Background
Corona virus disease 2019 (COVID-19) is caused by severe acute respiratory syndrome (SARS)-corona virus (CoV)-2. The first outbreak occurred at the end of 2019, causing symptoms such as fever and pneumonia. In serious cases, the patient might die. As of the early March 2021, the COVID-19 epidemic had appeared in all continents except Antarctica, about 117 million people have been diagnosed worldwide, and the death toll has approached 2.6 million, seriously threatening global public health [
1].
SARS-CoV-2 was first isolated from epithelial cells of the human airway, and was identified by next-generation sequencing technology in January 2020 as a new member of the beta coronaviruses (β-CoVs) [
2]. Coronaviruses are enveloped, single-stranded RNA viruses [
2]. From 2002 to 2003, more than 8000 patients were infected by SARS-CoV, which causes SARS, and the World Health Organization (WHO) finally reported 774 related deaths. Since September 2012, a total of 2494 laboratory-confirmed Middle East respiratory syndrome (MERS)-CoV infected cases have been reported. The WHO has reported 858 MERS-CoV-related deaths [
3,
4]. These emerging infectious diseases with global transmission are caused by β CoVs.
Although coronaviruses cause respiratory tract infections, several studies have shown that the viral RNA of SARS-CoV [
5], MERS-CoV [
6], or SARS-CoV-2 [
7,
8] can be detected in blood plasma. As early as 2003, the WHO noted that blood products could be contaminated with SARS-CoV. Although no cases of SARS-CoV infection caused by blood transfusion have been reported, there is still a theoretical risk of transmitting SARS-CoV or other coronaviruses through blood transfusion [
9]. As more asymptomatic infections are identified among COVID-19 cases [
10], blood safety becomes more important [
11,
12]. In addition, there are currently no specific drugs or vaccines that are effective against SARS-CoV-2. Patient convalescent plasma therapy could be a rapid and effective treatment for this epidemic situation [
13]. However, the critical aspect of this method is to ensure the complete inactivation of SARS-CoV-2 in the plasma from donors. There is an urgent need for a reliable and practical method of plasma SARS-CoV-2 inactivation.
Photochemical treatment methods are used as pathogen inactivation/reduction technologies (PRTs). Photochemical methods to kill viruses are performed by adding methylene blue (MB) into blood products followed by visible light treatment. Methylene blue is a photosensitizer with a maximum absorption peak of 670 nm. It is usually used as an antidote to treat methemoglobinemia and cyanide poisoning caused by nitrite poisoning. The surface of MB carries a positive charge. It can be embedded into DNA or RNA, especially in combination with negatively charged G-C base pairs of viral nucleic acids. Under visible light, MB absorbs light energy, activates it from the ground state to a singlet state, and generates singlet oxygen through electron transfer, which damages and breaks nucleic acids to kill viruses. Viral envelopes and nucleic acids can be targets of MB attack. Alamdari and colleagues used leucomethylene blue, a reduced form of MB, as a therapeutic method for COVID-19 infection [
14]. Furthermore, they used a combination of MB-vitamin C-N-acetyl Cysteine to treat five patients with COVID-19 and four out of five survived [
15]. The possibility of using MB for either the prevention of viral infection or the development of photoactive fabrics has been proposed by Almeida et al. [
16]. Under light, MB can cause nucleic acid strand breaks [
17]. The visible light source can be a halogen lamp, a metal halide lamp, or a fluorescent lamp, with full-band white light. However, because of the low excitation efficiency of MB in full-band white light, this process also generates heat to destroy plasma components. The ‘BX-1 AIDS treatment instrument’, developed by Boxin Biotechnology Development LTD (Beijing, China), uses LED single wavelength light combined with MB and is highly effective at killing various lipid enveloped viruses, such as HIV-1 and other viruses [
18,
19]. As SARS-CoV-2 is a new type of coronavirus, its tolerance to physicochemical conditions is unclear. Therefore, in the present study, the ‘BX-1 AIDS treatment instrument’ was used to study the plasma inactivation of a SARS-CoV-2 isolate from Zhejiang University.
Methods
Cells, instruments, reagents, and viruses
VERO-E6 cells bought from ATCC (Manassas, VA, USA; Cat. (ATCC® CRL-1586™) were stored in the laboratory of Zhejiang University. Dulbecco’s modified Eagle’s medium (DMEM), fetal bovine serum (FBS), penicillin/streptomycin (P/S), and phosphate-buffered saline were bought from GIBCO (Grand Island, NY, USA). MB is a product of Jichuan Pharmaceutical Group Co., Ltd. (Taixin, China). Human plasma was donated by volunteers, and written informed consents were obtained. All experimental operations involving live viruses were carried out in Zhejiang University’s Biosafety Level 3 (BSL-3) Laboratory. The research protocol was approved by the Ethics Committee of the First Affiliated Hospital of Zhejiang University School of Medicine.
Methylene blue-light inactivated virus
To 180 mL of healthy human plasma, 20 mL of live SARS-CoV-2 spike virus was added. Diluted MB was added to 200 mL of the plasma-virus mixture and mixed to a final MB concentration of 1, 2, or 4 μM. The “BX-1 AIDS treatment instrument” was used at room temperature, and illumination was adjusted to 55,000 ± 0.5 million Lux. The plasma samples were irradiated for 0, 2, 5, 10, 20, or 40 mins under light at a single wavelength of 630 nm. About 1 mL of plasma was taken at each time point, diluted 10-fold with DMEM medium containing 2% FBS, and filtered through a 0.45-μm filter (Millipore, Billerica, MA, USA) for virus titer detection. At the same time, a virus control was set (only virus in the plasma, left at room temperature for 40 mins as an untreated control), a control with pure MB was set (virus and 4 μM MB added to the plasma, with no light treatment, and allowed to stand for 40 mins as a control for the effect of MB on the virus), and finally a light-only control was set (only the virus was added to the plasma, and light was used for 40 mins as a control of the effect of light on the virus). This experiment was repeated three times.
Virus titer measurement
After trypsinization of VERO-E6 cells, 1 × 104 cells/well were inoculated into 96-well cell culture plates in 100 μL of culture medium per well. After the cells grew into a single layer in the 96-well plate, the culture medium was discarded and the treated plasma was seeded into the wells. The treated plasma was log-diluted with 2% FBS in DMEM medium from 102–107times. This process was repeated for 4 wells per dilution, 200 μL/well. Normal cell control wells were established (with cells, virus-free). The 96-well plate was placed in an incubator with 5% CO2 at 37 °C. After 3 h of incubation, the supernatant was washed off, and 200 μL /well of 2% FBS DMEM medium was added. Cell lesions were observed every 24 h until 6 d. The TCID50 (median tissue culture infectious dose) was calculated according to the Reed-Muench method. The cell culture supernatant at 6 d of the culture was pipetted, and the viral nucleic acid load was measured. This experiment was repeated three times.
Three generations of blind tests
One milliliter of the test plasma with virus and 1,2, and 4 μM MB was irradiated for 40 min. It was then diluted 10 times with 2% FBS DMEM medium, filtered through a 0.45-μm filter, and added to VERO-E6 cells. After 48 h, 1 mL of the supernatant of the culture was diluted 10 times with 2% FBS DMEM medium, and added to VERO-E6 cells for three passages. These cells were observed for cytopathic effects. For the duration of the 3rd generation of cell blind transmission, the sample was deemed positive (+) if cytopathic lesions appeared at any time, indicating that the virus was not completely inactivated; samples were deemed negative (−) if no cytopathic lesions appeared, indicating that the virus had been completely inactivated. This experiment was repeated three times.
Viral load of culture supernatant measured using quantitative reverse transcription-polymerase chain reaction (qRT-PCR)
Nucleic acid extraction: Using 200 μL of virus culture supernatant, the MVR01 magnetic bead method nucleic acid extraction kit was used (article number: ZM-0044, Shanghai Zhijiang Biotechnology Co., Ltd., Shanghai, China) in an EX2400 automatic nucleic acid extraction instrument (Shanghai Zhijiang Biotechnology Co., Ltd). Virus RNA was extracted, and the elution volume was about 50 μL.
qRT-PCR: A new coronavirus nucleic acid assay kit (Cat. No. Z-RR-0479-02-50, Shanghai Zhijiang Biotechnology Co., Ltd.) was used for qRT-PCR to detect the viral load, following the manufacturer’s instructions. Briefly, the qRT-PCR amplification reaction tube was placed on a LightCycler® 480II (Roche, Basel, Switzerland) qPCR instrument, and FAM and VIC (or TEXAS RED) fluorescence channels were selected for detection. The recommended cycle parameter settings were: 45 °C for 10 min and 95 °C for 15 min; then 45 cycles of 95 °C for 15 s and 60 °C for 60 s; with single-point fluorescence detection at 60 °C. A cycle threshold (CT) value below 35 was considered effective amplification, and a CT value above 35 was considered undetected.
Statistical analysis
The statistical analyzes were performed using SPSS 20.0 (IBM Corp., Armonk, NY USA). Student’s t-test was employed if the measurement data exhibited a normal distribution, and non-parametric test if it did not exhibit a normal distribution. P < 0.05 was considered to indicate statistical significance.
Discussion
The new coronavirus SARS-CoV-2, which appeared in December 2019, spread globally within 3 months and is being monitored closely worldwide. The following are safety considerations for blood transfusions or blood products: (1) Viral RNA in plasma or serum can be detected in patents with COVID-19 2 or 3 d before the onset of symptoms [
8]; (2) most patients, especially young adults who can donate blood, experience milder symptoms than do the elderly; (3) multiple asymptomatic carriers have been found in China and other countries, which increases the possibility of blood donation by COVID-19 or virus carriers [
10]; (4) infection rates of patients in the incubation period are still uncertain, and there is yet no data on viral load in plasma, serum, or lymphocytes during the incubation period. Blood transfusions carry the risk of transmitting SARS-CoV-2, and thus measures to inactivate pathogens in blood products should be explored as soon as possible.
Coronaviruses are enveloped, single-stranded RNA viruses. Previous studies indicated that coronaviruses are generally susceptible to acid, alkaline, and heat [
20]. After the outbreak of SARS and MERS, some studies investigated the potential of PRTs to reduce or completely eliminate the potential risks of coronavirus transmission through blood products or derivatives [
21]. Research on plasma inactivation methods has focused on heat and photochemical treatment methods. (1) Heat method, in general, 30 mins at 60 °C is sufficient to reduce SARS-CoV from cell-free plasma [
22], and 25 mins at 56 °C reduced MERS virus by more than 4 log10 TCID50/mL [
23]. Heating can denature proteins in blood products; therefore, it cannot be used to manufacture plasma-derived products. (2) Photochemical treatment methods. Different wavelengths of light affect the viability of SARS and MERS viruses in the blood. UV light, Amotosalen, or riboflavin can inactivate pathogenic nucleic acids [
22]. Keil et al. performed SARS-CoV-2 inactivation of blood products in standard blood bags using the Riboflavin and the UV methodand the data indicated that the reductions of the viral titres were ≥ 3.40 Logs and ≥ 4.53 Logsin plasma and platelets, respectively [
24], which are on the same order of magnitude as our data. It has been previously reported that MB plus visible light is capable of inactivating coronavirus in plasma [
21,
25] Previously, the prototype ‘plasma virus inactivator’ JY-1 developed by Boxin (Beijing) Biotechnology Development LTD, under the condition of a single-wavelength LED illumination of 40,000 lx, was used for treatment together with 1 μM MB for 30 min [
26,
27]. The new BX-1 ‘AIDS treatment instrument’ used in this study can reduce the titer of new coronavirus SARS-CoV-2 by 4.5 log10 TCID50/mL in 2 mins (Fig.
2), which is a strong advantage for inactivation of viruses in plasma.
MB and LED based BX-1 technology provides a new approach for inactivation of SARS-CoV-2 in plasma, which may be useful for convalescent plasma therapy of critical ill patients with COVID-19. Convalescent plasma therapy is a rapid and effective treatment that has been applied for severe infectious diseases for over 100 years [
13]. In 1890, Emil von Behring from Germany and Saburo Kitari from Japan announced an important discovery: They kept injecting small amounts of non-lethal tetanus into animals, which produced an antitoxin in the blood. This could neutralize the bacillus toxicity of tetanus injected into the body. The serum could also be isolated from animals that have acquired tetanus immunity and injected into other animals to enhance their immunity to tetanus. Emil Behring won the 1901 Nobel Prize in Medicine for his research on diphtheria serum therapy. The earliest application of convalescent plasma therapy allowed humans to overcome diphtheria [
13]. In 2014, during Ebola virus disease outbreaks, the WHO recommended the use of convalescent plasma as an empirical treatment [
28]. Previously, in the clinical treatment of SARS coronavirus, doctors in Hong Kong, Taiwan, and Singapore had shown that convalescent plasma therapy could improve the conditions for critical ill patients with SARS for whom comprehensive treatment had not been effective [
29]. Given this long history of serum-based treatment in the modern era, and its established safety and efficacy, convalescent plasma transfusion should be used to treat patients with COVID-19 [
30].
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