ViroVision™ Infection Medium
ViroVision™ Infection Medium is a viral infection enhancer designed to facilitate viral penetration of the cortical actin barrier, thereby greatly enhancing productive viral infection. ViroVision™ Infection Medium can be used to facilitate the infection of a variety of host cells by different viruses and viral vectors. ViroVision™ Infection Medium can enhance viral infection rates by 5 to 20 fold. Virongy developed It is based on the scientific theory that the actin cytoskeleton is a natural barrier for viral entry and post-entry intracellular migration.
(Yoder et al., Cell, 2008, 134:782).
Applications
- Enhancing lenti- or retroviral transduction of target cells
- Enhancing infection rates of other enveloped viruses
- Facilitating recovery of infectious viruses from cell or tissue cultures
- Facilitating anti-viral drug screening efficiency
Table1:10 x Concentrated ViroVision™ Infection Medium
| Catalog NO. | Product |
| CUBME0011 |
ViroVision™ Infection Medium (200 µl) |
| CUBME0012 | ViroVision™ Infection Medium (1 ml) |
| CUBME0013 | ViroVision™ Infection Medium (5 Vials X 1 ml) |
Protocol
Example 1 - ViroVision™ Infection Medium used to enhance lentiviral infection of suspension CEM-SS cells:
(See Table 2 for scale-up recommendations)
1. Count cells to be infected, and pellet cells by centrifugation at 300 x g for 5 minutes.
Note: Cell viability should be ≥ 80%.
2. Resuspend cells in complete media at a concentration of ~2 x 106 cells mL-1.
3. Use 100 μl of cells (~2 x 105) per ViroVision™ Infection Medium.
4. Pre-treat cells by adding 10 μl of ViroVision™ Infection Medium so that ViroVision™ Infection Medium concentration is ~1X. Mix and incubate for 30–60 minutes.
For best results, when using ViroVision™ Infection Medium for the first time, start with a higher concentration (final ViroVision™ Infection Medium concentration may be 2X or 3X). The lowest effective dosage can be determined through a titration experiment (final ViroVision™ Infection Medium concentration may be as low as 1X).
5. Add virus to the cells and mix. Note volume of virus used.
6. Add ViroVision™ Infection Medium in an amount equal to 1/10 of the virus volume used, e.g., if 100 μl of virus is used, add 10 μl of ViroVision™ Infection Medium. Incubate at 37°C for 2-4 hours.
7. Add 1 ml fresh complete media to wash cells. Pellet cells as above and remove supernatant. Optional: Repeat once for a total of 2 washes.
8. After washing, resuspend cells in 1 ml complete medium.
9. Culture infected cells as usual to quantify viral replication.
Table 2: Scaleup Recommendations Using ViroVision™ Infection Medium
|
Cell Number (For ViroVision™ Infection Medium) |
Cell Volumn |
ViroVision™ Infection Medium 10X |
Final Cell Culture Volumn |
| 2 x 105 | 100ul | 10ul | 1ml |
| 5 x 105 | 250ul | 25ul | 2.5ml |
| 1 x 106 | 500ul | 50ul | 5ml |
| 2 x 106 | 1ml | 100ul | 10ml |
| 5 x 106 | 2.5ml | 250ul | 25ml |
| 1 x 107 | 5ml | 500ul | 50ml |
| 5 x 107 | 25ml | 2.5ml | 250ml |
| 1 x 108 | 50ml | 5ml | 500ml |
Example 2 - ViroVision™ Infection Medium enhances lentiviral transduction of adherent HDFn cells:
1. Count HDFn (Human Dermal Fibroblast, neonatal) cells to be infected and seed ~5 x 105 cells per well into 6-well plates (2 ml per well).
2. Culture cells until cells stably adhere to the plates (4–12 hours).
Note: Cell viability should be ≥ 80%.
3. Before infection, wash cells with 2 ml medium, and leave 0.5 ml medium in each well.
4. Pre-treat cells by adding 50 μl of ViroVision™ Infection Medium so that Infectin concentration is ~1X. Mix and incubate for 30–60 minutes.
For best results, when using ViroVision™ Infection Medium for the first time, start with a higher concentration (final Infectin concentration may be 2X or 3X). The lowest effective dosage can be determined through a titration experiment (final ViroVision™ Infection Medium concentration may be as low as 1X).
5. Add virus to cells and mix. Note volume of virus used.
6. Add ViroVision™ Infection Medium in an amount equal to 1/10 of the virus volume used, e.g., if 100 μl of virus is used, add 10 μl of ViroVision™ Infection Medium. Incubate at 37°C for 2–4 hours.
7. Add 2 ml fresh media to wash cells.
8. After washing, add 2 ml fresh complete medium.
9. Culture infected cells as usual.
Viral Enhancement Results:
ViroVision™ Infection Medium enhances lentiviral transduction of Hep G2 cells:
-
- Hep G2 cells were transduced with lenti-GFP vector in the presence or absence of ViroVision™ Infection Medium.
| Catalog No: | CUBME0012 |
| Description: | ViroVision™ Infection Medium (patent pending) is a unique, HIV-specific infection enhancer that does.. |
| Applications: | Enhancing lenti- or retroviral transduction of target cells; Enhancing infection rates of other enveloped viruses; Facilitating recovery of infectious viruses from cell or tissue cultures; Facilitating anti-viral drug screening efficiency. |
| Catalog No: | CUBME0011 |
| Description: | ViroVision™ Infection Medium (patent pending) is a unique, HIV-specific infection enhancer that does.. |
| Applications: | Enhancing lenti- or retroviral transduction of target cells; Enhancing infection rates of other enveloped viruses; Facilitating recovery of infectious viruses from cell or tissue cultures; Facilitating anti-viral drug screening efficiency. |
| Catalog No: | CUBME0013 |
| Description: | ViroVision™ Infection Medium (patent pending) is a unique, HIV-specific infection enhancer that does.. |
| Applications: | Enhancing lenti- or retroviral transduction of target cells; Enhancing infection rates of other enveloped viruses; Facilitating recovery of infectious viruses from cell or tissue cultures; Facilitating anti-viral drug screening efficiency. |