Zeocin说明书-其它资料-资讯-生物在线

Zeocin说明书

作者:北京索莱宝科技有限公司 2014-05-09T00:00 (访问量:3464)

北京索莱宝科技有限公司 张净花 010-56371206

Zeocin

Catalog no.                      Quantity                                        Store at -20°C

R250-01                       1 g (8 × 1.25 ml)

R250-05                        5 g (50 ml)

Description

Zeocin™ is a formulation of phleomycin D1, a basic, water-soluble, copperchelated

glycopeptide isolated from Streptomyces verticillus and shows

strong toxicity against bacteria, fungi (including yeast), plants, and

mammalian cell lines. The blue color of the solution is due to the presence

of copper and the copper-chelated form of Zeocin™ 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 copper removal,

Zeocin™ is activated, and binds and cleaves DNA, causing cell death.

A Zeocin™ resistance protein of 13,665 Da, has been isolated and

characterized. The protein is 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™.

Note: Basic information on using Zeocin™ is described in this insert. For

details including Zeocin™ structure and photographs of Zeocin™ treated

cells, download the Zeocin™ manual from www.invitrogen.com.

Specifications

Contents: 100 mg/ml solution in deionized, autoclaved water.

Shipping/Storage: Shipped on blue ice. Store at -20°C.

E. coli Selection: 25-50 μg/ml in low salt LB medium*

*(NaCl concentration should not exceed 5 g/liter.)

Yeast Selection: 50-300 μg/ml in YPD or minimal medium

Mammalian Cells 50-1000 μg/ml in suitable medium (varies with cell

Selection: line).

Part No. R250.pps

Handling Zeocin™

• Always wear gloves, a laboratory coat, and safety glasses when

handling Zeocin™ containing solutions.

• Zeocin™ is light sensitive. Store the antibiotic and plates or medium

containing the antibiotic in the dark.

• Reduce the salt in bacterial medium and adjust the pH to 7.5 to keep

Zeocin™ active as high ionic strength and acidity or basicity inhibit

Zeocin™ activity.

• Store Zeocin™ at -20ºC and thaw on ice before use.

Zeocin™ Selection in E. coli

Host: Must not contain the Tn5 transposon (i.e. TOP10, DH5, DH10).

Medium: Use Low Salt LB Medium (10 g Tryptone, 5 g NaCl, and 5 g

Yeast Extract) at pH 7.5 to prevent inactivation of Zeocin™.

Selection: Use 25-50 μg/ml of Zeocin™ for selection in E. coli.

Zeocin™ Selection in Yeast

Yeast: Saccharomyces cerevisiae, Pichia pastoris

Medium: YPD with 1 M sorbitol (electroporated cells); YPD or minimal

plates (chemically transformed cells). Test the medium adjusted to pH

values ranging from 6.5-8.0 and select the pH that allows you to use lowest

Zeocin™ concentration.

Transformation Method: Use electroporation, lithium cation protocols, or

EasyComp™ Kits. Do not use spheroplasting for yeast transformation with

Zeocin™ containing plasmids as it results in complete cell death.

Selection: Use 50-300 μg/ml of Zeocin™, depending on the yeast strain,

and media pH and ionic strength. Perform a kill curve to determine the

lowest Zeocin concentration required to kill the untransformed host strain.

Note: Allow the cells to recover for 1 hour in YPD medium after

transformation. To obtain efficient Zeocin™ selection, plate at low cell

densities (use 10, 25, 50, 100, and 200 μl of transformation reaction).

Zeocin™ Selection in Mammalian Cells

Use 50-1000 μg/ml of Zeocin™ to select stable cell lines (the

average is about 250-400 μg/ml). Depending on the cell line, it

takes 2-6 weeks to generate foci with Zeocin™. Determine the

minimum concentration required to kill your untransfected

host cell line prior to generating stable cell lines (see below).

Determining Zeocin™ Sensitivity

1. Plate or split a confluent plate to obtain cells at ~25%

confluency. Prepare a set of 8 plates. Grow cells for

24 hours. Remove the medium.

2. Add medium with varying Zeocin™ concentrations (0, 50,

100, 200, 400, 600, 800, and 1000 μg/ml) to each plate.

3. Replenish selective medium every 3-4 days and observe

the percentage of surviving cells. Select the concentration

that kills the majority of cells within 1-2 weeks.

Selecting Stable Integrants

1. Transfect your cell line and plate onto 100 mm culture

plates. Include a sample of untransfected cells as a

negative control.

2. After transfection, wash the cells once with 1X PBS and

add fresh medium to the cells.

3. 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.

To have a better chance at identifying and selecting foci, we

recommend using different cell dilutions.

4. Feed the cells with selective medium every 3-4 days until

cell foci are identified.

5. Pick and transfer colonies to 96- or 48-well plates. Grow

cells to near confluence before expanding to larger wells or

plates.

Zeocin™ Selection in Mammalian Cells, Continued

Selection Tip

If your cells are more resistant to Zeocin™, split cells into medium

containing Zeocin™ and incubate the cells at 37ºC for 2-3 hours to let cells

attach. Place the cells at 4ºC for 2 hours. Remember to buffer the medium

with HEPES. Return the cells to 37ºC.

Incubating the cells at 4°C stops the cell division process for a short time,

allowing Zeocin™ to act, resulting in cell death.

Maintaining Stable Cell Lines

• Maintain cells in the same Zeocin™ concentration used for selection

• Reduce the Zeocin™ concentration by half or to a concentration that

just prevents growth of sensitive cells but does not kill them (refer to

the kill curve experiment)

Product Qualification

Zeocin™ is lot qualified by demonstrating that LB media containing

25 μg/ml Zeocin™ prevents growth of the E. coli strain, TOP10.

Accessory Products

Media for bacteria and mammalian cells as well as transformation

products (yeast and bacteria) and transfection reagents are available from

Invitrogen. Visit www.invitrogen.com for details.

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