Hepatitis B virus replication is upregulated in proliferated peripheral blood lymphocytes
- Authors:
- Published online on: March 3, 2016 https://doi.org/10.3892/mmr.2016.4973
- Pages: 3581-3587
Abstract
Introduction
The hepatitis B virus (HBV) is a hepatotropic virus that predominantly infects and replicates in hepatocytes. However, previous studies have demonstrated that HBV is present in peripheral blood mononuclear cells (PBMCs) (1–3), which are considered to be a reservoir contributing to chronic HBV infection (4,5). The risk for HBV transmission by infected PBMCs has also been demonstrated. For example, HBV-infected mothers may transmit the HBV infection to newborns during the perinatal period (6) and livers from donors who were hepatitis B surface antigen (HBsAg)-negative, but hepatitis B core antibody (anti-HBc)-positive may transmit the HBV infection to recipients following liver transplantation (7). HBV infection may occur as a result of blood transfusion and hemodialysis using blood that is contaminated with HBV (8,9), in addition to immunosuppressant therapy-induced hepatitis B reactivation (10). All of these transmissions are closely associated with HBV infection in PBMCs. Thus, the detection of HBV infection in PBMCs is considered to be clinically significant.
HBV replication in PBMCs is at a low level (5) and current methods, including polymerase chain reaction (PCR), are not sensitive enough to detect the minute quantities of viral products (11). It is particularly difficult to detect covalently closed circular DNA (cccDNA), which functions as a template for transcription and a marker for HBV replication. Currently, it is unclear whether HBV replicates in PBMCs (12–16) and whether the virus readily infects PBMCs (17) due to a lack of cccDNA detection methods. Thus, further studies are required to develop more sensitive methods to detect small quantities of viral products in PBMCs, and eventually determine whether HBV infects and replicates in PBMCs.
El-Awady et al (18) demonstrated that hepatitis C virus (HCV) infects PBMCs, and that phytohemagglutinin (PHA)-induced proliferation of PBMCs increases HCV replication. Furthermore, it was reported that woodchuck HBV replication is upregulated in PBMCs with mitogen stimulation (19–21). Our previous studies also suggested that HBV gene expression is increased following expansion of bone marrow hematopoietic stem cells isolated from chronic hepatitis B patients, via a non-specific mitogen stimulus (22,23). Based on these findings, the aim of the present study was to establish a method to increase HBV replication in PBMCs via mitogen stimulation in vitro. It was demonstrated that the detection of HBV DNA and HBsAg in PBMCs is markedly improved following in vitro mitogen treatment. Thus, this method may be used for evaluating antiviral treatment responses, organ transplantation screening and for the diagnosis of occult hepatitis B.
Materials and methods
Preparation of PBMCs
PBMCs were obtained from six healthy volunteers (two males and four females; age, 32.3±10.7 years). All participants were negative for hepatitis A, C, D, E, and HIV antibodies, and negative for hepatitis B serological markers and HBV DNA. Participants exhibited normal alanine transaminase levels and were not vaccinated against HBV. The present study was approved by the Ethics Committee of the Institutional Review Board of The First Affiliated Hospital of Harbin Medical University (Harbin, China). The experimental protocol was established, according to the ethical guidelines of the Helsinki Declaration. Written informed consent was obtained from individual participants.
PBMCs were separated from 20 ml ethylenediaminetetraacetic acid (EDTA)-treated blood by Ficoll density gradient centrifugation (Tianjin Haoyang Biological Technology Co., Ltd., Tianjin, China) at 1,000 × g for 20 min at 20°C, resulting in a yield of ~6.32±2.11×106 cells/ml blood. The cells were washed three times with phosphate-buffered saline (PBS) prior to seeding into culture wells.
In vitro infection of PBMCs with HBV and stimulation with mitogen
PBMCs were seeded in 24-well plates at a final concentration of 105 cells/ml with 0.95 ml RPMI-1640 (Hyclone; GE Healthcare Life Sciences, Logan, UT, USA) and 0.05 ml HBV-positive serum (HBV DNA 107 IU/ml, genotype C) filtered through a Millex-GP 0.22-μm filter (EMD Millipore, Billerica, MA, USA). The culture medium was supplemented with 10% fetal calf serum (Hyclone; GE Healthcare Life Sciences). Cells were stimulated by PHA (Sigma-Aldrich, St. Louis, MO, USA) with a final concentration of 5 μg/ml and interleukin (IL)-2 (Sigma-Aldrich) with a final concentration of 20 U/ml. Plates were incubated at 37°C and 5% CO2 for 12 days. This experiment was repeated six times with PBMCs. Three wells of cells were harvested at day 0, 1, 6 and 12. The number of viable cells was estimated by 0.04% Trypan Blue exclusion (Sigma-Aldrich). A mean of the cell numbers of three wells was used for calculation at each time-point. Cells were stored at −80°C for further analysis.
Quantification of HBV DNA within PBMCs
DNA was isolated from 1 ml cell suspension using the Cobas AmpliPrep automated extractor (Roche Diagnostics GmbH, Mannheim, Germany), according to the manufacturer's protocols. HBV DNA was quantitatively detected from the isolated DNA prep using a Cobas TaqMan 48 analyzer (version 3.3; Roche Diagnostics GmbH). Data were analyzed with Amplilink software (Roche Diagnostics GmbH). Cobas AmpliPrep/Cobas TaqMan HBV test kit (version 2.0) was used to measure the lower limit of detection with primers located in the pre-C/C highly conserved region (Table I) (11). The mean of the copy numbers from three detection wells indicated that 20 IU/ml was the lower limit of detection.
Detection of HBV RNA isolated from PBMCs by reverse transcription (RT)-PCR
PBMCs that were cultured as described above were harvested at day 0, 1, 6 and 12, with a cell density of 1.0×105, 1.8×105, 5.8×105, and 1.1×106 cells/ml, respectively. PBMCs were washed three times with PBS. Total cellular RNA was extracted using 1ml TRIzol reagent (Invitrogen; Thermo Fisher Scientific, Inc., Waltham, MA, USA), 200 μl chloroform (Tianjin Haoyang Biological Technology Co., Ltd.), 0.5 ml isopropyl alcohol and 1 ml ethanol (75%; both Tianjin Fuyu Chemical Co., Tianjin, China). Complementary DNA (cDNA) was synthesized using Qiagen OneStep RT-PCR kit (Qiagen GmbH, Hilden, Germany). The cDNA primer sequence within the S region was used as previously described (Table I; Boster Biological Technology, Ltd., Wuhan, China) (24). Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) served as an internal reference (Table I; Boster Biological Technology, Ltd.). RT was conducted on a Mastercycler (Eppendorf AG Hamburg, Germany) at 60°C for 1 min, 42°C for 10 min, 50°C for 30 min, and 95°C for 15 min. The cDNA was amplified as follows: 40 Cycles of 94°C for 30 sec, 56°C for 30 sec, 72°C for 1 min; and 72°C for 10 min. PCR products (length, 452 bp) were stored at 4°C prior to visualization via 1% agarose electrophoresis. Electrophoresis was performed using 10 μl cDNA, 6 μl DNA marker (D2000; Tiangen Biochemical Technology, Co., Ltd., Tiangen, China) and loading buffer (Takara Biotechnology, Co., Ltd., Dalian, China) at 110 V for 30 min. Images were captured using a GL-3120 Compact Desktop UV Transmissometer (Korea Biotech Co., Ltd., Seoul, Korea) software.
In situ hybridization detection of HBV DNA in PBMCs
The HBV-inoculated PBMCs that were cultured for 12 days, were harvested and washed three times with PBS. Hepatitis B virus nucleic acid in situ hybridization kit (Tianjin Haoyang Biological Technology Co., Ltd.) was used to detect HBV DNA on PBMC slides, according to the manufacturer's protocols. Hybridization was conducted in a hybrid oven (Abbott Stat Spin®; Abbott Laboratories, Chicago, IL, USA). The hybridization signal was generated with fluorescein isothiocyanate (FITC) fluorescent dye. Hybridization solution containing no specific probe served as a negative control, whereas HepG2.2.15 cells, which were gifted from Professor Hong Ren (Chongqing Medical University, Yuzhong, China), served as a positive control. The HBV probe sequence (Tianjin Haoyang Biological Technology Co., Ltd.) was derived from a highly conserved region that is located in the overlapped P and pre-C open reading frame (Table I). Slides were examined under a Nikon Eclipse TS100 80i microscope (Nikon Corporation, Tokyo, Japan) and Olympus BX53 fluorescence microscope (Olympus Corporation, Tokyo, Japan).
Quantification of HBsAg in PBMCs
The same PBMCs from the three wells described above were harvested at day 0, 1, 6 and 12 and washed three times with PBS. The cells were lysed with 10 mM Tris-Hcl (Sangon Biotech Co., Ltd., Shanghai, China) and 1% Triton X-100 (Solarbio Science & Technology Co., Ltd., Beijing, China) and intracellular HBsAg was quantified using an Architect HBsAg assay (Abbott Laboratories), according to the manufacturer's protocols. The lowest limit of detection was 0.00–0.05 IU/ml.
Immunohistochemistry of HBsAg in PBMCs
At day 12, the cultured PBMCs were collected, washed three times with PBS, and smeared onto slides. Immunostaining of HBsAg was performed using an Immunostain SP kit (Beijing Zhongshan Jingqiao Biotechnology, Co., Ltd., Beijing, China). A mouse monoclonal antibody against HBsAg (1:50; ZM-0122; Beijing Zhongshan Jingqiao Biotechnology, Co., Ltd.) was used as the primary antibody, whereas a goat anti-mouse IgG without dilution (ZDR-5117; Beijing Zhongshan Jingqiao Biotechnology, Co., Ltd.) was used as the secondary antibody. The reaction was subsequently visualized using 3,3′-diaminobenzidine (Beijing Zhongshan Jingqiao Biotechnology, Co., Ltd.). HepG2.2.15 cells served as a positive control.
Statistical analysis
All statistical analyses was performed using SAS 9.2 statistical analysis software (SAS Institute, Cary, NC, USA). Data are expressed as the mean ± standard error of the mean. The mixed-effects model was used to analyze the changes in cell proliferation and viral replication with culture time. The same analysis was also used to analyze the association between cellular proliferation and viral replication subsequent to adjusting for the time factor. P<0.05 was considered to indicate a statistically significant difference.
Results
HBV DNA was detected in PBMCs by in situ hybridization
The PBMCs inoculated with HBV and cultured for 12 days demonstrated a positive signal following hybridization with an FITC-labeled probe. A similar fluorescence signal was also detected in HepG2.2.15 cells. No fluorescence signal was observed in the PBMCs that were hybridized without the specific probe (Fig. 1).
HBsAg was detected in PBMCs by immunohistochemistry
The PBMCs were stained with the HBsAg-specific antibody. The immunohistochemistry staining demonstrated the presence of HBsAg in the cytoplasm of PBMCs that were harvested at day 12. The same staining pattern was detected in HepG2.215 cells, however, it was absent in the negative control cells (Fig. 2).
Levels of HBV DNA were increased in proliferated PBMCs induced by PHA and IL-2 in vitro
HBV DNA levels in the PBMC suspension isolated from three of six healthy volunteers were increased with the proliferation of PBMCs induced by PHA and IL-2. The mean PBMC number isolated from the three cases at day 12 was expanded by 13.61 times compared with the initially seeded density (P<0.01). The mean load of HBV DNA at day 12 was increased by 2.98 times from the initial level (P<0.05). However, the correlation between the proliferation of PBMCs and the increase in viral replication was not identified as statistically significant (P>0.05; Fig. 3).
HBV RNA was detected in PBMCs by RT-PCR
To investigate whether HBV genes are transcribed in the inoculated PBMCs, HBV RNA transcripts were analyzed by RT-PCR. No PCR amplicon was detected in PBMCs harvested until days 6 and 12. The HBV RNA level was higher on day 12 than on day 6, and the increase of HBV RNA transcription was associated with an increase in HBV DNA level. Negative controls replacing cDNA with PBS, and the PCR mix with PBS, did not demonstrate any effect. GAPDH served as an internal RT-PCR control (Fig. 4).
HBsAg levels increase with PBMC amplification
Intracellular HBsAg was quantitatively determined and increased HBV DNA replication was only detected in one of the three PBMC cultures. Furthermore, the HBsAg level increased as the proliferation of PBMCs increased. Intracellular HBsAg was 0.043±0.0047 IU/ml at day 0 and was increased to 0.48±0.12 IU/ml (Fig. 5) at day 12.
Discussion
PBMCs consist of various types of immune cell, including T and B lymphocytes, macrophages and natural killer cells. These cells circulate in the blood to fight infection and travel to different organs to actively engage the immune response. It has been suggested that PBMCs may be infected with HBV. HBV-infected PBMCs compromise the immune response of the host and potentially facilitate the persistence of HBV infection (25,26). However, there is no robust method for detecting HBV infection and replication in PBMCs, which may be due to the HBV infection presenting at a low level in PBMCs. The proliferation of PBMCs is promoted by certain non-specific mitogens, which may assist effective detection of HBV replication. In the present study, PBMCs were inoculated with HBV in vitro, then stimulated with PHA and IL-2, and cultured for 12 days. The levels of HBV DNA and HBsAg were quantified at different time-points. HBV DNA was detected in PBMC suspensions that were isolated from three of six donors, and it was observed that the HBV DNA levels increased in a time-dependent manner. In addition, intracellular HBsAg was detected only in one group of cultured PBMCs that also demonstrated the most marked increase in HBV DNA levels. These findings suggest that HBV infects PBMCs, and the infected PBMCs induce HBV replication. Furthermore HBV DNA replication was increased with active cell proliferation. Similar observations were reported by Budkowska et al (17), no detectable cccDNA was observed when PBMCs were co-cultured with a HBV binding factor-digested virus that modified the structure of the envelope proteins and enhanced the capacity of HBV to bind and enter into PBMCs. However, the HBV DNA signal did not decline over time in the cell culture (if there is no virus replication in PBMCs, a progressive reduction of HBV products would be expected). Furthermore, additional evidence supporting HBV replication was generated in the present study; HBV nucleic acid, HBsAg and HBV RNA were detected in PBMCs by in situ hybridization, immunohistochemical staining and RT-RCR, respectively.
Various methodological approaches have previously been used to investigate HBV infection in PBMCs. The present study optimized experimental procedures and our findings demonstrated that cell number influences HBV replication in PBMCs. Once the cell number underwent proliferation under stimulation, the HBV DNA level became increasingly detectable, suggesting that the HBV DNA did replicate, otherwise HBV DNA copies would have been diluted out due to multiple cycles of cell division. Previous studies cultured PBMCs for 7 days (16,25–27). However, the present study prolonged PBMC culture to the logarithmic phase to ensure maximum proliferation was reached. Secondly, to ascertain HBV replication in PBMCs, the current study investigated the kinetics of HBV DNA level over time, which was different from the previous studies where the detection of HBV infection was performed at a single time-point (16,22). The present study improved the procedures for detecting particularly low levels of viral replication.
Southern blotting is the classic method for detecting cccDNA in infected liver tissues, it is specific and reliable, however, it is not sensitive enough to detect low levels of cccDNA (28), and, thus, is not suitable for detecting cccDNA in PBMCs. The results from the present study indicated for the first time, to the best of our knowledge, that HBV was present in PBMCs and that it replicated at particularly low levels. This was supported by the evidence of detectable HBV RNA, which had to be transcribed from the cccDNA template. The results of the current study suggest that mitogen stimulation of infected PBMCs may upregulate viral replication and increase detectability of HBV infection that otherwise may be missed due to the low level of HBV DNA in PBMCs. This procedure may also improve diagnosis of the HBV occult infection, serve as an effective screening tool for organ transplant donors, and assess the efficacy of antiviral therapy. Limitations of the present study were that the PBMCs were provided by individual donors, which may have resulted in certain variations and that the efficiency of HBV inoculation in PBMCs may have affected detection and replication of the HBV infection.
HBV reactivation in PBMCs has been reported following liver transplantation, immunosuppression treatment and chemotherapy (10,29,30). Results from the present study support the hypothesis that HBV may be harbored in PBMCs without being recognized as targets by immune effectors (31,32). Once division of PBMCs is activated by mitogen stimulation, the resulting proliferative PBMCs may facilitate productive virus replication and lead to the reactivation of latent infection to a relatively high level for detection (26). However, further investigations are required to validate the findings of the present study.
In conclusion, the current study demonstrated that HBV infects PBMCs, and HBV replication is upregulated in mitogen-stimulated PBMCs. As HBV DNA in extrahepatic tissues is usually at a particularly low level, ex vivo stimulation of PBMCs using the conditions established in the present study may improve detection of HBV occult infection, and enable more effective treatment.
Acknowledgments
The present study was supported by the National Key Technologies Research and Development Program of China (grant nos. 2008ZX10002-006 and 2012ZX10002007) and the National Natural Science Foundation of China (grant no. 30571638).
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