Tly, ISG15 was demonstrated to play an anti-DENV function via protein ISGylation. ISG12b2 was identified as a novel inner mitochondrial membrane ISG that regulates mitochondria-mediated apoptosis during DENV infection [22,23]. In our current study, we report that the expression of ISG BST2 (bone marrow stromal cell antigen 2), also known as CD317, HM1.24 or tetherin [24?26], plays a role in inhibiting DENVE production.Materials and Methods Plasmid construction and establishment of cell linesPlasmid pcDNA5/FRT/BST2 was constructed as described previously [22]. To construct plasmid pcDNA5/FRT/BST2CV5, BST2 cDNA (Gene ID: 684) was amplified from pcDNA5/FRT/BST2 with a pair of primers (Forward: 59-GAGCTTAAGATGGCATCTACTTCGTATGACTA-39. Reverse: 59-CACGCGGCCGCCCTGCAGCAGAGCGCTGAGGCCC-39). The PCR product was digested with Afl II and Not I (New England Biolabs, Ipswich, MA, USA), and ligated with vector fragment recovered from Afl II and Not I digested pcDNA5/FRT/Viperin-CV5 [27]. To establish stable Huh7 cell lines that express BST2 (Huh7-BST2) and carboxyl-terminally V5 tagged BST2 (Huh7-BST5CV5), Huh7 cells (Institute of Cytology, Chinese Academy of Sciences, Shanghai, China) were transfected with plasmidTetherin Inhibits DENV SecretionpCDNA5/FRT/BST2CV5 or pCDNA5/FRT/BST2CV5 and pcDNA3 at a molar ratio of 9 to 1 and cultured with complete DMEM containing 250 mg/ml G418. G418-resistant cell clones that express BST2 or BST2CV5 were identified by detection of the desired proteins in cell lysates by western blot.Infectious foci countCells were seeded into 24-well plate at a density of 26105/well (100 confluence) over night. Cells were infected with DENV at different MOI 18297096 in replicates of six for 1 hour, and culture media were removed and replaced with media containing 0.5 methocellulose prevent cell-free virus infection. Two days after infection, cells were fixed and infected cell foci were revealed by In-Cell Western assay or indirect immunofluorescence. Quantitative analyses of 100 foci from each cell line were performed to reveal the average number of DENV-positive cells per focus. The experiment was performed in 3 replicates to generate statistically significant data.Cell culture and virus infectionA cell-based flavivirus immunodetection (CFI) assay was used to determine the in vitro anti-dengue activity of BST2. Briefly, 26104 of parent Huh7, Huh7-BST2 or Huh7-BST2CV5 cells were seeded in 96-well plate for overnight before they were infected with DENV (serotype II, TSV01 strain) at the given multiplicity of infection (MOI) for 1 h [28]. Cells were incubated in complete Dulbecco’s modified minimal essential Ises a possibility that the spinal receptors for bombesin-related peptides may medium (DMEM, Invitrogen, Carlsbad, CA) for 2 days.RNA quantification by qRT-PCRCellular RNA or viral RNA in culture medium were extracted using TRIzol Reagent (Invitrogen) or QIAamp viral RNA minikit (Qiagen, Valencia, CA) and reverse transcribed using Title Loaded From File SuperScript III (Invitrogen). Quantitative PCR (qPCR) reaction was performed on the ABI 7500 thermocycler 1379592 (Applied Biosystems, Foster City, CA). The probe for DENV was 6-carboxyfluorescein [FAM]-59-AGCATCATTCCAGGCAC-39-MGBNFQ (molecular-groove binding nonfluorescence quencher; Applied Biosystems), forward primer 59-GARAGACCA GAGATCCTGCTGTCT-39 and reverse primer 59ACCATTCCATTTTCTGGCGTT-39 (SBS Genetech, Beijing, China). The standard curve was generated using serial 10-fold dilutions of in vitro transcribed full-length DENV RNA (TSV01 strain). The housekeeping gene b-actin was used as cont.Tly, ISG15 was demonstrated to play an anti-DENV function via protein ISGylation. ISG12b2 was identified as a novel inner mitochondrial membrane ISG that regulates mitochondria-mediated apoptosis during DENV infection [22,23]. In our current study, we report that the expression of ISG BST2 (bone marrow stromal cell antigen 2), also known as CD317, HM1.24 or tetherin [24?26], plays a role in inhibiting DENVE production.Materials and Methods Plasmid construction and establishment of cell linesPlasmid pcDNA5/FRT/BST2 was constructed as described previously [22]. To construct plasmid pcDNA5/FRT/BST2CV5, BST2 cDNA (Gene ID: 684) was amplified from pcDNA5/FRT/BST2 with a pair of primers (Forward: 59-GAGCTTAAGATGGCATCTACTTCGTATGACTA-39. Reverse: 59-CACGCGGCCGCCCTGCAGCAGAGCGCTGAGGCCC-39). The PCR product was digested with Afl II and Not I (New England Biolabs, Ipswich, MA, USA), and ligated with vector fragment recovered from Afl II and Not I digested pcDNA5/FRT/Viperin-CV5 [27]. To establish stable Huh7 cell lines that express BST2 (Huh7-BST2) and carboxyl-terminally V5 tagged BST2 (Huh7-BST5CV5), Huh7 cells (Institute of Cytology, Chinese Academy of Sciences, Shanghai, China) were transfected with plasmidTetherin Inhibits DENV SecretionpCDNA5/FRT/BST2CV5 or pCDNA5/FRT/BST2CV5 and pcDNA3 at a molar ratio of 9 to 1 and cultured with complete DMEM containing 250 mg/ml G418. G418-resistant cell clones that express BST2 or BST2CV5 were identified by detection of the desired proteins in cell lysates by western blot.Infectious foci countCells were seeded into 24-well plate at a density of 26105/well (100 confluence) over night. Cells were infected with DENV at different MOI 18297096 in replicates of six for 1 hour, and culture media were removed and replaced with media containing 0.5 methocellulose prevent cell-free virus infection. Two days after infection, cells were fixed and infected cell foci were revealed by In-Cell Western assay or indirect immunofluorescence. Quantitative analyses of 100 foci from each cell line were performed to reveal the average number of DENV-positive cells per focus. The experiment was performed in 3 replicates to generate statistically significant data.Cell culture and virus infectionA cell-based flavivirus immunodetection (CFI) assay was used to determine the in vitro anti-dengue activity of BST2. Briefly, 26104 of parent Huh7, Huh7-BST2 or Huh7-BST2CV5 cells were seeded in 96-well plate for overnight before they were infected with DENV (serotype II, TSV01 strain) at the given multiplicity of infection (MOI) for 1 h [28]. Cells were incubated in complete Dulbecco’s modified minimal essential medium (DMEM, Invitrogen, Carlsbad, CA) for 2 days.RNA quantification by qRT-PCRCellular RNA or viral RNA in culture medium were extracted using TRIzol Reagent (Invitrogen) or QIAamp viral RNA minikit (Qiagen, Valencia, CA) and reverse transcribed using SuperScript III (Invitrogen). Quantitative PCR (qPCR) reaction was performed on the ABI 7500 thermocycler 1379592 (Applied Biosystems, Foster City, CA). The probe for DENV was 6-carboxyfluorescein [FAM]-59-AGCATCATTCCAGGCAC-39-MGBNFQ (molecular-groove binding nonfluorescence quencher; Applied Biosystems), forward primer 59-GARAGACCA GAGATCCTGCTGTCT-39 and reverse primer 59ACCATTCCATTTTCTGGCGTT-39 (SBS Genetech, Beijing, China). The standard curve was generated using serial 10-fold dilutions of in vitro transcribed full-length DENV RNA (TSV01 strain). The housekeeping gene b-actin was used as cont.