Cells and viruses

Huh-7 cells were obtained from C. M. Rice and were cultured as described previously. ^{Reference Amador-Canizares, Bernier, Wilson and Sagan10} HCT-8 and VeroE6 cells (ATCC) were grown in Dulbecco’s modified Eagle medium (DMEM) with 10% heat-inactivated fetal bovine serum (FBS), L-glutamine, and nonessential amino acids. HCoV-229E (ATCC) was propagated and titered in Huh-7 cells at 33°C under a 5% CO₂ atmosphere, based on reported optimal growth conditions. ^{Reference Dijkman, Jebbink and Koekkoek8,Reference Szczepanski, Owczarek and Bzowska11} For propagation, infections were performed for 2 hours in OPTI-MEM (Life Technologies) with rocking every 15 minutes. The inoculum was then removed and replaced with infection media (complete DMEM + 2% FBS). When cytopathic effects (CPE) were apparent in ∼80% of cells (∼5 days after infection), viral supernatants and cell-associated virus were recovered using 3 freeze–thaw cycles. Cellular debris was pelleted by centrifugation, and viral stocks were recovered and stored at −80°C. HCoV-OC43 (ATCC) was propagated in HCT-8 and titered in Vero-E6 cells as described above.

SARS-CoV-2 (isolate RIM-1, Genbank accession no. MW599736) was isolated from a quantitative reverse-transcriptase polymerase chain reaction (PCR)–positive patient sputum sample at the RI-MUHC using tosyl phenylalanyl chloromethyl ketone (TPCK)–treated VeroE6 cells as previously described. ^{Reference Banerjee, Nasir and Budylowski12} Viral stocks prepared in VeroE6 cells at 37^oC under 5% CO₂. Supernatants were collected 3 days after infection, were concentrated 5–10-fold using an Amicon Ultra-15 centrifugal filter unit (100 KDa cutoff), and stored at −80°C. All cell lines were routinely screened for mycoplasma contamination using the MycoAlert mycoplasma detection kit (Lonza).

Plaque assays

HCoV-229E was titered by plaque assay using 10-fold serial dilutions in Huh-7 cells. Infections were carried out as for viral propagation, with the exception that 2% methylcellulose was included in the media to restrict viral diffusion. At 5 days after infection, cells were washed with phosphate-buffered saline (PBS) and fixed with formal saline for 1 hour at RT. Cells were washed with ddH₂O and stained with 0.1% crystal violet for 30 minutes. Excess of stain was removed, and viral titers (in plaque-forming units, PFU) were estimated using equation 1:

(1) $$PFU/mL = average\;no.\;of\;plaques/(dilution\;factor \times \;infection\;volume)$$

TCID ₅₀ assays

For HCoV-OC43 and SARS-CoV-2, sample titers were measured using the median tissue culture infectious dose (TCID₅₀) assay using 10-fold serial dilutions in Vero-E6 cells. Cells were infected for 1 hour, after which the inoculum was removed and replaced with infection media. After 3 or 5 days for SARS-CoV-2 and HCoV-OC43, respectively, cells were fixed and stained as described above. Viral titers were calculated using the the Reed-Muench method that estimates TCID₅₀/mL. ^{Reference Ramakrishnan13}

Quantitative RT-PCR analysis

For total RNA isolation, infection was monitored for CPE and cells were harvested at day 4 after infection. Briefly, cells were washed with PBS, lysed in TriZol, and total RNA was isolated according to the manufacturer’s instructions. Two sets of primers (targeting the RNA-dependent RNA polymerase (RdRp) and Nucleocapsid (N) genes) were used for gene-specific reverse transcription and amplification, except for SARS-CoV-2, which was analyzed using RdRp only (Supplementary Table 1 online). Complementary DNA (cDNA) was synthesized with M-MuLV RT (NEB) using 500 ng of total RNA, according to the manufacturer’s instructions. Quantitative real-time PCR amplification was carried out using SYBR Green technology with the iTaq Universal SYBR Green PCR master mix according to the manufacturer’s instructions. Genome copies were calculated using a standard curve, and fold differences in gene expression were calculated using the 2^–ΔΔCt method. ^{Reference Livak and Schmittgen14}

HCoV inactivation assays

Using procedures established by NIOSH, 2 × 2-cm coupons were cut from sterile N95 respirators in the biological safety cabinet (BSC) and affixed with a single staple. Coupons were placed in a 6-well tissue culture dish and 20 × 3 µL droplets of HCoV-229E stock (4.8 × 10⁸ PFU/mL), HCoV-OC43 (1.67 × 10⁴ TCID₅₀/mL), or SARS-CoV-2 (1 × 10⁷ TCID₅₀/mL) were placed on each coupon. Coupons were dried in the BSC for 0.5–1 hour and were either untreated (no UV) or treated with GUV using the small (Sanuvox Technologies) or large (LifeAire Systems LLC) devices. The small device is a cardboard box [38 cm × 30.5 cm × 24 cm (15 inches × 12 inches × 9.5 inches); 1.3 kg (3 pounds)] with 2 U-shaped bulbs (above and below) and capacity for 1 respirator suspended by its straps. The exposure time can be manipulated as needed. The large device is a polished aluminum box [109 cm × 71 cm × 61 cm (43 inches × 28 inches × 24 inches)] with a capacity of ∼20 N95 respirators. Both devices are designed to deliver 0.5 to 1.0 J/cm ^{Reference Kowalski, Bahnfleth and Hernandez2} .

For the small UV device, coupons in a 6-well plates were placed in the center of the unit and exposed to UV for 2.5 minutes. For the large device, coupons were treated for 2.5 minutes, flipped with sterile tweezers, and treated for another 2.5 minutes (UV delivery is top down in this device). UV exposure was confirmed using UVC 1,000 dosimeters, and according to the indicator, coupons were exposed to 0.5 J/cm ^{Reference Kowalski, Bahnfleth and Hernandez2} . Coupons were then rehydrated in 1.5 mL OPTI-MEM for 1 hour at RT and the media was recovered using a cell strainer (40 µm) and centrifugation at 4,000 rpm for 2 minutes. For HCoV-229E, recovered virus was titered by plaque assay; for HCoV-OC43 and SARS-CoV-2, recovered virus was titered by TCID₅₀ assay. Log reductions were calculated using equation 2:

(2) $$log\ reduction\ value = R_c - R_u$$

where R _c is mean viable virus recovered from control coupons (log PFU/mL or log TCID₅₀) and R _u is viable recovery from UV-exposed coupons (log PFU/mL or log TCID₅₀).

For whole-mask testing, intact N95 respirators (folded particulate respiratory, SAS Safety Corp) were spotted with HCoV-229E (as described above) in 4 zones: (1) nose, (2) right cheek, (3) left cheek, and (4) chin. Contaminated respirators were subjected to GUV treatment, then coupons were cut and processed as described above.

Data analysis

Statistical analyses were performed using GraphPad Prism version 7 software (GraphPad, San Diego, CA). No a priori statistical power calculation was conducted. Sample size was based on similar previous studies. ^{Reference Mills, Harnish, Lawrence, Sandoval-Powers and Heimbuch4,Reference van Vlymen, Magnus and Jaeger15,Reference Fisher, Noti, Lindsley, Blachere and Shaffer16} All data are representative of 3 independent experiments with 3 independent replicates per experiment (n = 9). All data points represent 3 independent measurements per replicate, and error bars represent standard deviation (SD). Statistical significance was determined using an unpaired t test.