key: cord-0839177-0ky48bvb
authors: Baldelli, Giulia; Aliano, Mattia Paolo; Amagliani, Giulia; Magnani, Mauro; Brandi, Giorgio; Pennino, Carmelo; Schiavano, Giuditta Fiorella
title: Airborne Microorganism Inactivation by a UV-C LED and Ionizer-Based Continuous Sanitation Air (CSA) System in Train Environments
date: 2022-01-29
journal: Int J Environ Res Public Health
DOI: 10.3390/ijerph19031559
sha: 1b8ef82f6ec0026438530a67e071660ae70839a4
doc_id: 839177
cord_uid: 0ky48bvb

Improving indoor air quality present in environments where people live is important to protect human health. This particularly applies to public transportation, where air quality may affect the health and safety of passengers, workers and staff. To provide better air quality, many buildings and transports are provided with heating, ventilation and air conditioning (HVAC) systems, which are always equipped with filters to retain the particulate present in the airflow, but they lack continuous air sanitization systems. In this study, a new UV-C LED and ionizer-based continuous sanitation air (CSA) system to be installed in a train HVAC was developed (international patent: N.PCT/IB2021/054194) and its sanitation efficacy against various microbial species (bacteria and fungi) was assessed. The device proved to be very effective at the microbial killing of aerodispersed microorganisms, both in its experimental configuration (ISO 15714:2019) and in a train setting. The installation of this CSA system on public transportation appears to be a promising solution to guarantee high microbiological air quality with a very low environmental impact due to its eco-friendly components.

The hygienic quality of the air and surfaces of indoor environments can affect the health of people living and working in them due the presence of different microorganisms, physical and chemical factors, pollutants, and particulate matter [1] . Eight major sources of airborne microbiotes found in indoor environments have been identified, including: humans; pets; plants; plumbing systems; heating, ventilation, and air-conditioning (HVAC) systems; mold; dust resuspension; and the outdoor environment [2] . Moreover, the type, survival and spread of airborne microorganisms are also tightly linked to physically favorable environmental parameters, such as relative humidity (RH, %) and temperature (T, • C) [3] . The daily air inhaled by a human typically contains average loads of 10 6 airborne microorganisms [4] , some of which can be pathogenic and cause illnesses of different severity, from flu to COVID-19, pneumonia, asthma, or allergies [5] [6] [7] [8] .

Indoor airborne microbial content is detected in variable concentrations, depending on seasonal changes and on the considered environment [9] [10] [11] . Microbial loads of 10 2 -10 3 CFU/m 3 have been detected in public transportation environments [12, 13] . Particular The UV-C LEDs produce light rays with a specific wavelength (275 ± 5 nm) starting from small amounts of electricity (in the order of a few mWs) with a low thermal resistance. To maximize UV-C radiation, the sub-ducts were designed with particular geometries and special surface treatments that increase the number of UV-C ray reflections in the air path ( Figure 2 ). The color scale is representative of the radio frequency exposure power (mW/cm 2 ) and to the refraction.

Escherichia coli (ATCC 25922), Bacillus subtilis (ATCC 6633) and Cladosporium spp. were selected as test microorganisms, in accordance with the ISO 15714:2019 standard [26] . Bacillus subtilis (ATCC 6633) and Cladosporium spp. were selected in accordance with the ISO 15714:2019 standard [26] . The same standard also included Serratia marcescens. However, instead of this species, the microorganism Escherichia coli was used as it belongs to the same family (Enterobacteriaceae) and shows a similar UV-C susceptibility (as reported in the ISO 15714:2019, Annex C), but entails a lower biological risk for operators. The UV-C LEDs produce light rays with a specific wavelength (275 ± 5 nm) starting from small amounts of electricity (in the order of a few mWs) with a low thermal resistance. To maximize UV-C radiation, the sub-ducts were designed with particular geometries and special surface treatments that increase the number of UV-C ray reflections in the air path ( Figure 2 ). ionizer and the filter in the first portion. After the filter, the main duct is split into subportions that divide the airflow in the sub-conducts. The UV-C LEDs are arranged in these sub-ducts to sanitize the airflow and the internal surface of the filter; moreover, some other LEDs are placed on the ionizer to sanitize the external filter surface. The sensor platform, placed at the end of the duct, make it possible to continuously check the air quality parameters such as pressure, airflow speed, temperature, relative humidity, atmospheric particulate matter (PM10, PM4, PM2), and gaseous pollutants (VOC, CO2, O3, H2S). The UV-C LEDs produce light rays with a specific wavelength (275 ± 5 nm) starting from small amounts of electricity (in the order of a few mWs) with a low thermal resistance. To maximize UV-C radiation, the sub-ducts were designed with particular geometries and special surface treatments that increase the number of UV-C ray reflections in the air path ( Figure 2 ). The color scale is representative of the radio frequency exposure power (mW/cm 2 ) and to the refraction.

Escherichia coli (ATCC 25922), Bacillus subtilis (ATCC 6633) and Cladosporium spp. were selected as test microorganisms, in accordance with the ISO 15714:2019 standard [26] . Bacillus subtilis (ATCC 6633) and Cladosporium spp. were selected in accordance with the ISO 15714:2019 standard [26] . The same standard also included Serratia marcescens. However, instead of this species, the microorganism Escherichia coli was used as it belongs to the same family (Enterobacteriaceae) and shows a similar UV-C susceptibility (as reported in the ISO 15714:2019, Annex C), but entails a lower biological risk for operators. 

Escherichia coli (ATCC 25922), Bacillus subtilis (ATCC 6633) and Cladosporium spp. were selected as test microorganisms, in accordance with the ISO 15714:2019 standard [26] . Bacillus subtilis (ATCC 6633) and Cladosporium spp. were selected in accordance with the ISO 15714:2019 standard [26] . The same standard also included Serratia marcescens. However, instead of this species, the microorganism Escherichia coli was used as it belongs to the same family (Enterobacteriaceae) and shows a similar UV-C susceptibility (as reported in the ISO 15714:2019, Annex C), but entails a lower biological risk for operators. E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/L cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32 • C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32 • C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD 600 ), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/mL. Cladosporium spp.

was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/L chloramphenicol at 25 • C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD 530 ) to a final concentration of 10 6 CFU/mL. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed.

E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred Air-intake/air inlet/inflow/entrance; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred variable flow rate blower;

E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred HEPA filter; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred upstream duct; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred UVGI device mounting duct; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. Figure 3 . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred downstream duct; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. Figure 3 . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred off-gas pipe; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred nebulizer; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred upstream microorganism sampling port; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. Figure 3 . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred CSA system; E. coli was grown in tryptic soy agar (TSA) plates supplemented with 0.05 g/l cycloheximide and B. subtilis (vegetative form) in brain heart infusion (BHI) agar, both at 32°C. Overnight cultures of bacterial strains in tryptic soy broth (TSB) at 32°C were washed and resuspended in saline solution (NaCl 0.9%), then adjusted at optical densities at 600 nm (OD600), corresponding to a final concentration of 10 8 (E. coli) and 10 7 (B. subtilis) CFU/ml. Cladosporium spp. was grown in agar slant tubes containing malt extract agar (MEA) with 0.05 g/l chloramphenicol at 25 °C for at least 72 h. The fungal suspension was prepared pouring saline solution over Cladosporium spp. slants to gently swirl and detach fungal conidia. The fungal suspension was then diluted to optical density at 530 nm (OD530) to a final concentration of 10 6 CFU/ml. The microorganism suspensions' concentrations were experimentally confirmed by plate culture. All culture materials were purchased from Thermo Fisher Scientific (Waltham, MA USA).

A test rig was built in compliance with the standard for the experimental testing procedures ( Figure 3 ) [26] . It included: (a) a variable flow rate blower, used to control the flow rate of the test system, installed in front of the test rig; (b) a HEPA filter placed before the upstream duct to remove potentially contaminating airborne microorganisms present in the air, in order to prevent their impact on test microorganism quantification; (c) an upstream duct equipped with a nebulizer connected to a test microorganism injection port less than 20 mm in diameter, set near the left flange of the duct; (d) the CSA system mounting duct; (e) a downstream duct with a sampling port for downstream sampling, set near the right flange of the duct; (f) an off-gas pipe. The ducts were made of aluminum and had a square cross-section and an inner side length of 600 mm. The individual ducts had a length of 1250 mm each and were connected and sealed by an insulating material, to avoid air leakage during the experiment. Inside each sampling port, a perforated cylindric tube (110 mm in diameter, with five holes of 20 mm in diameter) was placed to accommodate the head of the air sampler. The sampling ports were set to the central line of the lower wall and were closed during the test. The air outflow was funneled in a chamber with a single outtake opening and a HEPA filter of 110 m 3 in volume. Inside this chamber, a digitally controlled thermic nebulizer, equipped with an HP3 germicide, was placed. Figure 3 . Test rig configuration. ① Air-intake/air inlet/inflow/entrance; ② variable flow rate blower; ③ HEPA filter; ④ upstream duct; ⑤ UVGI device mounting duct; ⑥ downstream duct; ⑦ off-gas pipe; ⑧ nebulizer; ⑨ upstream microorganism sampling port; ⑩ CSA system; ⑪ downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred downstream microorganism sampling port.

The air was sampled with a Surface Air System sampler (SAS, PBI International, Milan, Italy), collecting air for 1 min, with an air volume of 180 L impacting the agar plates (TSA 0.05 g/L cycloheximide, BHI agar and MEA 0.05 g/L chloramphenicol). For each test, the air was sampled three times. After the air samplings, the agar plates were transferred to the laboratory in refrigerated conditions, then incubated at 32 • C for 24-48 h (E. coli and B. subtilis) or 25 • C for 72-120 h (Cladosporium spp.). The colony forming unit per cubic meter of air (CFU/m 3 ) was then calculated using the following formula: CFU/m 3 = number of colonies in each plate air volume sampled (l) × 1000 (1)

The assessment of the performance of the CSA system was carried out according to the standard [26] . A liquid nebulizer for suspensions (Collison nebulizer, AGK 2000 Palas GmbH, Karlsruhe, Germany) was used to generate an aerosol of the test microorganisms, upstream of the CSA system. The nebulizer was connected to a compressor equipped with particulate, water and oil repellent filters. The pressure was set at 3 atm throughout the tests. The nebulization was maintained for 2 min for each test, which was the time required to nebulize 1 ml of the microbial suspension. To achieve a correct initial microbial dispersion, during the aerosolization of the microorganisms, the airflow rate was maintained at 320 m 3 /h. The disinfection efficacy of the CSA system was tested at three different airflow rates: 1000, 2000 and 3000 m 3 /h. The air was sampled upstream and downstream of the CSA system; the downstream samples were obtained with the sanitation system switched off and switched on to calculate the sanitation efficiency. Moreover, the contribution of each CSA system component (UV-C LED, Electrostatic Space Charge System (ESCS) ionizer and ISO Coarse 90% filter) to the induction of the air sanitation was separately considered in the test rig configuration, nebulizing E. coli suspension, with a 3000 m 3 /h airflow rate. For this purpose, the experiment was repeated by switching on one element at a time or removing/installing the filter. Temperature ( • C) and relative humidity (% RH) were registered with the validated sensor of the CSA system before and after each experimental session.

The assessment of the performance of the CSA system was subsequently carried out in a Vivalto train setting.

Background microbial load. Before each experiment, an initial air sample from the train car (in a median position in the coach and in the proximity of the air vents) was obtained to determine the environmental bacteria (TSA) and fungi (Potato Dextrose Agar) concentrations.

Inactivation test. The nebulization step was performed as previously described. To produce a dispersed aerosol of E. coli and to reach the desired concentration of aerosolized microorganism, a nebulization pre-chamber was built and located in the vicinity of the train car return air panels. After nebulizing the suspension for 2 min, the aerosolized microorganisms were aspirated by the conditioning system and passed through the CSA system. The air was sampled in the vicinity of the train car supply air panels, with the airflow switched on. To obtain results as representative as possible of the entire train car, eight different air vents were selected as sampling points: the proximal, centra, and distal air vent panels of the upper central section of the train car; the proximal, central and distal air vent panels of the lower central section of the train car; and the proximal and distal air vent panels in the terminal section of the train car ( Figure 4 ). In the Vivalto air handling unit, the airflow rate was 4000 m 3 /h. The airflow rate overflowing from the air vent panels was measured with an anemometer at each sampling point considered. Air samples at the nebulization pre-chamber were also obtained The experiments were carried out in the train car without the CSA system; next, the disinfection device was placed in the air conditioning system and the tests were performed with the CSA system switched on. Temperature and relative humidity were registered as described above. 

The air disinfection efficiency of CSA system was expressed as inactivation rate (% IR), applying the following formula:

in which A is the microbial concentration (CFU/m 3 ) sampled downstream of the CSA system with the disinfection device switched off and the ISO Coarse 90% filter removed, while B is the microbial concentration (CFU/m 3 ) sampled downstream of the CSA system with the disinfection device switched on and ISO Coarse 90% filter installed.

The UV dose needed for the inactivation of the microbial species used in this study can be determined by the inactivation rate and the microbial susceptibility (k). The UV dose was determined according to the standard [26] :

where N0 is the original active microorganism concentration, N is the active microorganism concentration after disinfection, D is the UV dose and k is the susceptibility constant. k was obtained from Annex C of the standard and it was 0.38 m 2 /J for E. coli (average of different studies), 0.16858 m 2 /J for B. subtilis and 0.0021 for Cladosporium spp. [26] . 

The air disinfection efficiency of CSA system was expressed as inactivation rate (% IR), applying the following formula:

in which A is the microbial concentration (CFU/m 3 ) sampled downstream of the CSA system with the disinfection device switched off and the ISO Coarse 90% filter removed, while B is the microbial concentration (CFU/m 3 ) sampled downstream of the CSA system with the disinfection device switched on and ISO Coarse 90% filter installed.

The UV dose needed for the inactivation of the microbial species used in this study can be determined by the inactivation rate and the microbial susceptibility (k). The UV dose was determined according to the standard [26] :

where N 0 is the original active microorganism concentration, N is the active microorganism concentration after disinfection, D is the UV dose and k is the susceptibility constant. k was obtained from Annex C of the standard and it was 0.38 m 2 /J for E. coli (average of different studies), 0.16858 m 2 /J for B. subtilis and 0.0021 for Cladosporium spp. [26] .

The experiments were carried out over periods of different months. The temperature and % RH registered before and after each experimental session were included in a range of 18-33 • C and 42-63% RH. In the train setting, the microclimatic parameters ranged as follows: 19-24 • C and 43-57% RH. The duplicate assessment of each parameter indicated that the relative difference in the same index was less than 10%, ensuring the stability of the testing system. However, the relative variations of the same parameters at the beginning and at the end of the experimental session were occasionally higher than 10%.

The air samples taken upstream of the CSA system in the test rig were useful to check the concentration of microorganisms aerosolized during the tests. These concentrations, after a 2 min aerosolization during which an airflow rate of 320 m 3 /h was maintained, were the following: 7.5 ± 0.17 × 10 3 CFU/m 3 (E. coli); 1.91 ± 0.13 × 10 3 CFU/m 3 (B. subtilis); 1.09 ± 0.02 × 10 3 CFU/m 3 (Cladosporium spp.). The microbial concentrations of the aerodispersed microorganisms were also measured downstream of the CSA system, with the sanitation system switched off and the ISO Coarse 90% filter removed, or with the sanitation system switched on and the ISO Coarse 90% filter installed. Inactivation percentages of the bacterial species, E. coli and B. subtilis, were always very high and ranged from 98.96 to 100%. Lower % IR were instead obtained for Cladosporium spp. (67.88-69.45%) ( Table 1) . These data showed a mean reduction of 2 log for aerosolized E. coli and 2-3 log for aerosolized B. subtilis. For all tested microorganisms, the % IR were not affected by the three different airflow rates used in this study (Table 1) . 67.88 ± 1.3 * "off": test performed with the sanitation system switched off and the ISO Coarse 90% filter removed; "on": test performed with the sanitation system switched on and the ISO Coarse 90% filter installed. % IR: inactivation rate.

The assessment of each CSA system component (UV-C LED, ESCS ionizer and ISO Coarse 90% filter) contribution to the sanitization of the air from E. coli, with a 3000 m 3 /h airflow rate, showed that the greatest % IR was achieved by the UV-C LED, leading to a 97.02 ± 1.06% efficiency, in comparison to the 98.96 ± 0.6% achieved by the entire CSA system. On the other hand, the ESCS or the ISO Coarse 90% filter alone led to lower sanitation efficiency (89.48 ± 0.08% and 88.69 ± 0.37%, respectively) ( Figure 5 ).

system. On the other hand, the ESCS or the ISO Coarse 90% filter alone led to lower sanitation efficiency (89.48 ± 0.08% and 88.69 ± 0.37%, respectively) ( Figure 5 ). (Table 2) were, on average, 95.45 ± 1.46%, 92.69 ± 3.00% and 93.12 ± 1.19% in the upper, lower and terminal sections of the train car, respectively. 

The background microbial load was always around 50-200 CFU/m 3 (bacteria) and 100 CFU/m 3 (fungi). Near the air vents, a microbial load around 50 CFU/m 3 (bacteria) and 80 CFU/m 3 (fungi) was recorded. The airflow rate overflowing from the air vent panels, measured with an anemometer at each sampling point considered, ranged from 0. (Table 2) were, on average, 95.45 ± 1.46%, 92.69 ± 3.00% and 93.12 ± 1.19% in the upper, lower and terminal sections of the train car, respectively. 

The UV doses for each microorganism and at each airflow rate are reported in Table 3 . In the train setting, the UV doses ranged from 3.99 to 10.32 J/m 2 . 

Air sanitation in crowded environments, such as in public transportation, is of paramount importance to provide healthy and safe travel conditions to passengers and workers. In this study, a new air sanitation device, consisting of multiple components with a sanitizing effect (UV-C, filter and ionizer), was designed to be installed in an HVAC system and tested for its efficiency at microbial inactivation. The aerodispersed microorganism UV-C susceptibility strongly depends on different factors, including the ability of different microbial species to recover UV radiation-induced damage, the UV dose, irradiance, RH, exposure time, and the particulate/moisture present in the air [25, 28] . As required by the standard, three microorganisms with different UV-C susceptibility levels were chosen [26] . The first experiments aimed to calculate the percentage of IR of the CSA system for each microorganism in the test rig configuration [26] . The results highlighted the optimal inactivation efficiency with bacterial species (E. coli and B. subtilis) at all the airflow rates tested. A minor effect with filamentous fungi (Cladosporium spp.), known to be more resistant to UV-C, was instead noticed [26, 29] .

The estimated UV-C dose (D) required for the inactivation of each specific microorganism depends on different factors: the airflow rate, the microbial susceptibility, and the IR. Indeed, the longer a microbe is exposed to UV-C light, the higher the UV-C dose it will receive; therefore, D is inversely proportional to the airflow rate (1000, 2000, 3000 m 3 /h) used in the test rig. Moreover, the UV-C LED sanitation efficacy is inversely proportional to the distance from the UV-C LED source [30] . In the proposed device, the UV-C dose led to an optimal inactivation rate even with a high airflow rate, of 4000 m 3 /h. This result was due to the patented structure of the sub-ducts, which made it possible to subdivide the airflow, thus reducing the airflow rate, and to decrease the distance of the UV-C source. Considering the IR/retention separately provided by each different component of the CSA system, a prevalent effect of the UV-C was deduced. Our results allowed us to exclude that the filter or the ionizer alone may have a sufficient efficacy to provide optimal levels of microbial inactivation or retention in order to ensure air sanitation. According to previous results, the link between the inactivation of microorganisms and the ionizer seems to be mainly related to the ozone produced and not to the electroporation itself, suggesting that the bactericidal action attributed to ionizers may have been overestimated [31] . In the train setting, a very high IR was confirmed with E. coli. Besides the microbial susceptibility and flow rate, the performance of an in-duct sanitation device can be affected by temperature and RH, although microclimatic parameters have been considered less important [26] . In our experiments, these parameters were sometimes slightly different from those indicated as optimal in the standard method (25 ± 2.5 • C and 50 ± 10%) [26] , especially at the beginning of the experimental session, and reflected seasonal variations in climate. Moreover, it is important to highlight that an inverse relationship exists between RH, temperature, and the efficacy of UV devices, with a lower IR result at higher RH and lower temperature [28, 32] . Therefore, the initial RH of lower than 40% and the temperature higher than 27.5 • C assessed in some experimental sessions could have partially decreased the IR of the sanitation device. However, it should be noted that, during the experimental sessions, the parameters normalized and, in the second part of the tests, in which the sanitation device was switched on, they were almost always within the range of acceptability. For this reason, it can be hypothesized that these small differences did not affect the IR results. It is known that some components of the HVAC system could be sources of microbial contamination and spreading. In particular, filters, which retain microorganisms, dust, and particulate matter, can be colonized by the microbial component, which can grow and be released from the filter, in favorable environmental conditions [33] . Furthermore, HVAC systems are regularly stopped to save energy. Throughout these periods of ventilation stoppage, the microbial populations collected by the filters are not exposed to airflow and, consequently, the microorganisms are less subject to desiccation phenomena. Thus, if certain conditions occur (such as humidity level, temperature and nutrients), microorganisms can grow significantly during these stoppages of HVAC systems and fungal spores in particular can germinate and grow [34, 35] . Consequently, airborne pathogens may spread to other indoor spaces through air-conditioning return air ducts when they are reactivated. The CSA device proposed and evaluated in this study, with a filter exposed to UV-C LED irradiation, does not present these drawbacks. Previous studies have shown that the disinfection efficacy of in-duct UV-C lamps is increased by 20% when considering the duct wall reflection, compared to under non-reflection conditions [22] . In the CSA system, the reflecting surface inside the sub-ducts makes it possible to amplify the effect of the UV-C LEDs with a linear decrease in efficiency at the far ends (data not shown). Sanitation is considered a business topic in the COVID-19 era, having recorded a total turnover of 20 billion euros, for a counter-value of 500,000 employees in terms of workforce. Moreover, commercial and economic growth was followed by the consciousness of the need of low-environmental-impact techniques and technologies. Indeed, many chemical-based sanitation devices produce and release byproducts that are harmful and toxic to the environment. Other systems (i.e., ozonationand UV-based) can generate ozone and mercury emissions. Furthermore, some systems require the replacement of exhausted components, particularly in the case of devices based on sanitation through microorganism retention (i.e., HEPA filters) or UV lamps, that have a shorter lifetime than LEDs. For these reasons, a sanitation system founded on energysaving LED UV-C lamps (90% of the energy converted into UV-C rays) is an eco-friendly, ozone-free and sustainable solution with an extremely low impact on the environment.

In some trains, overcrowded environments in which a great percentage of the air is recycled, the placement of sanitation air systems able to maintain low levels of microorganisms and pollutants is essential. The device tested, thanks to the high efficiency it demonstrated at microbial inactivation, could be very useful in this regard and its use could be proposed in train settings. To the best of our knowledge, no data about the UV-C inactivation of aerosolized SARS-CoV-2 is yet available. However, recent studies demonstrated SARS-CoV-2's susceptibility to UV-C [24, 36] . The results of this study suggest the effectiveness of the CSA system at the inactivation of microorganisms other than those tested with lower inactivation UV doses, such as Coronavirus, included SARS-CoV-2 [24, 37] . Additionally, optimal ventilation in railway vehicles and increasing the number of air exchanges per hour, as well as proper cleaning and maintenance of conditioning systems, may contribute to further reducing the risk of spreading aerodispersed microorganisms, including SARS-CoV-2. 

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The CSA system is a continuously operating air sanitation and purification system that aims at killing airborne microorganisms and reducing potential pollutants in the air (e.g. PM1-10). The CSA system, which was developed for railway applications, was installed outside the passenger compartment, inside the HVAC box, and/or inside the ventilation ducts in an accessible position. The system (international patent application: N.PCT/IB2021/054194) consists of an ionizer, a ISO Coarse 90% self-sanitizing filter [27] , UV-C LEDs, a sensor platform for detecting air quality parameters and an electronic control Unit (ECU). The CSA system (Figure 1 ) is made of a metallic main duct that holds the ionizer and the filter in the first portion. After the filter, the main duct is split into sub-portions that divide the airflow in the sub-conducts. The UV-C LEDs are arranged in these sub-ducts to sanitize the airflow and the internal surface of the filter; moreover, some other LEDs are Acknowledgments: The authors acknowledge A.F. Frigo Clima Impianti Srl, Trenitalia S.p.A. and Hitachi rail STS S.p.A. for the assistance and collaboration provided.

MPA is an employee of and holds shares in the start-up STE-Sanitizing Technologies and Equipments Srl. The company develops air sanitation systems with innovative and eco-sustainable technologies. All the other authors do not have any conflict of interest.