Introduction

The novel coronavirus, severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), causing coronavirus disease 2019 (COVID-19) was identified in the Hubei province of China in December 2019 before spreading worldwide and causing serious health and economic burdens1. More than 79 million people have been infected, with a 2.2% death rate, as of 27 December 2020 (https://is.gd/WQEhWz). SARS-CoV-2 is an enveloped, single-positive sense RNA virus belonging to the Coronaviridae family2. The genome of SARS-CoV-2 is approximately 30 kb, encoding the genes for four structural proteins, two large replicase polyproteins which will be proteolytic cleaved into 16 putative non-structural proteins for viral replication/ transcription, and other small proteins with unknown function3,4,5. The spike (S) structural protein of SARS-CoV-2 is stalked on the virus membrane and is responsible for viral entry by interacting with the host receptor, angiotensin converting enzyme II6. The envelope (E) protein of coronaviruses participates in virus assembly, budding, morphogenesis, and trafficking7. The membrane (M) protein of coronaviruses is the most abundant glycoprotein in the virion and acts as a central organizer of virus assembly8. The nucleocapsid (N) protein of coronaviruses packages and protects the viral genome by binding to it and forming the ribonucleocapsid9.

The rapid outbreak of SARS-CoV-2 is due to its high transmission ability. The basic reproductive rate (R0) for SARS-CoV-2 is estimated to be 2.5 (range 1.8–3.6), compared to 2.0 for SARS-CoV, 1.5 for the 2009 influenza pandemic, and 3.0 for the 1918 influenza pandemic10. There are several routes of SARS-CoV-2 transmission that have been proposed, including air-borne transmission, surface contamination, and fecal–oral transmission11. Consistently, viral RNA is detectable in a patient’s quarantine environment, including personal items, room surfaces, and toilets. Furthermore, infectious virus is detected from hallway air samples and windowsills, suggesting the risk of virus transmission from a contaminated environment12,13. The half-life of SARS-CoV-2 on different materials has been reported; in aerosol, it is approximately 1.1 h, for stainless steel, it is 5.6 h, and for plastic, it may be as long as 6.8 h14. These results strongly emphasize the importance of surface and environmental disinfection to reduce the risk of SARS-CoV-2 transmission.

Ultraviolet (UV) light is a potent disinfectant; based on wavelength, UV is classified as UVA (320–400 nm), UVB (280–320 nm), and UVC (200–280 nm)15. UV wavelength is negatively related to anti-microbial ability; therefore, UVC is the most powerful UV light among the three that has been used in clinical disinfection with efficient disinfection ability16. Several mechanisms of virus inactivation by UVC have been reported. For example, UVC causes viral protein oxidation, which is linked to the reduction of virus infectivity in feline calicivirus and bacterial phage MS217,18,19. Second, UVC irradiation destroys murine norovirus 1 (MNV-1) viral capsid protein20. Third, UVC-induced virus protein-genome crosslinking is observed in poliovirus21. Fourth, UVC irradiation damages the genome of influenza virus22. However, UVC-induced damage varies in different virus types, as UVC damages the viral genome, but not viral proteins in adenovirus23. Consequently, the disinfection mechanism of UVC in different viruses requires testing.

Several findings12,13,14 highlight the importance of environmental contamination (air, liquid, and solid surfaces) and dissemination of SARS-CoV-2. UVC, which is the most powerful UV light, may be the most useful method to rapidly reduce SARS-CoV-2 viability in the environment. In fact, UVC has inactivated SARS-CoV-2 in different surfaces materials24,25,26. However, the mechanism of how UVC disinfects SARS-CoV-2 is unclear. Here, UVC mechanisms of SARS-CoV-2 inactivation were investigated by viral morphology analysis using transmission electronic microscopy (TEM), protein damage testing using immunoblotting, and viral genome integrity inspection using reverse-transcription quantitative-polymerase chain reaction (RT-qPCR) and long-RT PCR.

Results

Schematic of the UVC exposure system to inactivate SARS-CoV-2

Among various UVC light sources, a low pressure mercury lamp was used for inactivation of SAES-CoV-2, because it is more practical that has high average power with low cost. It generates the UV light at 253.7 nm. In previous works of UVC inactivation of corona viruses, dose of light were typically 2 mW/cm224,27. Therefore, we start the intensity of light and exposure time as 500 μW/cm2 and 5 s. For UVC irradiation, a UVC light tube was set at a 30 cm height inside a safety cabinet. The virus was placed in a 10 cm2 dish beneath the UVC light tube (Fig. 1).

Figure 1
figure 1

The ultraviolet C (UVC) light irradiation system. A UVC wavelength of 253.7 nm, 500 μW/cm2 is used. The length and diameter of the light tube are 295 ± 3 mm and 15.5 ± 0.5 mm, respectively. SARS-CoV-2 (5 mL) with a titer of 5 × 104 50% tissue culture infective dose (TCID50/mL) or (1 mL) with a titer of 1.78 × 106 TCID50/mL are placed in a 10 cm2 dish, 30 cm below the UVC light tube, and are continuously and individually irradiated using a UVC lamp for 0, 5, 15 or 30 s.

UVC inactivated SARS-CoV-2 in a time-dependent manner

To measure the SARS-CoV-2 inactivation efficiency of UVC, virus-containing medium was exposed to UVC for increasing periods of time from 5 to 30 s (Fig. 1). Virus titers after UVC irradiation were then quantified using a TCID50 assay with VeroE6/TMPRSS2 cells. As shown in Fig. 2A, UVC irradiation for 5, 15 and 30 s significantly (p < 0.05 and p < 0.01) decreases virus infectivity by a reduction of 1.0, 2.8, and 4.9 log10, respectively, and replication of SARS-CoV-2 completely ceases after 30 s. In addition, linear regression analysis indicated that UVC inactivated SARS-CoV-2 in a time-dependent manner and it was estimated that 29 s of UVC irradiation fully inhibited SARS-CoV-2 infectivity (R2 = 0.98) (Fig. 2B).

Figure 2
figure 2

Effect of ultraviolet C (UVC) irradiation on severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) infectivity. (A) Change in 50% tissue culture infective dose (TCID50) of SARS-CoV-2 after UVC irradiation. SARS-CoV-2 (5 mL) with a titer of 5 × 104 TCID50/mL was irradiated with a UVC light tube for 0, 5, 15 or 30 s and then was titrated using the TCID50 assay with Vero E6/TMPRSS2 cells. Assays are in triplicate and values represent the mean ± standard deviation (SD) of three replicates. Significance has been determined using one-way analysis of variance followed by Dunnett’s multiple comparisons test. The asterisk indicates a statistical difference (*p < 0.05; **p < 0.01). (B) Linear regression analysis to examine the correlation between UVC exposure time and SARS-CoV-2 infectivity.

UVC exposure had no effect on SARS-CoV-2 virion morphology

As UVC had potential to induce viral protein damage, whether UVC destroyed virion structure was tested using TEM analysis (Fig. 3A). The SARS-CoV-2 particle is a round shape, approximately 100 nm in diameter and stalked with the spike protein on the surface. After 1 min of UVC irradiation, the UVC-treated virus particle also showed a similar structure, while the virus totally lost infectivity. These results suggested that UVC inactivated virus infectivity, but had no apparent effect on viral particle morphology.

Figure 3
figure 3

Effect of ultraviolet C (UVC) irradiation on viral morphology and viral proteins. (A) Representative viral particle images analyzed by transmission electron microscopy (TEM, three pictures for each group). SARS-CoV-2 (1 mL) with a titer of 1.78 × 106 50% tissue culture infective dose (TCID50/mL) was irradiated with a UVC light tube for 60 s and then analyzed by TEM (Scale bar of 100 nm). (B) Representative immunoblot images of viral spike (S) and nucleocapsid (N) proteins. SARS-CoV-2 (1 mL) with a titer of 1.78 × 106 TCID50/mL was irradiated with a UVC light tube for increasing periods of time from 0 to 30 s. Equal volumes of irradiated virus suspension were then used for immunoblotting analysis using anti-SARS-CoV-2 spike monoclonal antibody (1A9) and anti-SARS-CoV-2 nucleocapsid monoclonal antibody (6H3) (upper panel). Positions of the S and N proteins are indicated. Full-length blots are shown in Supplementary Fig. S1. The intensity of both proteins is analyzed using CS Analyzer 4 software and quantitative results are shown in the bar diagram (lower panel). Data in the plot represent the mean ± standard deviation (SD) of three replicates. Significance has been determined using one-way analysis of variance followed by Dunnett’s multiple comparisons test.

UVC did not degrade SARS-CoV-2 spike (S) and nucleocapsid (N) proteins

To further investigate the effect of UVC on viral proteins, immunoblotting was performed to analyze the integrity of S and N proteins after UVC irradiation (Fig. 3B). The 180 kDa and 55 kDa bands were identified as S and N proteins, respectively (Fig. 3B upper panel). The blot intensities of the control and UVC-treated group showed no significant differences for both proteins (Fig. 3B lower panel). These results suggested that protein degradation might not be the major reason for UVC-induced virus inactivation. Note that the measurement was based on two monoclonal antibodies, whether there were protein damages that occurred outside the epitope regions need further investigation.

UVC damaged the SARS-CoV-2 genome

To clarify the mechanism of SARS-CoV-2 inactivation by UVC, RT-qPCR was performed to detect the damage of the viral genome. First, conventional RT-qPCR was performed, which detected genome damage of 128 bp within the N gene (Fig. 4A). After UVC irradiation, amounts of viral RNA showed no difference compared to the control group (Fig. 4B). These results are inconsistent with previous reports28. However, this observation might be due to the detection limitation of conventional RT-qPCR, which only detects a small region of the viral genome. Therefore, next, viral genome damage was tested using a long RT-qPCR that covered 1095 bp of the N gene region (Fig. 4C). Amounts of viral RNA decreased with UVC irradiation in a time-dependent manner, and 30 s UVC irradiation significantly decreased SARS-CoV-2 RNA levels to 56.6% (Fig. 4D). Linear regression analysis (Fig. 4E) of viral infectivity (derived from Fig. 2A) with genome damage indicated a negative correlation (R2 = 0.75). Although the long RT-qPCR only targeted 1095 bp, 3.8% of the full-length genome, 43.4% of virus was detected with RNA damage, suggesting that potentially almost all virions had RNA genome damage after 30 s of UVC irradiation.

Figure 4
figure 4

Reverse-transcription quantitative-polymerase chain reaction (RT-qPCR) to determine the effect of ultraviolet C (UVC) irradiation on the viral genome. (A) Schematic diagram of the conventional RT-qPCR RT-priming site and qPCR primer sites. (B) Quantitative results of conventional RT-qPCR. SARS-CoV-2 (5 mL) with a titer of 5 × 104 50% tissue culture infective dose (TCID50/mL) was irradiated with a UVC light tube for increasing periods of time from 0 to 30 s; the viral RNA was extracted and then viral RNA copy number was determined. (C) Schematic diagram of the long RT-qPCR RT-priming site and qPCR primer sites. (D) Quantitative results of long RT-qPCR. SARS-CoV-2 (5 mL) with a titer of 5 × 104 TCID50/mL was irradiated with a UVC light tube for increasing periods of time from 0 to 30 s. The relative RNA fold change compared to 0 s irradiation is calculated. Data in the plot represent the mean ± standard deviation (SD) of three replicates. Significance has been determined using one-way analysis of variance followed by Dunnett’s multiple comparisons test. The asterisk indicates a statistical difference (*p < 0.05). (E) Linear regression analysis between relative viral genome damage and virus infectivity (derived from Fig. 2A) based on the long-RT-qPCR results. Relative genome damage is calculated as follows: (1-relative RNA fold change compared to control) × 100%. The data points that outside the axis limits are not shown in the graph.

Next, to further confirm that UVC caused SARS-CoV-2 RNA damage, four primer sets that covered the full-length viral genome were used for long RT-PCR analysis (target size for region 1: 8005 bp, region 2: 8221 bp, region 3: 7951 bp, and region 4: 6957 bp), together with the S gene (target size was 3747 bp) and the N gene (target size was 1465 bp) (Fig. 5A). As shown in Fig. 5B, all four regions and the S gene showed RNA damage after UVC irradiation in a time-dependent manner: Band signals in agarose gels were barely detectable after 30 s of UVC irradiation, suggesting that almost the entire virus genome contained RNA damage. Note that for the N gene region, signals were detectable after 30 s of UVC irradiation, which totally inactivated virus infectivity (Fig. 5B). This might be because the detection range of the N gene was relatively short and not all the UVC-irradiated virus contained genome damage within this region. In the quantitative analysis, band intensities of the control and UVC-treated group after 30 s of UVC irradiation consistently showed significant differences for all six regions; however, there was no significant difference in the N gene band intensity after 15 s of UVC irradiation (Fig. 5C). Moreover, by linear regression analysis (Fig. 5D), the RNA damage caused by UVC irradiation was strongly correlated with virus infectivity (derived from Fig. 2A) in all regions tested: region 1 (R2 = 0.76), region 2 (R2 = 0.94), region 3 (R2 = 0.89), region 4 (R2 = 0.75), S gene (R2 = 0.96) and the N gene (R2 = 0.88). Taken together, these results indicated that genome damage was the main mechanism of UVC-induced SARS-CoV-2 inactivation.

Figure 5
figure 5

Long reverse-transcription polymerase chain reaction (RT-PCR) to determine the effect of ultraviolet C (UVC) irradiation on the viral genome. (A) Schematic diagram of the six pairs of long RT-PCR primer sets. (B) Representative PCR products are visualized by agarose gel electrophoresis. Full-length gels are shown in Supplementary Fig. S2. SARS-CoV-2 (5 mL) with a titer of 5 × 104 50% tissue culture infective dose (TCID50/mL) was irradiated with a UVC light tube for increasing periods of time from 0 to 30 s. Viral RNA was reverse transcribed with the reverse primer for each region and then amplified with the corresponding primer sets. The amplified PCR products were used for 0.8% agarose gel electrophoresis and detected by ethidium bromide staining. (C) Band intensity is analyzed using CS Analyzer 4 software and quantitative results are shown in the bar diagram. Data in the plot represent the mean ± standard deviation (SD) of three replicates. Significance has been determined using one-way analysis of variance followed by Dunnett’s multiple comparisons test. The asterisk indicates a statistical difference (*p < 0.05; **p < 0.01; ***p < 0.001). (D) Linear regression analysis between relative viral genome damage and virus infectivity (derived from Fig. 2A). Relative genome damage is calculated as follows: (1-relative PCR fold change compared to control) × 100%.

Discussion

Implementation of environmental cleaning and disinfection by irradiation with UVC adequately removes microbial contamination from the environment. Indeed, UVC has recently inactivated SARS-CoV-2 and therefore may be applied in healthcare facilities for environmental disinfection29. However, the mechanism of action of how UVC inactivates SARS-CoV-2 is unclear. In this study, UVC efficiently disinfected SARS-CoV-2, mainly through viral genome damage. By transmission electronic microscopy observation and immunoblotting analysis with two monoclonal antibodies, no apparent effects on viral morphology and viral proteins were found. However, by the limitation of our experiment, we could not conclude that UVC does not damage proteins of SARS-CoV-2. In conclusion, our results support the idea that UVC is an effective countermeasure for SARS-CoV-2 disinfection in high-risk places, such as hospitals and airports.

There are two possible hypotheses regarding the mechanism of virus disinfection by UVC, either viral genome or viral protein damage. For damage to the viral genome, the UVC wavelength ranges from 200 to 280 nm, which is close to the absorption wavelength of nucleic acids, and thus may induce damage to the viral genome30. Our results demonstrated that genome damage was the main mechanism of UVC-induced SARS-CoV-2 inactivation. At the protein level, UVC treatment causes photo-damage to proteins through disulfide photolysis and oxygen radical oxidation31. Additionally, a report shows that UVC irradiation decreases MNV-1 capsid protein amounts, as measured by Coomassie staining20. However, by testing the effect of UVC on viral morphology and levels of SARS-CoV-2 viral spike/nucleocapsid proteins, no obvious protein damage was observed in this study. Indeed, UV-inactivated SARS-CoV vaccine has been shown the ability eliciting systemic humoral immunity against viral spike and nucleocapsid proteins in mice32, supporting the possibility that SARS-CoV-2 viral morphology and proteins are not under severe damage after UV treatment. One possible reason to explain the discrepancy is that viral proteins between different viruses might have different UVC susceptibilities, as adenoviral proteins have different susceptibilities to UVC33. In fact, UVC treatment of Tulane virus damages the viral capsid binding protein, whereas protein damage is not observed in porcine rotavirus under the same experimental condition34, supporting the idea that UVC inactivation mechanisms may vary across different viruses. A second reason is that the UVC wavelength used in each study might be different and therefore lead to inconsistent results of viral protein damage. Compared to UVC 254 nm, which is used in this research, UVC 220 nm more efficiently affects viral protein integrity in adenovirus33. A third possible reason might due to differences in the UVC fluency used in each publication. For example, MNV-1 protein is destroyed by UVC after 10 min of 8 W/cm2 irradiation, which is much higher than the current study (30 s of 500 μW/ cm2)20. A fourth reason may be oxidation of viral proteins during irradiation with UV 254 nm. For example, several viruses, including MS2, astrovirus, and norovirus are inactivated via oxidative damage of viral proteins18,19. Finally, in our experimental setting, we applied two monoclonal antibodies for testing protein damage; however, we could not rule out the possibility of existence of potential protein damage that occurred outside the antibodies recognition regions. Additional experiments, for example, detecting protein damage with polyclonal antibodies, mass spectrometry or NMR may provide substantial results for confirmation. In addition, whether UVC caused SARS-CoV-2 protein oxidation leading to a reduction in infectivity requires further investigation.

PCR-based methods e.g., qPCR is widely used for virus detection and infectivity measurements35,36. However, we and others have noted that UVC-induced viral genome damage is not detectable using conventional RT-qPCR, which is used in the clinic, even when the virus completely loses infectivity28. This inconsistency might lead to misinterpretation of environmental virus infectivity measurements after UVC disinfection. The reason for the detection failure of viral genome damage by conventional qPCR is due to its short range (< 200 bp); the damage is not detectable if it does not occur within this region. Therefore, analysis of longer regions of virus genome may more accurately inspect genome integrity. A similar phenomenon has been reported in the detection of UVC-induced damage in porcine parvovirus that tested viral genome damage using RT-PCR; the data shows that targeting a genome size of 2000 bp compared to 300 bp more accurately reflects virus infectivity37. In the current study, one long RT-qPCR (1095 bp) and six long RT-PCR assays (targeting regions ranging from 1465 ~ 8221 bp) were designed and applied to inspect viral genome damage that potentially includes strand break and pyrimidine dimer formation. Consistently, in the six long RT-PCR assays, regions 1 ~ 4, which target approximately 8000 bp, with 565–684 potential thymidine dimer sites, accurately reflected virus infectivity, as the PCR signal was not detectable in the group with 30 s UVC irradiation, where the virus was completely inactivated. In contrast, slight bands were observed in the S gene amplification products (3747 bp, with 332 potential thymidine dimer sites) and a clear band was observed in the N gene (1465 bp, with 70 potential thymidine dimer sites) amplification products after 30 s irradiation, though the virus had totally lost infectivity. These results emphasize the importance of the PCR targeting length for genome damage analysis, even though the long RT-qPCR and six long RT-PCR assays correctly reflected UVC-induced genome damage with virus infectivity (R2 ranging from 0.75 to 0.96). Therefore, the long RT-qPCR and six long RT-PCR assays that were developed might contribute to rapid and accurate infectivity inspection of post UVC-irradiated environments.

There are various types of light-based technology for virus inactivation. Among all three types of UV, UVC 253.7 nm has the strongest antimicrobial activity38. However, care should be taken during application, as exposure to these lamps is associated with health risks involving damage to the eyes and skin39. UVC (222 nm) has recently shown potential for SARS-CoV-2 disinfection27,28. Interestingly, UVC 222 did not harm skin when used on a mouse model, and therefore, has the capacity to be applied on external areas40. However, the safety determination of UVC 222 on humans requires further investigation. UVA, and UVB, which are present in natural sunlight with a lower risk to the human body, also inactivate SARS-CoV-2, although they have relatively low efficiency compared to UVC24,41. These results provide an alternative for UV-based disinfection, as UVC application should be avoided in live animals due to safety concerns. Blue light (380–500 nm) is less harmful to the human body compared to UV and exhibits germicidal activities, especially within the wavelength 400–500 nm42. LED blue light (413 nm) irradiation inactivating SARS-CoV-2 is documented43. The potential antiviral mechanism is via the generation of reactive oxygen species and thus, induces damage to proteins, lipids, and nucleic acids in the presence of photosensitizers44. Red light (600–700 nm) has lower risk for humans, but shows disinfection ability for Middle East Respiratory Syndrome-CoV and Ebola virus when combined with the use of methylene blue, which is widely used in plasma transfusions for pathogen reduction45,46. However, overall, red light-based inactivation is less efficient compared to UVC and non-enveloped viruses are less sensitive than enveloped viruses45,47. Taken together, all of the light-based technologies, with the different characteristics mentioned above, could be applied to virus inactivation. Based on the application purpose, the advantages and drawbacks of these tools should be evaluated. Thus, light-based technologies are a powerful and chemical-free agent that broadly disinfect various types of viruses. Therefore, these tools could potentially save people from the risk of infectious diseases. Furthermore, these technologies are also ideal for drug-resistant viruses, emerging viruses, such as Ebola virus, SARS-CoV, or other new infectious diseases in the future.

Materials and methods

Cells and virus

Vero E6/TMPRSS2 cells were obtained from the Japanese Collection of Research Bioresources (JCRB) Cell Bank in Japan (JCRB no. JCRB1819) and maintained in Dulbecco's modified Eagle medium (Thermo Fisher Scientific, Waltham, MA, USA) supplemented with 10% fetal bovine sera (FBS) (Sigma-Aldrich, St. Louis, MO, USA), 1% penicillin/streptomycin/glutamine (PSG), 2% G418 and cultured at 37 °C with 5% CO2. SARS-CoV-2 (SARS-CoV-2/JPN/TY/WK-521 strain) was a kind gift from the National Institute of Infectious Diseases of Japan48. For SARS-CoV-2 virus infection in VeroE6/TMPRSS2 cells, infection medium (Minimum Essential Medium Eagle (MEM, Thermo Fisher Scientific) containing 2% FBS and 1% PSG) was used. SARS-CoV-2 was propagated at a multiplicity of infection (MOI) = 10–5 for 3 days in Vero E6/TMPRSS2 cells. Viruses were titrated using 50% tissue culture infective dose (TCID50) assays. For the TCID50 assay, in brief, Vero E6/TMPRSS2 cells in a 96 well plate (2 × 104 cells per well) were infected with 100 μL of tenfold serially diluted virus-containing infection medium (each dilution had eight replicates) and were incubated at 37 °C for 3 days. Following incubation, viral infection in each well was determined using the virus-induced cell cytopathic effect (CPE). Viral titers were calculated using the Reed-Muench method49.

Inactivation of SARS-CoV-2 by UVC irradiation

A UVC light tube with a wavelength of 253.7 λ, 500 μW/cm2 (Bactericidal lamp GL16KSH; SANKYO DENKI Co., Ltd., Kanagawa, Japan), was set at a 30 cm height above the virus for the inactivation experiments (Fig. 1). The environmental temperature was controlled at 24 °C with 55% humidity. SARS-CoV-2 (5 mL) with a titer of 5 × 104 TCID50/mL was placed in 10 cm dishes for UVC irradiation for 5, 15, or 30 s. The post-UVC irradiated virus was then titrated using the TCID50 assay.

Virus morphology observation by TEM

SARS-CoV-2 (1 mL) with a titer of 1.78 × 106 TCID50/mL was irradiated with a UVC light tube for 60 s. The post-irradiated virus (100 μL) was mixed with 2.5% glutaraldehyde (1 mL) for TEM negative staining. For TEM sample preparation, a droplet of the virus mixture was placed on a carbon-film grid for 10 s. After the grid was partially dried, a droplet of staining solution, 2% uranyl acetate, was added for a 10 s incubation. The excess liquid was wiped off with filter paper, and the grid was dried at room temperature before imagining using a HITACHI H-7600 electron microscope (Hitachi Global Life Solutions, Inc. Tokyo, Japan) at 100 kV.

Viral protein damage detection by immunoblotting

SARS-CoV-2 (1 mL) with a titer of 1.78 × 106 TCID50/mL was irradiated with a UVC light for 5, 15 or 30 s. A volume of 20 µL of virus-containing medium was mixed with 5 µL sample buffer (0.15 M Tris–HCl, 10% sodium dodecyl sulfate (SDS), 30% glycerol, and 0.5% bromophenol blue) and heated at 100 °C for 5 min. The 15 µL denatured virus solution was loaded onto a 10% (for spike protein detection) or 12% (for nucleocapsid protein detection) SDS–polyacrylamide gel and electrophoresed in running buffer containing 0.3% Tris, 0.1% SDS, and 1.44% glycine. The proteins were then transferred onto a polyvinylidene difluoride membrane (Millipore, Billerica, MA, USA) using a Trans-Blot Turbo apparatus (Bio-Rad, Hercules, CA, USA) and incubated with anti-SARS-CoV-2 spike monoclonal antibody (Mab) (1A9) (1:1000; Genetex, Irvine, CA, USA), anti-SARS-CoV-2 nucleocapsid Mab (6H3) (1:2000; Genetex) at 4 °C overnight. After washing, the membranes were incubated with horseradish peroxidase-conjugated AffiniPure goat anti-mouse IgG (1:2000; Jackson ImmunoResearch, West Grove, PA, USA) at room temperature for 1 h. Signals were visualized after treating the membrane with SuperSignal™ West Pico PLUS Chemiluminescent Substrate (Thermo Fisher Scientific). Images were acquired using a WSE-6100 LuminoGraph I (Atto Corporation, Tokyo, Japan). Densities of bands were analyzed using CS Analyzer ver.4 (Atto Corporation) (https://www.atto.co.jp/eng/products/geldocumentation/Image-analysis-software/Image-Analysis-Software2).

RT-qPCR

SARS-CoV-2 (5 mL) with a titer of 5 × 104 TCID50/mL was irradiated using a UVC light for 5, 15 or 30 s. Viral RNA was then extracted using a QIAamp Viral RNA Mini Kit (Qiagen, Hilden, Germany), following the manual instructions. For conventional RT-qPCR, a volume of 5 µL RNA was used for a one-step RT-qPCR reaction using a QuantiTect Probe RT-PCR Kit (Qiagen) with 600 nM forward primer (CACATTGGCACCCGCAATC), 800 nM reverse primer (GAGGAACGAGAAGAGGCTTG), 200 nM Taqman probe (FAM-ACTTCCTCAAGGAACAACATTGCCA-QSY), and an Applied Biosystems 7500 Fast Real-Time PCR system (Thermo Fisher Scientific), as reported previously50. For long RT-qPCR, a 5 µL volume of RNA was first used for reverse transcription with SARS-CoV-2 4R primer (CTCTTCCATATAGGCAGCTCT) using the SuperScript™ III First-Strand Synthesis System (Invitrogen, Foster, CA, USA), following the manual instructions. A total of 1.25 µL cDNA was used for the qPCR analysis, which was identical to the conventional RT-qPCR procedure above. Samples were evaluated in triplicate and data analysis was performed using the comparative CT method (∆∆CT).

Long RT-PCR

SARS-CoV-2 (5 mL) with a titer of 5 × 104 TCID50/mL was irradiated using UVC for 5, 15 or 30 s. Viral RNA was then extracted using a QIAamp Viral RNA Mini Kit (Qiagen), following the manual instructions. Reverse transcription was performed using the SuperScript™ III First-Strand Synthesis System (Invitrogen) and was followed by PCR amplification using PrimeSTAR GXL with a gene-specific primer. For region 1, RT was conducted using the SARS-CoV-2 reverse primer 1R2 (GAATCAACAAACCCTTGCCGA). The generated cDNA was then amplified with the SARS-CoV-2 primers 1F2 (GCTTACGGTTTCGTCCGTGT) and 1R2 using the following thermal cycling program: 98 °C for 1 min, followed by 30 cycles of 98 °C for 10 s, 57 °C for 15 s and 68 °C for 8 min. For region 2, RT was conducted using the SARS-CoV-2 reverse primer 2R (GACATCAGCATACTCCTGATTA). The generated cDNA was then amplified with the SARS-CoV-2 primers 2F (GACAACCTGAGAGCTAATAACAC) and 2R using the following thermal cycling program: 98 °C for 1 min, followed by 30 cycles of 98 °C for 10 s, 55 °C for 15 s and 68 °C for 8 min. For region 3, RT was conducted using the SARS-CoV-2 reverse primer 3R (TGCTGCATTCAGTTGAATCAC). The generated cDNA was then amplified with the SARS-CoV-2 primers 3F (GGACCTCATGAATTTTGCTCT) and 3R using the following thermal cycling program: 98 °C for 1 min, followed by 30 cycles of 98 °C for 10 s, 55 °C for 15 s and 68 °C for 8 min. For region 4, RT was conducted using the SARS-CoV-2 reverse primer 4R3 (GCCTCGGTGAAAATGTGGTG). The generated cDNA was then amplified with the SARS-CoV-2 primers 4F5 (TCAGACAAATCGCTCCAGGG) and 4R3 using the following thermal cycling program: 98 °C for 1 min, followed by 30 cycles of 98 °C for 10 s, 57 °C for 15 s and 68 °C for 7 min. For the S gene region, RT was conducted using the S gene reverse primer R2 (GACTCCTTTGAGCACTGGCT). The generated cDNA was then amplified with the S gene primers F2 (ACCAGAACTCAATTACCCCCTG) and R2 using the following thermal cycling program: 98 °C for 1 min, followed by 30 cycles of 98 °C for 10 s, 57 °C for 15 s and 68 °C for 4 min. For the N gene region, RT was conducted using the SARS-CoV-2 reverse primer 4R3. The generated cDNA was then amplified with the N gene primers F (ATGTCTGATAATGGACCCCA) and R (TTAGGCCTGAGTTGAGTCAG) using the following thermal cycling program: 98 °C for 1 min, followed by 30 cycles of 98 °C for 10 s, 57 °C for 15 s and 68 °C for 1.5 min. A volume of 5 μL of the amplified PCR products was then used for 0.8% agarose gel electrophoresis and bands were detected by ethidium bromide staining. The band intensities were quantitated using a WSE-6100 LuminoGraph I (Atto Corporation) and were analyzed using CS Analyzer ver.4 (Atto Corporation).

Statistical analysis

All data are expressed as the mean ± standard deviation based on at least three independent experiments. Data were analyzed using analysis of variance with Dunnett’s multiple comparison test in Prism (GraphPad, San Diego, CA, USA). p values smaller than 0.05 were considered significant. Linear regression analysis of virus infectivity with UVC irradiation time, and virus infectivity with virus genome damage were analyzed using Prism. Virus genome damage was calculated as follows: (1-relative PCR fold change compared to control) × 100%.