V.; Bourguet, F.A.; Hall, C.I.; Weilhammer, D.R. Evaluation of inactivation methods for Rift Valley fever virus in mouse microglia. Pathogens 2024, 13, 159. [Google Scholar] [CrossRef]
  96. Confort, M.-P.; Ratinier, M.; Arnaud, F. Validated methods for effective decontamination and inactivation of Rift Valley fever virus. In Rift Valley Fever Virus. Methods in Molecular Biology; Lozach, P.Y., Ed.; Humana: New York, NY, USA, 2024; Volume 2824. [Google Scholar] [CrossRef]
  97. Zargar, B.; Sattar, S.A.; McKinney, J.; Ijaz, M.K. The stability and elimination of mammalian enveloped and non-enveloped respiratory viruses in indoor air: Testing using a room-sized aerobiology chamber. J. Virol. Meth. 2025, 8, 115144. [Google Scholar] [CrossRef]
  98. Ijaz, M.K.; Sattar, S.A.; Rubino, J.R.; Nims, R.W.; Gerba, C.P. Combating SARS-CoV-2: Leveraging microbicidal experiences with other emerging/re-emerging viruses. PeerJ 2020, 8, e9914. [Google Scholar] [CrossRef]
  99. Ijaz, M.K.; Nims, R.W.; McKinney, J. Emerging SARS-CoV-2 mutational variants of concern should not vary in susceptibility to microbicidal actives. Life 2022, 12, 987. [Google Scholar] [CrossRef] [PubMed]
  100. Weber, D.J.; Rutala, W.A.; Fischer, W.A.; Kanamori, H.; Sickbert-Bennett, E.E. Emerging infectious diseases: Focus on infection control issues for novel coronaviruses (Severe Acute Respiratory Syndrome-CoV and Middle East Respiratory Syndrome-CoV), hemorrhagic fever viruses (Lassa and Ebola), and highly pathogenic avian influenza viruses, A(H5N1) and A(H7N9). Am. J. Infect. Control 2016, 44 (Suppl. S5), E91–E100. [Google Scholar] [CrossRef] [PubMed]
  101. U.S. Environmental Protection Agency. Disinfectants for Emerging Viral Pathogens (EVPs): List Q. 2024. Available online: https://www.epa.gov/pesticide-registration/disinfectants-emerging-viral-pathogens-evps-list-q (accessed on 10 April 2025).
  102. Hewson, R. Understanding viral haemorrhagic fevers: Virus diversity, vector ecology, and public health strategies. Pathogens 2024, 13, 909. [Google Scholar] [CrossRef]
  103. Madueme, P.-G.U.; Chirove, F. Understanding the transmission pathways of Lassa fever: A mathematical modeling approach. Infect. Dis. Model. 2023, 8, 27–57. [Google Scholar] [CrossRef]
  104. Stephenson, E.H.; Larson, E.W.; Dominik, J.W. Effect of environmental factors on aerosol-induced Lassa virus infection. J. Med. Virol. 1984, 14, 295–303. [Google Scholar] [CrossRef] [PubMed]
  105. Sagripanti, J.-L.; Rom, A.M.; Holland, L.E. Persistence in darkness of virulent alphaviruses, Ebola virus, and Lassa virus deposited on solid surfaces. Arch. Virol. 2010, 155, 2035–2039. [Google Scholar] [CrossRef] [PubMed]
  106. Mekibib, B.; Ariën, K.K. Aerosol transmission of filoviruses. Viruses 2016, 8, 148. [Google Scholar] [CrossRef]
  107. Lantagne, D.S.; Hunter, P.R. Comment on “Ebola virus persistence in the environment: State of the knowledge and research needs”. Env. Sci. Technol. 2015, 2, 48–49. [Google Scholar] [CrossRef]
  108. Osterholm, M.T.; Moore, K.A.; Kelley, N.S.; Brosseau, L.M.; Wong, G.; Murphy, F.A.; Peters, C.J.; LeDuc, J.W.; Russell, P.K.; Van Herp, M.; et al. Transmission of Ebola viruses: What we know and what we do not know. mBio 2015, 6, e00137-15. [Google Scholar] [CrossRef]
  109. Piercy, T.J.; Smither, S.J.; Steward, J.A.; Eastaugh, L.; Lever, M.S. The survival of filoviruses in liquids, on solid substrates and in a dynamic aerosol. J. Appl. Microbiol. 2010, 109, 1531–1539. [Google Scholar] [CrossRef] [PubMed]
  110. McMillen, C.M.; Hartman, A.L. Rift Valley fever in animals and humans: Current perspectives. Antivir. Res. 2018, 156, 29–37. [Google Scholar] [CrossRef]
  111. Talukdar, P.; Dutta, D.; Ghosh, E.; Bose, I.; Bhattacharjee, S. Molecular pathogenesis of Nipah virus. Appl. Biochem. Biotechnol. 2023, 195, 2451–2462. [Google Scholar] [CrossRef]
  112. Soni, M.; Kumar, V.; Singh, M.P.; Shabil, M.; Sah, S. Nipah virus resurgence: A call for preparedness across states. Infect. Med. 2024, 3, 100145. [Google Scholar] [CrossRef]
  113. Wong, K.T.; Shieh, W.-J.; Kumar, S.; Norain, K.; Abdullah, W.; Guarner, J.; Goldsmith, C.S.; Chua, K.B.; Lam, S.K.; Tan, C.T.; et al. Nipah virus infection. Pathology and pathogenesis of an emerging paramyxoviral zoonosis. Am. J. Pathol. 2022, 161, 2153–2167. [Google Scholar] [CrossRef]
  114. Rybicki, E.P. Panics and pandemics. In Cann’s Principles of Molecular Virology; Academic Press: Cambridge, MA, USA, 2023; pp. 307–355. [Google Scholar] [CrossRef]
  115. Lytle, C.D.; Sagripanti, J.-L. Predicted inactivation of viruses of relevance to biodefense by solar radiation. J. Virol. 2005, 79, 14244–14252. [Google Scholar] [CrossRef] [PubMed]
  116. Schneider, K.; Wronka-Edwards, L.; Leggett-Embrey, M.; Walker, E.; Sun, P.; Ondov, B.; Wyman, T.H.; Rosovitz, M.J.; Bohn, S.S.; Burans, J.; et al. Psoralen inactivation of viruses: A process for the safe manipulation of viral antigen and nucleic acid. Viruses 2015, 7, 5875–5888. [Google Scholar] [CrossRef] [PubMed]
  117. Lanteri, M.C.; Santa-Maria, F.; Laughhunn, A.; Girard, Y.A.; Picard-Maureau, M.; Payrat, J.-M.; Irsch, J.; Stassinopoulos, A.; Bringmann, P. Inactivation of a broad spectrum of viruses and parasites by photochemical treatment of plasma and platelets using amotosalen and ultraviolet A light. Transfusion 2020, 60, 1319–1331. [Google Scholar] [CrossRef] [PubMed]
  118. Gaspar, L.P.; Mendes, Y.S.; Yamamura, A.M.Y.; Almeida, L.F.C.; Caride, E.; Gonçalves, R.B.; Silva, J.L.; Oliveira, A.C.; Galler, R.; Freire, M.S. Pressure-inactivated yellow fever 17DD virus: Implications for vaccine development. J. Virol. Meth. 2008, 150, 57–62. [Google Scholar] [CrossRef]
Table 1. Efficacy of virucidal approaches for inactivating HFVs of the Arenaviridae family.
Table 1. Efficacy of virucidal approaches for inactivating HFVs of the Arenaviridae family.
Virus/Strain Active IngredientInactivating Agent TypeContact
Time (min) a		Concentration in Test Efficacy
(log10 Reduction) b		Ref.
Surface hygiene (glass carriers)
LassaN/A cUV-C (254 nm)N/AN/A0.27 log10/mJ/cm2[25]
Suspension inactivation
JuninCopper II ions, H2O2MicrobicideVarious1 mg/L, 100 mg/LD = 33 min[26]
Lassa/JosiahSodium hypochloriteMicrobicideVarious 5000, 10,000 ppm≥8 log10 in 5 min [27]
Lassa/SauerwaldSodium hypochloriteMicrobicideVarious 5000, 10,000 ppm≥8 log10 in 5 min [27]
Lassa/JosiahSodium hypochloriteMicrobicideVarious 5000 ppm≥6.7 log10 in 1 min [27]
EthanolMicrobicideVarious 67%≥6.7 log10 in 0.5 min[28]
Dual QAC dMicrobicideVarious 2%≥6.2 log10 in 0.5 min[28]
Accelerated H2O2MicrobicideVarious 2.5%≥7.3 log10 in 1 min[28]
LassaN/AGamma irradiationN/A @ −60 °CN/A0.53 log10/kGy[29]
Hand/skin hygiene
Lassa/JosiahChloroxylenol (PCMX)Antiseptic
liquid		Various 0.12%≥7.8 log10 in 1 min[28]
Sample disinfection procedures
Lassa/JosiahAcetic acidSample inactivant153% (pH 2.5)≥3[30]
LassaPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.0[31]
LujoPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.1[31]
GuanaritoPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥6.3[31]
MachupoPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.3[31]
SabiáPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥6.1[31]
Lassa/JosiahGuanidine thiocyanate, ethanolLysis buffer10, 350–70%, 95%8.0[32]
Lassa/GA391β-propiolactoneSample inactivant30 @ 37 °C0.2%≥7[33]
Lassa/JosiahFormalinCell fixative20 daysNeatComplete [34]
N/AGamma irradiationN/A @ −60 °CN/A~0.15 log10/kGy[35]
N/AHeatN/A @ 60 °CN/AD = 7.4 min[30]
Lassa/GA391N/AHeatN/A @ 60 °CN/AD = 6.0 min[33]
Lassa/JosiahPhenol/guanidine thiocyanateNucleic acid extractant10NeatComplete [36]
FormalinSample inactivant360 @ 4 °C10%Complete [36]
Phenol/guanidine thiocyanateNucleic acid extractant1075%8[36]
a Contact times at room temperature are provided unless otherwise indicated. b Inactivation matrix was virus stock (virus in cell culture medium) unless otherwise indicated in the cited papers. c Abbreviations used: D, decimal reduction time (the time required to inactivate 1 log10 of virus); HFVs, hemorrhagic fever viruses; H2O2, hydrogen peroxide; kGy, kiloGrays; min, minutes; mJ/cm2, milliJoules per square centimeter; N/A, not applicable; PCMX, para-chloro-meta-xylenol; ppm, parts per million; QAC, quaternary ammonium compound; UV-C, ultraviolet light in the C range. d Ingredients shown in blue font are incorporated into a formulated product. The cited papers may be consulted to obtain the product trade names.
Table 2. Efficacy of virucidal approaches for inactivating HFVs of the Filoviridae family.
Table 2. Efficacy of virucidal approaches for inactivating HFVs of the Filoviridae family.
Virus/Strain Active Ingredient Inactivating Agent TypeContact Time (min) a Concentration in Test Efficacy (log10 Reduction) bRef.
Surface hygiene (steel or aluminum carriers)
EBOV/MakSodium hypochloriteMicrobicide50.5%≥6.6[38]
Sodium hypochloriteMicrobicide50.5%≥6.8[39]
Sodium hypochloriteMicrobicide150.5%≥2.0[40]
Sodium hypochloriteMicrobicide150.5%<1 [40]
Sodium hypochloriteMicrobicide50.5%≥5.1[41]
Sodium hypochlorite dPre-impregnated wipe0.081%6.3[42]
EthanolAlcohol567%≥7.3[38]
EthanolAlcohol2.570%≥6.8[39]
EthanolAlcohol570%≥6.9[41]
EthanolDisinfectant spray558%≥4.5[41]
EthanolPre-impregnated wipe0.0866.5%6.6[42]
EthanolAlcohol270%1.7[40]
EthanolAlcohol270%<1 [40]
Peracetic acidMicrobicide 5%≥1.0[40]
Peracetic acidMicrobicide 5%≥2.0 [40]
Chloroxylenol (PCMX) cMicrobicide50.48%≥5.1[41]
H2O2Pre-impregnated wipe12.5%6.4[42]
H2O2, peroxyacetic acidMicrobicide5Net2.6[40]
H2O2, peroxyacetic acidMicrobicide5Neat<1 [40]
QACMicrobicide101.5%<1[40]
QACPre-impregnated wipe1As supplied6.6[42]
QACPre-impregnated wipe0.085%6.0[42]
EBOV/MaySodium hypochloriteMicrobicide50.5%≥6.6[39]
EthanolAlcohol170%≥6.6[39]
EBOV/KikSodium hypochloriteMicrobicide50.5%≥6.5[39]
EthanolAlcohol170%≥6.5[39]
EBOV/Yam-EcrSodium hypochloriteMicrobicide100.75%≥6.5[43]
Alcohol formulationMicrobicide1050%5.3[43]
QAC, alcoholMicrobicide101.5%2.5[43]
QAC, alkylamineMicrobicide102.5%4.2[43]
Suspension inactivation
EBOV/MakSodium hypochloriteMicrobicide0.335 ppm≥4.2[44]
EBOVPovidone-iodineMicrobicide0.251:10≥5.5[45]
N/AGamma irradiationN/A @ −60 °CN/A0.84 log10/kGy[29]
N/AGamma irradiationN/AN/A0.44 log10/kGy[46]
Sudan N/AGamma irradiationN/AN/A0.44 log10/kGy[46]
Marburg N/AGamma irradiationN/A @ −60 °CN/A0.68 log10/kGy[29]
Hand/skin hygiene
EBOV/MakChloroxylenol (PCMX)Antiseptic liquid10.48%≥4.8[47]
Salicylic acid, citric acidLiquid hand wash0.51:44.8[48]
EBOVPovidone-iodineSkin cleanser0.51:10≥4.5[45]
Povidone-iodineSurgical scrub0.251:10≥5.5[45]
Povidone-iodine, alcoholSkin cleanser0.25Neat≥5.7[45]
EBOV/MayEthanol, H2O2WHO formulation I hand rub (original)0.532%, 0.05%≥5[49]
2-Propanol, H2O2WHO formulation II hand rub (original)0.524%, 0.04%≥5[49]
Sample disinfection procedures
EBOVnonionic surfactantsDetergent600.1%4[50]
EBOV/Maknonionic surfactantsDetergent600.1%≥3 [51]
Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.7[31]
Sodium dodecyl sulfateDetergent600.1%≥3 [51]
Sodium dodecyl sulfateDetergent600.1%~1 [51]
Guanidine thiocyanate, ethanolLysis buffer10, 350–70%, 95%7.4 to 7.6[32]
Reston Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.1[31]
Sudan Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.1[31]
EBOV/MayAcetic acidSample inactivant153% (pH 2.5)≥3 [30]
N/AHeatN/A @ 60 °CN/AD = 4.4 min[30]
N/AHeat10 @ >99 °CN/AComplete [36]
N/AHeat10 @ >99 °CN/A>8[36]
Phenol/guanidine thiocyanateNucleic acid extractant10N/AComplete [36]
Phenol/guanidine thiocyanateNucleic acid extractant10N/A8[36]
N/AGamma irradiationN/A @ −60 °CN/A~0.3 log10/kGy[35]
N/AGamma irradiationN/A @ −60 °CN/A0.31 log10/kGy[52]
EBOVFormalinSample inactivant360 @ 4 °C10%8.4[36]
nonionic surfactantsSample inactivant200.8%Incomplete[53]
nonionic surfactants +
phenol/guanidine thiocyanate		Nucleic acid extractant100.08%Complete (6.0)[53]
EBOVPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.3[54]
Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.3[55]
Neutral buffered formalinTissue fixative≤1 week10%9.08[55]
Osmium tetroxideTissue fixative601%4.9[55]
EBOV/KikPhenol/guanidine thiocyanateNucleic acid extractant1080% of neatIncomplete (<6)[56]
Phenol/guanidine thiocyanate + ethanolNucleic acid extractant1080% of neat6[56]
Marburg/Ci67Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥6.5[31]
Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥6.8[54]
N/AGamma irradiationN/A @ −60 °CN/A~0.3 log10/kGy[35]
Marburg/371BatGuanidine thiocyanate, ethanolLysis buffer10, 350–70%, 95%6.5[32]
Marburg/MusokeeAcetic acidSample inactivant153% (pH 2.5)≥3[30]
Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥6.7[54]
N/AHeatN/A @ 60 °CN/AD = 7.4 min[30]
a Contact times at room temperature are provided unless otherwise indicated. b Inactivation matrix was virus stock (virus in cell culture medium) unless otherwise indicated in the cited papers. c Abbreviations used: D, decimal reduction time (the time required to inactivate 1 log10 of virus); HFVs, hemorrhagic fever viruses; H2O2, hydrogen peroxide; kGy, kiloGrays; min, minutes; N/A, not applicable; PCMX, para-chloro-meta-xylenol; ppm, parts per million; QAC, quaternary ammonium compound. d Ingredients shown in blue font are incorporated into a formulated product. The cited papers may be consulted to obtain the product trade names.
Table 3. Efficacy of virucidal approaches for inactivating HFVs of the Flaviviridae family.
Table 3. Efficacy of virucidal approaches for inactivating HFVs of the Flaviviridae family.
Virus/Strain Active Ingredient Inactivating Agent TypeContact Time (min) a Concentration
in Test 		Efficacy (log10 Reduction) bRef.
Surface hygiene (stainless steel carriers)
Yellow fever/17D1-Propanol, 2-propanol, ethanol dMicrobicide0.5 80%≥3.4[58]
Ethanol, 2-propanolMicrobicide0.580%≥3.4[58]
Glutaraldehyde, QAC cMicrobicide50.5%≥2.4[58]
Glutaraldehyde, QACMicrobicide50.5%≥2.4[58]
H2O2Microbicide0.580%1.7[58]
Suspension inactivation
Yellow fever/17DEthanol Microbicide0.540%≥5.5[58]
2-PropanolMicrobicide0.520%≥5.5[58]
H2O2 Microbicide1203%≥6[59]
Yellow feverN/AHeatN/A @ 60 °CN/AD = 13.2 min[60]
Alkhumra fever/AHFV/997/NJ/09/SAN/AHeatN/A @ 60 °CN/AD = 0.32 min[61]
N/AHeatN/A @ 45 °CN/AD = 11.1 min[61]
Hand/skin hygiene
Yellow fever/17DEthanol, H2O2WHO formulation I hand rub (original)0.540%≥5.5[58]
2-Propanol, H2O2WHO formulation II hand rub (original)0.530%≥5.5[58]
Sample disinfection procedures
Dengue serotype 1/HawaiiPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥4.1[54]
Dengue serotype 2/S16803Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.0[54]
Dengue serotype 3/CH53489Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥3.3[54]
Dengue serotype 4/H241Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥1.9[54]
Dengue serotype 2/92TPhenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥5.1[31]
AcetoneCell fixative1440 @ 4°C50%Incomplete[62]
ParaformaldehydeCell fixative1804%Complete[62]
Dengue/serotypes 1–4N/AHeat30 @ 56 °CN/A≥3.4 log10[63]
a Contact times at room temperature are provided unless otherwise indicated. b Inactivation matrix was virus stock (virus in cell culture medium) unless otherwise indicated in the cited papers. c Abbreviations used: D, decimal reduction time (the time required to inactivate 1 log10 of virus); HFVs, hemorrhagic fever viruses; H2O2, hydrogen peroxide; min, minutes; N/A, not applicable. d Ingredients shown in blue font are incorporated into a formulated product. The cited papers may be consulted to obtain the product trade names.
Table 4. Efficacy of virucidal approaches for inactivating HFVs of the Hantaviridae family.
Table 4. Efficacy of virucidal approaches for inactivating HFVs of the Hantaviridae family.
Virus/Strain Active Ingredient Inactivating Agent TypeContact Time (min) a Concentration
in Test 		Efficacy (log10 Reduction) bRef.
Surface hygiene (glass carriers)
Puumala N/A cHeat60 @ 56 °CN/AIncomplete (<5.8)[66]
Tula N/AHeat60 @ 56 °CN/AComplete (5.9)[66]
Suspension inactivation
Hantaan/76–118EthanolMicrobicide230% to 70%Complete (6.5)[67]
Puumala N/AHeat15 @ 56 °CN/AComplete (5.8)[66]
Puumala/CG1829EthanolMicrobicide3070%≥3.7[68]
Peracetic acidMicrobicide101%≥3.7[68]
Sodium hypochloriteMicrobicide101% (1000 ppm)≥3.7[68]
Chlorine dioxide dMicrobicide101%≥3.7[68]
Chloroxylenol (PCMX)Microbicide101%≥3.7[68]
Sodium p-toluenesulfonchloramide, trihydrateMicrobicide101%≥3.7[68]
Potassium peroxymonosulfateMicrobicide101%≥3.7[68]
TulaN/AHeat15 @ 56 °CN/AComplete (5.9)[66]
Hand/skin hygiene
No primary literature was identified
Sample disinfection procedures
Hantaan/76–118MethanolSample fixative8Absolute≥5.5[69]
ParaformaldehydeSample fixative201%≥4.3[69]
Acetone/methanolSample fixative1050%/50%≥5.6[69]
Lysis buffer + detergentSample extractant101% detergent≥2[69]
N/AUV-C (254 nm)N/A500 mJ/cm2Incomplete (3.9)[69]
N/AUV-C (254 nm)N/A1400 mJ/cm2Complete (≥5.2)[69]
Puumala/CG1829ß-propiolactoneVaccine inactivant300.025%≥5.4[70]
FormaldehydeVaccine inactivant140.025%≥5.4[70]
a Contact times at room temperature are provided unless otherwise indicated. b Inactivation matrix was virus stock (virus in cell culture medium) unless otherwise indicated in the cited papers. c Abbreviations used: HFVs, hemorrhagic fever viruses; mJ/cm2, milliJoules per square centimeter; min, minutes; N/A, not applicable; PCMX, para-chloro-meta-xylenol; ppm, parts per million; UV-C, ultraviolet light in the C range. d Ingredients shown in blue font are incorporated into a formulated product. The cited papers may be consulted to obtain the product trade names.
Table 5. Efficacy of virucidal approaches for inactivating HFVs of the Nairoviridae family.
Table 5. Efficacy of virucidal approaches for inactivating HFVs of the Nairoviridae family.
Virus/Strain Active IngredientProduct TypeContact Time (min) aConcentration in Test Efficacy (log10) bRef.
Surface hygiene
No primary literature was identified
Hand/skin hygiene
No primary literature was identified
Suspension inactivation
CCHFV/IbAr 10200EthanolMicrobicide220% to 70%Complete (4.6)[67]
Sample disinfection procedures
CCHFV/IbAr 10200N/A cHeat60 @ 60 °CN/A3.5 [75]
Hazara/JC280 dN/AX-irradiationN/AN/A1.04 log10/kGy[76]
a Contact times at room temperature are provided unless otherwise indicated. b Inactivation matrix was virus stock (virus in cell culture medium) unless otherwise indicated in the cited papers. c Abbreviations used: CCHFV, Crimean–Congo hemorrhagic fever virus; HFVs, hemorrhagic fever viruses; kGy, kiloGrays; min, minutes; N/A, not applicable. d Hazara virus is a nairovirus that has not been found to be pathogenic for humans and has been used as a CCHFV surrogate in inactivation efficacy testing [74].
Table 6. Efficacy of virucidal approaches for inactivating non-typical HFVs of the Paramyxoviridae family.
Table 6. Efficacy of virucidal approaches for inactivating non-typical HFVs of the Paramyxoviridae family.
Virus/Strain Active IngredientProduct TypeContact Time (min) aConcentration in Test Efficacy (log10) bRef.
Surface hygiene
No primary literature was identified
Suspension inactivation
Nipah/BangladeshDual QAC c,dMicrobicide0.5 0.28%>4[81]
Dual QACMicrobicide10.095%>4[81]
EthanolMicrobicide0.2519%>4[81]
Nipah/MalaysiaSodium hypochloriteMicrobicide110%≥5.5[82]
EthanolMicrobicide180%≥5.5[82]
NipahLow pHHCl60pH 2≥3[83]
High pHNaOH60pH 12≥3[83]
HendraLow pHHCl60pH 3≥3[83]
High pHNaOH60pH 12≥3[83]
Hand/skin hygiene agents
No primary literature was identified
Sample disinfection procedures
Nipah/MalaysiaFormalinFixative144010%≥5[82]
ParaformaldehydeSample inactivant304%Complete [84]
N/AGamma irradiationN/A @ −60 °CN/A~0.15 log10/kGy[35]
Nipah/Ma-JMR-01-98N/AHeat60 @ 56 °CN/A≥4.9 [85]
N/AHeat30 @ 60 °CN/A≥4.9 [85]
N/AUV-C (312 nm)30N/A0.0075 log10/mJ/cm2 [85]
N/AUV-C (312 nm)30N/A0.0033 log10/mJ/cm2 [85]
NipahParaformaldehydeSample inactivant154%Complete [86]
FormalinTissue fixative288010%Complete [86]
Nipah/BangladeshPhenol/guanidine thiocyanateNucleic acid extractant10NeatComplete [36]
FormalinSample inactivant360 @ 4 °C10%Complete [36]
Phenol/guanidine thiocyanateNucleic acid extractant1075%7.1[36]
N/AHeat30 @ 60 °CN/AComplete [87]
HendraN/AGamma irradiationN/A @ −60 °CN/A~0.15 log10/kGy[35]
a Contact times at room temperature are provided unless otherwise indicated. b Inactivation matrix was virus stock (virus in cell culture medium) unless otherwise indicated in the cited papers. c Abbreviations used: HFVs, hemorrhagic fever viruses; kGy, kiloGrays; min, minutes; mJ/cm2, milliJoules per square centimeter; N/A, not applicable; QAC, quaternary ammonium compound; UV-C, ultraviolet light in the C range. d Ingredients shown in blue font are incorporated into a formulated product. The cited papers may be consulted to obtain the product trade names.
Table 7. Efficacy of virucidal approaches for inactivating HFVs of the Phenuiviridae family.
Table 7. Efficacy of virucidal approaches for inactivating HFVs of the Phenuiviridae family.
Virus/Strain Active IngredientProduct TypeContact Time (min) aConcentration in Test Efficacy (log10) bRef.
Surface hygiene
No primary literature was identified
Hand/skin hygiene
No primary literature was identified
Suspension inactivation
RVFVN/A cHeatN/A @ 70 °CN/AD = 2.2 min[92]
N/AHeatN/A @ 80 °CN/AD = 1.2 min[92]
RVFV/Menya/Sheep/258N/AHeatN/A @ 95 °CN/AD = 0.34 min[92]
β-propiolactoneVaccine inactivant2403.5 mM≥5.5[93]
Formalin dVaccine inactivant3600.2%≥5.4[93]
Sample disinfection procedures e
RVFV/AH-501Phenol/guanidine thiocyanateNucleic acid extractant1080% of neat≥6.8[31]
RVFVFormaldehydeCell fixative10800.4%≥7.1 [94]
RVFV/MP12FormalinCell fixative210 @ 4 °CNeatComplete [34]
RVFV/ArB 1976N/AHeat60 @ 60 °CN/A6.7 [75]
RVFVN/AHeat5 @ 95 °CN/AComplete [92]
RVFV/MP12Guanidine isothiocyanateNucleic acid extractantNot givenNeatComplete [95]
RVFV/ZH501Guanidine isothiocyanateNucleic acid extractantNot givenNeatComplete [95]
RVFV/MP12FormaldehydeCell fixative20 @ 4 °C4.2%Complete [95]
RVFV/ZH501FormaldehydeCell Fixative20 @ 4 °C4.2%Complete [95]
N/AGamma irradiationN/A @ −60 °CN/A~0.15 log10/kGy[35]
N/AX-irradiationN/AN/A0.38 log10/kGy[76]
N/AX-irradiationN/A @ −30 °CN/A0.26 log10/kGy[76]
SFTSV/YGIN/AHeatN/A0 @ 60 °CN/A≥4.8 [89]
N/AUV-C (312 nm)30 @ 60 °C52 mJ/cm2≥4.8 [89]
N/AUV-C (312 nm)30 @ 60 °C1548 mJ/cm2≥4.5 [89]
a Contact times at room temperature are provided unless otherwise indicated. b Inactivation matrix was virus stock (virus in cell culture medium) unless otherwise indicated in the cited papers. c Abbreviations used: D, decimal reduction time (the time required to inactivate 1 log10 of virus); HFVs, hemorrhagic fever viruses; kGy, kiloGrays; mJ/cm2, milliJoules per square centimeter; min, minutes; N/A, not applicable; RVFV, Rift Valley fever virus; SFTSV, severe fever with thrombocytopenia syndrome virus; UV-C, ultraviolet light in the C range. d Ingredients shown in blue font are incorporated into a formulated product. The cited papers may be consulted to obtain the product trade names. e A set of validated procedures for inactivation of Rift Valley fever virus has also been proposed by Confort et al. [96].
Disclaimer/Publisher’s Note: The statements, opinions and data contained in all publications are solely those of the individual author(s) and contributor(s) and not of MDPI and/or the editor(s). MDPI and/or the editor(s) disclaim responsibility for any injury to people or property resulting from any ideas, methods, instructions or products referred to in the content.

Share and Cite

MDPI and ACS Style

Nims, R.W.; Ijaz, M.K. Virucidal Approaches for Hemorrhagic Fever Viruses. Viruses 2025, 17, 663. https://doi.org/10.3390/v17050663

AMA Style

Nims RW, Ijaz MK. Virucidal Approaches for Hemorrhagic Fever Viruses. Viruses. 2025; 17(5):663. https://doi.org/10.3390/v17050663

Chicago/Turabian Style

Nims, Raymond W., and M. Khalid Ijaz. 2025. "Virucidal Approaches for Hemorrhagic Fever Viruses" Viruses 17, no. 5: 663. https://doi.org/10.3390/v17050663

APA Style

Nims, R. W., & Ijaz, M. K. (2025). Virucidal Approaches for Hemorrhagic Fever Viruses. Viruses, 17(5), 663. https://doi.org/10.3390/v17050663

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