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Overview
Zeocin™ is a member of the bleomycin/phleomycin family of antibiotics isolated from Streptomyces. It shows strong toxicity against bacteria, fungi (including yeast), plants and mammalian cell lines (Calmels et al., 1991; Drocourt et al., 1990; Gatignol et al., 1987; Mulsant et al., 1988; Perez et al., 1989). Since Zeocin™ is active in both bacteria and mammalian cell lines, vectors can be designed that carry only one drug resistance marker for selection.
Description
Zeocin™ is a formulation of phleomycin D1, a basic, watersoluble, copper-chelated glycopeptide isolated from Streptomyces verticillus. The presence of copper gives the solution its blue color. This copper-chelated form is inactive. When the antibiotic enters the cell, the copper cation is reduced from Cu2+ to Cu1+ and removed by sulfhydryl compounds in the cell. Upon removal of the copper, Zeocin™ is activated and will bind DNA and cleave it, causing cell death.
Resistance to Zeocin™
A Zeocin™ resistance protein has been isolated and characterized (Calmels et al., 1991; Drocourt et al., 1990). This 13,665 Da protein, the product of the Sh ble gene (Streptoalloteichus hindustanus bleomycin gene), binds stoichiometrically to Zeocin™ and inhibits its DNA strand cleavage activity. Expression of this protein in eukaryotic and prokaryotic hosts confers resistance to Zeocin™.
Handling Zeocin™
- High ionic strength and acidity or basicity inhibit the activity of Zeocin™. Therefore, we recommend that you reduce the salt in bacterial medium and adjust the pH to 7.5 to keep the drug active (see Low Salt LB Medium).
- Store Zeocin™ at -20°C and thaw on ice before use.
- Zeocin™ is light sensitive. Store the drug and plates or medium containing the drug in the dark.
- Wear gloves, a laboratory coat, and safety glasses when handling Zeocin™ containing solutions.
- Do not ingest or inhale solutions containing the drug.
- Be sure to bandage any cuts on your fingers to avoid exposure to the drug.
Concentrations of Zeocin™ to use for Selection
Zeocin™ and the Sh ble gene can be used for selection in mammalian cells (Drocourt et al., 1990; Mulsant et al., 1988), plants (Perez et al., 1989), yeast (Calmels et al., 1991; Gatignol et al., 1987), and prokaryotes (Drocourt et al., 1990). Suggested concentrations of Zeocin™ to use for selection in mammalian tissue culture cells, yeast, and E. coli are listed below.
| Organism | Zeocin™ Concentration and Selective Medium |
|---|---|
| E. coli | 25-50 μg/ml in Low Salt LB medium* |
| Yeast 50 | 50-300 μg/ml in YPD or minimal medium |
| Mammalian cells | 50-1000 μg/ml (varies with cell line) |
*For efficient selection, the concentration of NaCl should not exceed 5 g/liter.
Introduction
Use 25-50 μg/ml of Zeocin™ for selection in E. coli. High salt and extremes in pH will inhibit the activity of Zeocin™ (see recommendations below).
E. coli Host
Any E. coli strain that contains the complete Tn5 transposable element (i.e. DH5αF´IQ, SURE, SURE2) encodes the ble (bleomycin) resistance gene. These strains will confer resistance to Zeocin™. For the most efficient selection, use an E. coli strain that does not contain the Tn5 gene (i.e. TOP10, DH5, DH10, etc.).
Ionic Strength and pH
Extremes in pH and high ionic strength will inhibit the activity of Zeocin™. To optimize selection in E. coli, the salt concentration must be < 110 mM and the pH must be 7.5. A recipe for Low Salt LB is provided below to optimize selection in E. coli.
Low Salt LB Medium
10 g Tryptone
5 g NaCl
5 g Yeast Extract
- Combine the dry reagents above and add deionized, distilled water to 950 ml. Adjust pH to 7.5 with 1 N NaOH and bring the volume up to 1 liter. For plates, add 15 g/L agar before autoclaving.
- Autoclave on liquid cycle at 15 psi and 121°C for 20 minutes.
- Thaw Zeocin™ on ice and vortex before removing an aliquot.
- Allow the medium to cool to at least 55°C before adding the Zeocin™ to 25 μg/ml final concentration.
Store plates and unused medium at +4°C in the dark. Plates and medium containing Zeocin™ are stable for 1-2 weeks.
Introduction
We have successfully transformed plasmids conferring Zeocin resistance into Saccharomyces cerevisiae and Pichia pastoris. The concentration of Zeocin™ required to select resistant transformants may range from 50 to 300 μg/ml, depending on the strain, pH, and ionic strength. Guidelines are provided below to assist you with selecting Zeocin™-resistant transformants.
We do not recommend spheroplasting for transformation of yeast with plasmids containing the Zeocin™ resistance marker. Spheroplasting involves removal of the cell wall to allow DNA to enter the cell. Cells must first regenerate the cell wall before they are able to express the Zeocin™ resistance gene. Plating spheroplasts directly onto selective medium containing Zeocin™ will result in complete cell death.
Transformation Method
We recommend electroporation, lithium cation protocols, or our EasyComp™ Kits for transformation of yeast with vectors that encode resistance to Zeocin™. Electroporation yields 103 to 104 transformants per μg of linearized DNA and does not destroy the cell wall of yeast. If you do not have access to an electroporation device, use chemical methods or one of the EasyComp™ Kits listed below.
| Kit | Reactions | Catalog no. |
|---|---|---|
| S. c. EasyComp Transformation Kit (for Saccharomyces cerevisiae) | 6 x 20 transformations | K5050-01 |
| Pichia EasyComp Transformation Kit (for Pichia pastoris) | 6 x 20 transformations | K1730-01 |
Ionic Strength and pH
Since yeast vary in their susceptibility to Zeocin™, we recommend that you perform a kill curve to determine the
lowest concentration of Zeocin™ needed to kill the untransformed host strain. In addition, the pH of the selection medium may affect the concentration of Zeocin™ needed to select resistant transformants. We recommend that you test media adjusted to different pH values (6.5 to 8) for the one that allows you to use the lowest possible concentration of Zeocin™.
Selection in Yeast
For successful selection of Zeocin™-resistant transformants we recommend the following:
- After transformation (either by electroporation or chemical transformation), allow the cells to recover for one hour in YPD medium.
- For electroporated cells, plate your transformants on YPD containing 1 M sorbitol. Sorbitol allows better recovery of the cells after electroporation.
- For chemically transformed cells, plate cells on YPD or minimal plates.
- Plate several different volumes (i.e. 10, 25, 50, 100, and 200 μl) of the transformation reaction. Plating at low cell densities favors efficient Zeocin™ selection.
Introduction
Mammalian cells exhibit a wide range of susceptibility to Zeocin™. Concentrations of Zeocin™ used to select stable cell lines may range from 50 to 1000 μg/ml, with the average being around 250 to 400 μg/ml. Factors that affect selection include ionic strength, cell line, cell density, and growth rate. Review the guidelines below to ensure successful selection of stable cell lines.
Important
Zeocin™ mechanism of killing is quite different from neomycin and hygromycin. Cells do not round up and detach from the plate. Sensitive cells may exhibit the following morphological changes upon exposure to Zeocin™:
Eventually, these cells will completely break down and only cellular debris will remain.
Zeocin™-resistant cells should continue to divide at regular intervals to form distinct colonies. There should not be any distinct morphological changes in Zeocin™-resistant cells when compared to cells not under selection with Zeocin™.
Mammalian cells exhibit a wide range of susceptibility to Zeocin™. Concentrations of Zeocin™ used to select stable cell lines may range from 50 to 1000 μg/ml, with the average being around 250 to 400 μg/ml. Factors that affect selection include ionic strength, cell line, cell density, and growth rate. Review the guidelines below to ensure successful selection of stable cell lines.
Important
Zeocin™ mechanism of killing is quite different from neomycin and hygromycin. Cells do not round up and detach from the plate. Sensitive cells may exhibit the following morphological changes upon exposure to Zeocin™:
- Vast increase in size (similar to the effects of cytomegalovirus infecting permissive cells)
- Abnormal cell shape, including the appearance of long appendages
- Presence of large empty vesicles in the cytoplasm (breakdown of the endoplasmic reticulum and Golgi apparatus or scaffolding proteins)
- Breakdown of plasma and nuclear membrane (appearance of many holes in these membranes)
Eventually, these cells will completely break down and only cellular debris will remain.
Zeocin™-resistant cells should continue to divide at regular intervals to form distinct colonies. There should not be any distinct morphological changes in Zeocin™-resistant cells when compared to cells not under selection with Zeocin™.
Ionic Strength and pH
For selection in mammalian cells, physiological ionic strength and pH are much more important for cell growth, so more Zeocin™ may be needed for selection relative to yeast or bacteria.
Selection in Mammalian Cell Lines
To generate a stable cell line that expresses your protein from an expression construct, you need to determine the minimum concentration required to kill your untransfected host cell line (see Determination of Zeocin™ Sensitivity, below). In general, it takes 2-6 weeks to generate foci with Zeocin™, depending on the cell line. Because individual cells can express protein at varying levels, it is important to isolate several foci to expand into stable cell lines.
Determining Zeocin™ Sensitivity
Determine the minimal concentration of Zeocin™ required to kill the untransfected parental cell line using the protocol below.
If you have trouble distinguishing viable cells by observation, we recommend counting the number of viable cells by trypan blue exclusion to determine the appropriate concentration of Zeocin™ required to prevent growth.
Selection Tip
Some cells may be more resistant to Zeocin™ than others. If cells are rapidly dividing, Zeocin™ may not be effective at low concentrations. We suggest trying the following protocol to overcome this resistance:
Incubating the cells at +4°C will stop the cell division process for a short time, allow Zeocin™ to act, and result in cel death.
For selection in mammalian cells, physiological ionic strength and pH are much more important for cell growth, so more Zeocin™ may be needed for selection relative to yeast or bacteria.
Selection in Mammalian Cell Lines
To generate a stable cell line that expresses your protein from an expression construct, you need to determine the minimum concentration required to kill your untransfected host cell line (see Determination of Zeocin™ Sensitivity, below). In general, it takes 2-6 weeks to generate foci with Zeocin™, depending on the cell line. Because individual cells can express protein at varying levels, it is important to isolate several foci to expand into stable cell lines.
Determining Zeocin™ Sensitivity
Determine the minimal concentration of Zeocin™ required to kill the untransfected parental cell line using the protocol below.
- Plate or split a confluent plate so the cells will be approximately 25% confluent. Prepare a set of 8 plates. Grow cells for 24 hours.
- Remove medium and then add medium with varying concentrations of Zeocin™ (0, 50, 100, 200, 400, 600, 800, and 1000 μg/ml) to each plate.
- Replenish the selective medium every 3-4 days and observe the percentage of surviving cells over time. Select the concentration that kills the majority of the cells in the desired number of days (within 1-2 weeks).
If you have trouble distinguishing viable cells by observation, we recommend counting the number of viable cells by trypan blue exclusion to determine the appropriate concentration of Zeocin™ required to prevent growth.
Selection Tip
Some cells may be more resistant to Zeocin™ than others. If cells are rapidly dividing, Zeocin™ may not be effective at low concentrations. We suggest trying the following protocol to overcome this resistance:
- Split cells into medium containing Zeocin™.
- Incubate cells at 37°C for 2-3 hours until the cells have attached to the culture dish.
- Remove the plates from the incubator and place the cells at +4°C for 2 hours. Be sure to buffer the medium with HEPES.
- Return the cells to 37°C.
Incubating the cells at +4°C will stop the cell division process for a short time, allow Zeocin™ to act, and result in cel death.
Selecting Stable Integrants
Once you have determined the appropriate Zeocin™ concentration to use for selection, you can generate a stable cell line with your construct.
Maintaining Stable Cell Lines
To maintain stable cell lines, you may:
Once you have determined the appropriate Zeocin™ concentration to use for selection, you can generate a stable cell line with your construct.
- Transfect your cell line and plate onto 100 mm culture plates. Include a sample of untransfected cells as a negative control.
- After transfection, wash the cells once with 1X PBS and add fresh medium to the cells.
- Forty-eight to 72 hours after transfection, split the cells using various dilutions into fresh medium containing Zeocin™ at the pre-determined concentration required for your cell line. By using different dilutions, you will have a better chance at identifying and selecting foci.
- Feed the cells with selective medium every 3-4 days until cell foci are identified.
- Pick and transfer colonies to either 96- or 48-well plates. Grow cells to near confluence before expanding to larger wells or plates.
Note: If your cells are more resistant to Zeocin™, you may want to use the selection tip described above. Simply split cells into medium containing Zeocin™, incubate at 37°C for 2-3 hours to let cells attach, then
place the cells at +4°C for 2 hours. Remember to buffer the medium with HEPES.
Maintaining Stable Cell Lines
To maintain stable cell lines, you may:
- Maintain the cells in the same concentration of Zeocin™ you used for selection
- Reduce the concentration of Zeocin™ by half
- Reduce the concentration of Zeocin™ to the concentration that just prevents growth of sensitive cells but does not kill them (refer to your kill curve experiment).
TOP
- Berdy, J. (1980) Bleomycin-Type Antibiotics. In Amino Acid and Peptide Antibiotics, J. Berdy, ed. (Boca Raton, FL: CRC Press), pp. 459-497.
- Calmels, T., Parriche, M., Burand, H., and Tiraby, G. (1991). High Efficiency Transformation of Tolypocladium geodes Conidiospores to Phleomycin Resistance. Curr. Genet. 20, 309-314.
- Drocourt, D., Calmels, T. P. G., Reynes, J. P., Baron, M., and Tiraby, G. (1990). Cassettes of the Streptoalloteichus hindustanus ble Gene for Transformation of Lower and Higher Eukaryotes to Phleomycin Resistance. Nucleic Acids Res. 18, 4009.
- Gatignol, A., Baron, M., and Tiraby, G. (1987). Phleomycin Resistance Encoded by the ble Gene from Transposon Tn5 as a Dominant Selectable Marker in Saccharomyces cerevisiae. Molecular and General Genetics 207, 342-348.
- Graham, F. L., Smiley, J., Russell, W. C., and Nairn, R. (1977). Characteristics of a Human Cell Line Transformed by DNA from Human Adenovirus Type 5. J. Gen. Virol. 36, 59-74.
- Mulsant, P., Tiraby, G., Kallerhoff, J., and Perret, J. (1988). Phleomycin Resistance as a Dominant SelectableMarker in CHO Cells. Somat. Cell Mol. Genet. 14, 243- 252.
- Perez, P., Tiraby, G., Kallerhoff, J., and Perret, J. (1989). Phleomycin Resistance as a Dominant Selectable Marker for Plant Cell Transformation. Plant Mol. Biol. 13, 365-373.
TOP
25-0078 Version J 22-Aug-2002