luciferase reporter assay Search Results


luciferase reporter assay kit vazyme cat  (Vazyme Biotech Co)
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Vazyme Biotech Co luciferase reporter assay kit vazyme cat
Luciferase Reporter Assay Kit Vazyme Cat, supplied by Vazyme Biotech Co, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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ready to glow tm nf κb secreted luciferase reporter system  (TaKaRa)
95
TaKaRa ready to glow tm nf κb secreted luciferase reporter system
Ready To Glow Tm Nf κb Secreted Luciferase Reporter System, supplied by TaKaRa, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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luciferase reporter  (BPS Bioscience)
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BPS Bioscience luciferase reporter
Luciferase Reporter, supplied by BPS Bioscience, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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luciferase reporter assay 570 cells  (Addgene inc)
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Addgene inc luciferase reporter assay 570 cells
Luciferase Reporter Assay 570 Cells, supplied by Addgene inc, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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gal4uas luciferase reporter  (Addgene inc)
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Addgene inc gal4uas luciferase reporter
Gal4uas Luciferase Reporter, supplied by Addgene inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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luciferase reporter  (Addgene inc)
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Addgene inc luciferase reporter
Luciferase Reporter, supplied by Addgene inc, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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hepg2 nrf2 cells  (BPS Bioscience)
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BPS Bioscience hepg2 nrf2 cells
Comparison of AOP1 EC 50 s evaluated in Caco-2 and <t> HepG2 cells </t> for the 12 natural extracts selected for the intestinal barrier transport study. Extracts were selected according to the best EC 50 s obtained with AOP1 assay. In order to increase the diversity of tested extracts, some Vitis vinifera extracts were removed from the list because of redundancy with each other. ND = not determined (no full effect observed).
Hepg2 Nrf2 Cells, supplied by BPS Bioscience, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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luciferase lentivirus  (BPS Bioscience)
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BPS Bioscience luciferase lentivirus
NFATc4 expression and NFAT transcriptional activity following lentiviral transduction. ( A ) Nfatc4 mRNA expression was assessed in primary hippocampal neurons following transduction with either Lenti-GFP-NFATc4 or Lenti-GFP, using real-time PCR. Raw data were normalized to Gapdh endogenous expression and calculated using 2 −ΔΔCt method. Nfatc4 expression level in non-transduced cells was set as 1. The data are presented as means ± SEM, with individual values obtained from n = 4 replicate treatment. ( B ) Primary hippocampal neurons were co-transduced with NFAT dual-reporter <t>lentivirus</t> and Lenti-GFP-NFATc4 (or other viruses as indicated on the graph) on DIV0 and cultured until DIV3. NFAT transcriptional activity was determined in cell lysates by measuring <t>luciferase</t> activity (n = 4). The results are expressed as a fold induction above baseline activity. The data are presented as means ± SEM, with individual values indicated on the graphs. * P < 0.05, *** P < 0.001. ( C ) Lenti-GFP or Lenti-GFP-NFATc4 were intravitreally injected into NFATc4 −/− retinas, followed by NFATc4 staining three weeks later. The retinas were stained using the antibodies indicated in Retina cryosection staining (primary: NFATc4, 1:500, Merck, USA; secondary: anti-rabbit conjugated to Alexa Fluor 488, 1:500, Thermo Fisher, USA). Representative images are presented. Scale bar: 100 μm
Luciferase Lentivirus, supplied by BPS Bioscience, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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tead luciferase reporter lentivirus  (BPS Bioscience)
93
BPS Bioscience tead luciferase reporter lentivirus
NFATc4 expression and NFAT transcriptional activity following lentiviral transduction. ( A ) Nfatc4 mRNA expression was assessed in primary hippocampal neurons following transduction with either Lenti-GFP-NFATc4 or Lenti-GFP, using real-time PCR. Raw data were normalized to Gapdh endogenous expression and calculated using 2 −ΔΔCt method. Nfatc4 expression level in non-transduced cells was set as 1. The data are presented as means ± SEM, with individual values obtained from n = 4 replicate treatment. ( B ) Primary hippocampal neurons were co-transduced with NFAT dual-reporter <t>lentivirus</t> and Lenti-GFP-NFATc4 (or other viruses as indicated on the graph) on DIV0 and cultured until DIV3. NFAT transcriptional activity was determined in cell lysates by measuring <t>luciferase</t> activity (n = 4). The results are expressed as a fold induction above baseline activity. The data are presented as means ± SEM, with individual values indicated on the graphs. * P < 0.05, *** P < 0.001. ( C ) Lenti-GFP or Lenti-GFP-NFATc4 were intravitreally injected into NFATc4 −/− retinas, followed by NFATc4 staining three weeks later. The retinas were stained using the antibodies indicated in Retina cryosection staining (primary: NFATc4, 1:500, Merck, USA; secondary: anti-rabbit conjugated to Alexa Fluor 488, 1:500, Thermo Fisher, USA). Representative images are presented. Scale bar: 100 μm
Tead Luciferase Reporter Lentivirus, supplied by BPS Bioscience, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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nfat luciferase reporter  (BPS Bioscience)
93
BPS Bioscience nfat luciferase reporter
NFATc4 expression and NFAT transcriptional activity following lentiviral transduction. ( A ) Nfatc4 mRNA expression was assessed in primary hippocampal neurons following transduction with either Lenti-GFP-NFATc4 or Lenti-GFP, using real-time PCR. Raw data were normalized to Gapdh endogenous expression and calculated using 2 −ΔΔCt method. Nfatc4 expression level in non-transduced cells was set as 1. The data are presented as means ± SEM, with individual values obtained from n = 4 replicate treatment. ( B ) Primary hippocampal neurons were co-transduced with NFAT dual-reporter <t>lentivirus</t> and Lenti-GFP-NFATc4 (or other viruses as indicated on the graph) on DIV0 and cultured until DIV3. NFAT transcriptional activity was determined in cell lysates by measuring <t>luciferase</t> activity (n = 4). The results are expressed as a fold induction above baseline activity. The data are presented as means ± SEM, with individual values indicated on the graphs. * P < 0.05, *** P < 0.001. ( C ) Lenti-GFP or Lenti-GFP-NFATc4 were intravitreally injected into NFATc4 −/− retinas, followed by NFATc4 staining three weeks later. The retinas were stained using the antibodies indicated in Retina cryosection staining (primary: NFATc4, 1:500, Merck, USA; secondary: anti-rabbit conjugated to Alexa Fluor 488, 1:500, Thermo Fisher, USA). Representative images are presented. Scale bar: 100 μm
Nfat Luciferase Reporter, supplied by BPS Bioscience, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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tet on inducible fto knockdown vectors  (Addgene inc)
92
Addgene inc tet on inducible fto knockdown vectors
NFATc4 expression and NFAT transcriptional activity following lentiviral transduction. ( A ) Nfatc4 mRNA expression was assessed in primary hippocampal neurons following transduction with either Lenti-GFP-NFATc4 or Lenti-GFP, using real-time PCR. Raw data were normalized to Gapdh endogenous expression and calculated using 2 −ΔΔCt method. Nfatc4 expression level in non-transduced cells was set as 1. The data are presented as means ± SEM, with individual values obtained from n = 4 replicate treatment. ( B ) Primary hippocampal neurons were co-transduced with NFAT dual-reporter <t>lentivirus</t> and Lenti-GFP-NFATc4 (or other viruses as indicated on the graph) on DIV0 and cultured until DIV3. NFAT transcriptional activity was determined in cell lysates by measuring <t>luciferase</t> activity (n = 4). The results are expressed as a fold induction above baseline activity. The data are presented as means ± SEM, with individual values indicated on the graphs. * P < 0.05, *** P < 0.001. ( C ) Lenti-GFP or Lenti-GFP-NFATc4 were intravitreally injected into NFATc4 −/− retinas, followed by NFATc4 staining three weeks later. The retinas were stained using the antibodies indicated in Retina cryosection staining (primary: NFATc4, 1:500, Merck, USA; secondary: anti-rabbit conjugated to Alexa Fluor 488, 1:500, Thermo Fisher, USA). Representative images are presented. Scale bar: 100 μm
Tet On Inducible Fto Knockdown Vectors, supplied by Addgene inc, used in various techniques. Bioz Stars score: 92/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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nfat luciferase reporter lentivirus  (BPS Bioscience)
93
BPS Bioscience nfat luciferase reporter lentivirus
NFATc4 expression and NFAT transcriptional activity following lentiviral transduction. ( A ) Nfatc4 mRNA expression was assessed in primary hippocampal neurons following transduction with either Lenti-GFP-NFATc4 or Lenti-GFP, using real-time PCR. Raw data were normalized to Gapdh endogenous expression and calculated using 2 −ΔΔCt method. Nfatc4 expression level in non-transduced cells was set as 1. The data are presented as means ± SEM, with individual values obtained from n = 4 replicate treatment. ( B ) Primary hippocampal neurons were co-transduced with NFAT dual-reporter <t>lentivirus</t> and Lenti-GFP-NFATc4 (or other viruses as indicated on the graph) on DIV0 and cultured until DIV3. NFAT transcriptional activity was determined in cell lysates by measuring <t>luciferase</t> activity (n = 4). The results are expressed as a fold induction above baseline activity. The data are presented as means ± SEM, with individual values indicated on the graphs. * P < 0.05, *** P < 0.001. ( C ) Lenti-GFP or Lenti-GFP-NFATc4 were intravitreally injected into NFATc4 −/− retinas, followed by NFATc4 staining three weeks later. The retinas were stained using the antibodies indicated in Retina cryosection staining (primary: NFATc4, 1:500, Merck, USA; secondary: anti-rabbit conjugated to Alexa Fluor 488, 1:500, Thermo Fisher, USA). Representative images are presented. Scale bar: 100 μm
Nfat Luciferase Reporter Lentivirus, supplied by BPS Bioscience, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


Comparison of AOP1 EC 50 s evaluated in Caco-2 and HepG2 cells for the 12 natural extracts selected for the intestinal barrier transport study. Extracts were selected according to the best EC 50 s obtained with AOP1 assay. In order to increase the diversity of tested extracts, some Vitis vinifera extracts were removed from the list because of redundancy with each other. ND = not determined (no full effect observed).

Journal: Antioxidants

Article Title: Cell-Based Antioxidant Properties and Synergistic Effects of Natural Plant and Algal Extracts Pre and Post Intestinal Barrier Transport

doi: 10.3390/antiox11030565

Figure Lengend Snippet: Comparison of AOP1 EC 50 s evaluated in Caco-2 and HepG2 cells for the 12 natural extracts selected for the intestinal barrier transport study. Extracts were selected according to the best EC 50 s obtained with AOP1 assay. In order to increase the diversity of tested extracts, some Vitis vinifera extracts were removed from the list because of redundancy with each other. ND = not determined (no full effect observed).

Article Snippet: The HepG2/Nrf2 cells were treated with conditions for 17 h; then, they were treated with a mix (BPS Bioscience, USA) comprising cell lysis solution and luciferin (substrate of luciferase) for 40 min. Luminescence was read on a Varioskan Flash Spectral Scanning Multimode Reader.

Techniques:

Indirect antioxidant ARE/Nrf2 assay data obtained for Syzygium aromaticum extract (given as an example) in HepG2/Nrf2 cells. All other extracts were subjected to the same protocol and data analyses. ( A ) Assay of increasing concentrations showing the typical bell-shaped profile (see text for explanation). Sulforaphane 25 µM was used as positive control; ( B ) dose–response and sigmoid fit curve used for Efficacy Concentration (EC) estimations.

Journal: Antioxidants

Article Title: Cell-Based Antioxidant Properties and Synergistic Effects of Natural Plant and Algal Extracts Pre and Post Intestinal Barrier Transport

doi: 10.3390/antiox11030565

Figure Lengend Snippet: Indirect antioxidant ARE/Nrf2 assay data obtained for Syzygium aromaticum extract (given as an example) in HepG2/Nrf2 cells. All other extracts were subjected to the same protocol and data analyses. ( A ) Assay of increasing concentrations showing the typical bell-shaped profile (see text for explanation). Sulforaphane 25 µM was used as positive control; ( B ) dose–response and sigmoid fit curve used for Efficacy Concentration (EC) estimations.

Article Snippet: The HepG2/Nrf2 cells were treated with conditions for 17 h; then, they were treated with a mix (BPS Bioscience, USA) comprising cell lysis solution and luciferin (substrate of luciferase) for 40 min. Luminescence was read on a Varioskan Flash Spectral Scanning Multimode Reader.

Techniques: Positive Control, Concentration Assay

ARE/Nrf2 EC 50 s established in HepG2 cells for the 12 natural extracts selected for the Caco-2 intestinal barrier transport study. ND = not determined; R 2 = determination coefficient.

Journal: Antioxidants

Article Title: Cell-Based Antioxidant Properties and Synergistic Effects of Natural Plant and Algal Extracts Pre and Post Intestinal Barrier Transport

doi: 10.3390/antiox11030565

Figure Lengend Snippet: ARE/Nrf2 EC 50 s established in HepG2 cells for the 12 natural extracts selected for the Caco-2 intestinal barrier transport study. ND = not determined; R 2 = determination coefficient.

Article Snippet: The HepG2/Nrf2 cells were treated with conditions for 17 h; then, they were treated with a mix (BPS Bioscience, USA) comprising cell lysis solution and luciferin (substrate of luciferase) for 40 min. Luminescence was read on a Varioskan Flash Spectral Scanning Multimode Reader.

Techniques:

Effect of post-intestinal barrier transport compartments on ARE/NRF2 pathway activation in HepG2 cells. Results are expressed as fold increase compared to constitutive medium ARE/Nrf2 gene expression. Values represent means of quadruplicates obtained from two independent intestinal barrier transport experiments. Sulforaphane 25 µM data is provided as positive control; *** p < 0.005.

Journal: Antioxidants

Article Title: Cell-Based Antioxidant Properties and Synergistic Effects of Natural Plant and Algal Extracts Pre and Post Intestinal Barrier Transport

doi: 10.3390/antiox11030565

Figure Lengend Snippet: Effect of post-intestinal barrier transport compartments on ARE/NRF2 pathway activation in HepG2 cells. Results are expressed as fold increase compared to constitutive medium ARE/Nrf2 gene expression. Values represent means of quadruplicates obtained from two independent intestinal barrier transport experiments. Sulforaphane 25 µM data is provided as positive control; *** p < 0.005.

Article Snippet: The HepG2/Nrf2 cells were treated with conditions for 17 h; then, they were treated with a mix (BPS Bioscience, USA) comprising cell lysis solution and luciferin (substrate of luciferase) for 40 min. Luminescence was read on a Varioskan Flash Spectral Scanning Multimode Reader.

Techniques: Activation Assay, Expressing, Positive Control

Effect of combinations of post-intestinal barrier compartments on ARE/NRF2 pathway in HepG2 cells. Results are expressed as ARE/Nrf2 gene expression fold increase compared to constitutive medium. Values represent means of pentaplicates for all 50/50 combinations and of triplicates for all others. All data were normalized to constitutive medium values; *** p < 0.001; ** p < 0.01.

Journal: Antioxidants

Article Title: Cell-Based Antioxidant Properties and Synergistic Effects of Natural Plant and Algal Extracts Pre and Post Intestinal Barrier Transport

doi: 10.3390/antiox11030565

Figure Lengend Snippet: Effect of combinations of post-intestinal barrier compartments on ARE/NRF2 pathway in HepG2 cells. Results are expressed as ARE/Nrf2 gene expression fold increase compared to constitutive medium. Values represent means of pentaplicates for all 50/50 combinations and of triplicates for all others. All data were normalized to constitutive medium values; *** p < 0.001; ** p < 0.01.

Article Snippet: The HepG2/Nrf2 cells were treated with conditions for 17 h; then, they were treated with a mix (BPS Bioscience, USA) comprising cell lysis solution and luciferin (substrate of luciferase) for 40 min. Luminescence was read on a Varioskan Flash Spectral Scanning Multimode Reader.

Techniques: Expressing

Synergistic effects on ARE/Nrf2 gene expression of post-intestinal barrier compartment combinations. Combin. FI = gene expression fold increase (FI) measure for the combination; S indep. FI = sum of the increase in gene expression fold increase (FI) measures of each of the two extracts taken independently as depicted in <xref ref-type= Figure 6 ; Var. (%) = variation in percentage of the two values. A positive percentage value indicates a synergistic effect." width="100%" height="100%">

Journal: Antioxidants

Article Title: Cell-Based Antioxidant Properties and Synergistic Effects of Natural Plant and Algal Extracts Pre and Post Intestinal Barrier Transport

doi: 10.3390/antiox11030565

Figure Lengend Snippet: Synergistic effects on ARE/Nrf2 gene expression of post-intestinal barrier compartment combinations. Combin. FI = gene expression fold increase (FI) measure for the combination; S indep. FI = sum of the increase in gene expression fold increase (FI) measures of each of the two extracts taken independently as depicted in Figure 6 ; Var. (%) = variation in percentage of the two values. A positive percentage value indicates a synergistic effect.

Article Snippet: The HepG2/Nrf2 cells were treated with conditions for 17 h; then, they were treated with a mix (BPS Bioscience, USA) comprising cell lysis solution and luciferin (substrate of luciferase) for 40 min. Luminescence was read on a Varioskan Flash Spectral Scanning Multimode Reader.

Techniques: Expressing

NFATc4 expression and NFAT transcriptional activity following lentiviral transduction. ( A ) Nfatc4 mRNA expression was assessed in primary hippocampal neurons following transduction with either Lenti-GFP-NFATc4 or Lenti-GFP, using real-time PCR. Raw data were normalized to Gapdh endogenous expression and calculated using 2 −ΔΔCt method. Nfatc4 expression level in non-transduced cells was set as 1. The data are presented as means ± SEM, with individual values obtained from n = 4 replicate treatment. ( B ) Primary hippocampal neurons were co-transduced with NFAT dual-reporter lentivirus and Lenti-GFP-NFATc4 (or other viruses as indicated on the graph) on DIV0 and cultured until DIV3. NFAT transcriptional activity was determined in cell lysates by measuring luciferase activity (n = 4). The results are expressed as a fold induction above baseline activity. The data are presented as means ± SEM, with individual values indicated on the graphs. * P < 0.05, *** P < 0.001. ( C ) Lenti-GFP or Lenti-GFP-NFATc4 were intravitreally injected into NFATc4 −/− retinas, followed by NFATc4 staining three weeks later. The retinas were stained using the antibodies indicated in Retina cryosection staining (primary: NFATc4, 1:500, Merck, USA; secondary: anti-rabbit conjugated to Alexa Fluor 488, 1:500, Thermo Fisher, USA). Representative images are presented. Scale bar: 100 μm

Journal: Molecular Neurobiology

Article Title: NFATc4 Knockout Promotes Neuroprotection and Retinal Ganglion Cell Regeneration After Optic Nerve Injury

doi: 10.1007/s12035-024-04129-0

Figure Lengend Snippet: NFATc4 expression and NFAT transcriptional activity following lentiviral transduction. ( A ) Nfatc4 mRNA expression was assessed in primary hippocampal neurons following transduction with either Lenti-GFP-NFATc4 or Lenti-GFP, using real-time PCR. Raw data were normalized to Gapdh endogenous expression and calculated using 2 −ΔΔCt method. Nfatc4 expression level in non-transduced cells was set as 1. The data are presented as means ± SEM, with individual values obtained from n = 4 replicate treatment. ( B ) Primary hippocampal neurons were co-transduced with NFAT dual-reporter lentivirus and Lenti-GFP-NFATc4 (or other viruses as indicated on the graph) on DIV0 and cultured until DIV3. NFAT transcriptional activity was determined in cell lysates by measuring luciferase activity (n = 4). The results are expressed as a fold induction above baseline activity. The data are presented as means ± SEM, with individual values indicated on the graphs. * P < 0.05, *** P < 0.001. ( C ) Lenti-GFP or Lenti-GFP-NFATc4 were intravitreally injected into NFATc4 −/− retinas, followed by NFATc4 staining three weeks later. The retinas were stained using the antibodies indicated in Retina cryosection staining (primary: NFATc4, 1:500, Merck, USA; secondary: anti-rabbit conjugated to Alexa Fluor 488, 1:500, Thermo Fisher, USA). Representative images are presented. Scale bar: 100 μm

Article Snippet: NFAT luciferase reporter lentivirus and firefly luciferase lentivirus were sourced from BPS Bioscience (USA).

Techniques: Expressing, Activity Assay, Transduction, Real-time Polymerase Chain Reaction, Cell Culture, Luciferase, Injection, Staining