Abstract
This study investigated the antiviral activities of Radix Isatidis polysaccharide (RIP) against type II herpes simplex virus (HSV-2) in vitro. RIP was prepared from the Radix Isatidis root. The toxicity of RIP on Vero cells was detected. The direct killing effect of RIP on HSV-2, inhibitory effect of RIP on HSV-2 replication and inhibitory effect of RIP on HSV-2 adsorption were determined. Results showed that, RIP in concentration range of 25-800 mg/L had no toxic effect on Vero cells. RIP with different concentrations could not directly inactivate the HSV-2. The effective rates on inhibition of HSV-2 replication and adsorption in 800 mg/L RIP group were 71.57% and 48.37%, respectively, which were the highest among different groups. In conclusion, RIP has the antiviral effect against HSV-2 in vitro. This effect mainly occurs in inhibiting the virus duplication and adsorption.
Keywords: Radix Isatidis; polysaccharide; HSV-2
1 Introduction
Type II herpes simplex virus (HSV-2) is a virus which majorly causes the genital herpes. HSV-2 infection is one of the major problems that affect the health of adults, especially in patients with immune impairment (Schiffer & Corey, 2013). At present, the antiviral drug acyclovir is often clinically used to treat the HSV-2 infection. This drug exerts the antiviral action mainly by interfering with viral DNA replication. However, as the virus is easy to produce variation, the drug resistance still exists, so the treat outcome is not very satisfactory (Bacon et al., 2003). Therefore, it is urgent to develop a new mode of anti-HSV-2 drugs. In recent years, drug researchers have paid more and more attention to screening antiviral drugs from natural products. Isatidis Radix is a traditional herb in China. It is firstly collected in Shennong's Classic of Materia Medica. In traditional Chinese medicine (TCM), Isatidis Radix is bitter and cold, and has the efficacy of clearing away heat and toxicity and relieving sore throat. It is clinically used in treating viral and bacterial infection diseases (Ke et al., 2012). Polysaccharide is the main chemical component of Radix Isatidis. It is often obtained by water extraction from the root of Radix Isatidis. Many studies have shown that, Radix Isatidis polysaccharide (RIP) has the antioxidant and anti-inflammatory activities (Du et al., 2013), and can resist the viruses and enhance the body immunity (Zhao et al., 2008; Fang et al., 2009). Until now, the effect of RIP on HSV-2 is less reported. If it is confirm that RIP has antiviral activities against HSV-2, this will further broaden the range of therapeutic medicine for HSV-2 related diseases and the application range of RIP. In this study, it was the first time to investigate the antiviral activities of RIP against HSV-2. The objective of this study was to provide a basis for further studying the in vivo anti-HSV-2 activity of RIP and broadening the application scope of RIP.
2 Materials and methods
2.1 Preparation of RIP
Radix Isatidis root (500 g) was decocted (micro boiling) with 3000 mL distilled water for 4 h. After heat filtering, the filter residue was decocted with 2000 mL of distilled water for 2 h. The filtrates of two decoctions were merged, and were concentrated to volume of 200 mL. 800 mL anhydrous ethanol was added, and the final alcohol concentration was adjusted to 80%. After standing overnight, the supernatant was discarded, and the precipitate was dissolved in 100 mL of distilled water, and 400 mL anhydrous ethanol was added. The final alcohol concentration was adjusted to 80%. After standing overnight, the supernatant was discarded, and the precipitate was collected. After freeze-drying, and the crude polysaccharide product was obtained. After deproteinization using Sevage method (Yanhua et al., 2014), the refined RIP was obtained. The sulfuric acid-phenol method showed the content of polysaccharide was 80%.
2.2 Cell culture
Vero cells were cultured with Dulbecco's Modified Eagle's medium (DMEM) containing mL/L fetal bovine serum (FBS), 100 U/mL penicillin and 100 μg/mL streptomycin at condition of 37 °C and 5% CO2. All the cell culture reagents were provided by Sigma-Aldrich Corp., MO (USA).
2.3 Determination of virus virulence
HSV-2 (333 strains) was provided by Institute of Virology, Wuhan University (Wuhan, China). HSV-2 stock solution was diluted into 8 dilutions (10-1, 10-2, 10-3, 10-4, 10-5, 10-6, 10-7, 10-8) using cell maintenance medium containing 2% FBS. The virus fluid with each dilution was inoculated to the 96-well culture plate of monolayer Vero cells, 4 repeated wells for each dilution, followed by culture at 37 °C with 5% CO2. The normal Vero cells were set as control. The cytopathy was observed under the inverted microscope. Two fields of vision were selected from each well using the eyepiece micrometer, and 100 squares of each field of vision were selected to calculate the percentage of normal and abnormal cells. The 50% tissue culture infection dose (TCID50) was determined using the Reed-Muench method (Gustafsson et al., 2012).
2.4 Determination of toxicity of RIP on Vero cells
Vero cells were digested with trypsin, and the cell suspension (1×106 cell/mL) was prepared. The cell suspension was seeded into 96-well culture plates, 200 μL in each well. After culture for 24 h, RIP was added to the well. Based on the suitable dose range obtained in preliminary experiments, the concentration of RIP was set as 25, 50, 100, 200, 400, 800 mg/L, 6 wells for each concentration. The continued culture was performed for 48 h at 37 °C with 5% CO2 and saturated humidity. At 4 h before the end of culture, 20 μL of methylthiazolyldiphenyl-tetrazolium bromide (MTT) was added to each well. At the end of culture, the supernatant was discarded and 200 μL of dimethyl sulphoxide was added to each well, followed by oscillation for 5 min. The optical density (OD) of each well was measured by the microplate reader (wavelength 570 nm). The higher OD value represented the higher cell activity.
2.5 Determination of direct killing effect of RIP on HSV-2
RIP with different concentration (25, 50, 100, 200, 400, 800 mg/L) was mixed with the same amount of 100TCID50 HSV-2 fluid, followed by standing at 37 °C for 4 h. The incubation fluid was added to the monolayer of Vero cells, 200 μL for each well, followed by standing at 37 °C for 1.5 h. The supernatant liquid was changed by 200 μL of 2% DMEM, followed by continued culture for 72 h. The cytopathic effect (CPE) was observed under inverted microscope, and the results were recorded as follows: 0% CPE: -; 1-25%: +; 25-50%: ++; 50-75%: +++; 75-100%: ++++. At the same time, the virus group and normal cell group were set, 6 wells for each group. The OD value of each well was measured by MTT method.
2.6 Determination of inhibitory effect of RIP on HSV-2 replication
100TCID50 HSV-2 fluid was inoculated into monolayer of Vero cells, 100 μL for each well, followed by adsorption at 37 °C for 2 h. The virus fluid was discarded, and the 2% DMEM containing RIP with different concentration (25, 50, 100, 200, 400, 800 mg/L) was added, followed by continued culture for 72 h. The CPE was observed under inverted microscope, and the results were recorded. At the same time, the virus group and normal cell group were set, 6 wells for each group. The OD value of each well was measured by MTT method. The antiviral effective rate of RIP was calculated as follows: effective rate (%) = (average ODRIP group- average ODvirus group) / average ODvirus group × 100%.
2.7 Determination of inhibitory effect of RIP on HSV-2 adsorption
RIP with different concentration (25, 50, 100, 200, 400, 800 mg/L) was mixed with the same amount of 100TCID50 HSV-2 virus, followed by direct inoculating into monolayer of Vero cells, 200 μL of mixture for each well, followed by adsorption at 37 °C of 2 h. The supernatant was removed, and the 2% DMEM was added, 200 μL for each well, followed by continued culture for 72 h. The CPE was observed under inverted microscope, and the results were recorded. At the same time, the virus group and normal cell group were set, 6 wells for each group. The OD value of each well was measured by MTT method. The antiviral effective rate of RIP was calculated.
2.8 Statistical analysis
All statistical analysis was carried out using SPSS20.0 software (SPSS Inc., Chicago, IL, USA). The data were presented as mean ± SD, and were compared using y one-way ANOVA with SNK-q test. P < 0.05 was considered as statistically significant.
3 Results
3.1 Virus virulence test result
The test of Reed-Muench method showed that, the TCID50 of the virus was 10-5. The virus concentration used in this study was 100TCID50.
3.2 Toxicity of RIP on Vero cells
Microscopy showed that, the morphology of Vero cells treated by RIP presented a tight and orderly arrangement, without shedding, fusion or round retraction, which was not significantly different from the morphology of normal cells. At the same time, MTT test showed that, there was no significant difference in cell proliferation between each concentration of RIP and normal cells (P > 0.05). This indicated that, RIP in the concentration range of 25-800 mg/L had no toxic effect on Vero cells (Table 1).
3.3 Direct killing effect of RIP on HSV-2
The CPE of HSV-2 infection of Vero cells was characterized by swelling, rounding, intercellular fusion, abscission and fragmentation. The typical CPE caused HSV-2 infection appeared in RIP group with different concentrations. MTT showed that, the cell proliferation activity (OD570nm) of virus group was significantly lower than that in normal cell group (P < 0.05). The OD570nm in each RIP group was also significantly lower than that in normal cell group (P < 0.05), with no significant difference with the virus group (P > 0.05). This indicated that, the RIP with different concentrations could not directly inactivate the HSV-2 (Table 2).
3.4 Inhibitory effect of RIP on HSV-2 replication
Compared with the normal cell group, the virus group showed typical CPE features including swelling, rounding, intercellular fusion, abscission and fragmentation, and the cell proliferation activity (OD570nm) decreased significantly (P < 0.05). Compared with virus group, the typical CPE features in RIP group with concentrations of 200, 400 and 800 mg/L were reduced, and the cell proliferation activity (OD570nm) was decreased significantly, respectively (P < 0.05). The effective rate on inhibition of HSV-2 replication in 800 mg/L RIP group was 71.57%, which was the highest (Table 3).
3.5 Inhibitory effect of RIP on HSV-2 adsorption
Compared with the normal cell group, the virus group also showed typical CPE features, and the cell proliferation activity (OD570nm) decreased significantly (P < 0.05). Compared with virus group, the typical CPE features in RIP group with concentrations of 400 and 800 mg/L were reduced, and the cell proliferation activity (OD570nm) was decreased significantly, respectively (P < 0.05). The effective rate on inhibition of HSV-2 adsorption in 800 mg/L RIP group was 48.37%, which was the highest (Table 4).
4 Discussion
HSV-2 is a common human infectious disease virus. It can cause herpes simplex, genital herpes, encephalitis, keratitis, visceral infection and so on. In addition, HSV-2 is associated with cervical cancer (Cao et al., 2014). At present, there are more than 50 kinds of medicine for resisting the herpes virus, but only a few drugs including acyclovir are recognized effective and applied in clinic for systemic infection. The targets of the vast majority of antiviral drug are DNA synthetases. The virus resistant to one drug often show cross resistance to other drugs (Tchesnokov et al., 2006). In recent years, in the process of seeking effective antiviral drugs, a variety of natural products are discovered, which have inhibitory effect on virus (Lin et al., 2014).
Many Chinese herbal medicines have the function of enhancing immunity and inhibiting and killing pathogenic microorganisms. These medicines have the characteristic of low toxic effect, low residue, safety and high efficiency. They have always been the focus of new drug research and development (Yang et al., 2008). As the antipyretic and detoxification drug, Radix Isatidis can be directly act with the immune organs, immune cells and the secreted antibodies, cytokines or the central nervous system. It can modulate the immune system, and stimulate the antibacterial, antiviral and antioxidant ability of body through improving the immune function (Kong et al., 2008; Fang et al., 2009). In TCM, Radix Isatidis is one of antiviral medicines. RIP is the main active component of Radix Isatidis, and has many biological activities such as immunoregulation (Zhao et al., 2008), anti-inflammation (Du et al., 2013) and liver protection (He et al., 2011). In recent years, the antiviral effect of RIP has obtained more and more attention. Chen et al. (2006) has isolated an antiviral polysaccharide with relatively uniform molecular weight distribution from Radix Isatidis. They find that, the polysaccharide can not only act directly on the virus, but also promote the generation of anti-influenza virus IgG antibodies. Therefore, the polysaccharide can be used as adjuvant for antiviral vaccines. In addition, Zhao et al. (2008) have used RIP solution to intraperitoneally inject the modeled mice infected with influenza virus. The mouse survival time and lung index are observed, and the changes of serum antiviral IgG level and spleen cell IFN-γ level are determined. Results find that, RIP can promote nonspecific immunity and enhance humoral immune function. In addition, it can participate in the regulation of cellular immune function, thereby enhancing the ability of mice to resist influenza virus infection.
This study has investigated the antiviral activities of RIP against HSV-2 in vitro. Results indicated that, RIP in the concentration range of 25-800 mg/L had no toxic effect on Vero cells. This indicates that, RIP is the safe drug to the cells. MTT assay showed that, the RIP with different concentrations could not directly inactivate the HSV-2, but could inhibit the replication and adsorption of HSV-2. This indicates that, PSP has significant anti-HSV-2 effects in vitro. This effect mainly occurs in inhibiting the virus duplication and adsorption, which is obviously different from acyclovir, so it is difficult to produce drug resistance. RIP is a natural compound, and has the characteristics of non-toxicity and high efficiency. Moreover, it has both antiviral and immunomodulatory effects. This is also an advantage that synthetic drugs do not have. Therefore, RIP has the prospect of developing new antiviral drugs.
5 Conclusions
RIP has the antiviral effect against HSV-2 in vitro. This effect mainly occurs in inhibiting the virus duplication and adsorption. However, the exact mechanism on RIP affecting the replication cycle of viruses in host cells remains to be further studied.
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Practical Application: Radix Isatidis polysaccharide may be applied to treating type II herpes simplex virus related diseases.
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Publication Dates
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Publication in this collection
22 Mar 2018 -
Date of issue
Dec 2018
History
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Received
06 June 2017 -
Accepted
10 Dec 2017