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Team:Macquarie Australia/Protocols/SDS Page
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(Created page with "{{Team:Macquarie_Australia/Style2}} {{Team:Macquarie_Australia/Header}} <center> <h1>SDS Page</h1> </center> Pelleted cells were resuspended in 200 uL Milli-Q H2O. Transferr...") |
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| - | Pelleted cells | + | [[File:800px-Stain_for_SDS-PAGE_gel.jpg|500px|thumb|left|SDS-Page, image by Andra MIhali]] |
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| + | <b>1)</b> Resuspend Pelleted cells in 200 uL Milli-Q H2O. | ||
| - | + | <b>2)</b> Transfer 50 uL of suspension into new Eppendorf tubes and combined with 50 uL 2x TruSep sample buffer. | |
| - | Using a Hamilton syringe, the cells | + | <b>3)</b> Using a Hamilton syringe, shear the cells. |
| - | + | <b>4)</b> Centrifuge the preparations for 3 mins @ 13,000 rpm. | |
| - | + | <b>5)</b> Load 20 uL of the supernatant in to the gel. | |
| - | + | <b>6)</b> Conduct electrophoresis at a constant voltage (200 V) for one hour. | |
Latest revision as of 06:29, 13 September 2013
SDS Page
1) Resuspend Pelleted cells in 200 uL Milli-Q H2O.
2) Transfer 50 uL of suspension into new Eppendorf tubes and combined with 50 uL 2x TruSep sample buffer.
3) Using a Hamilton syringe, shear the cells.
4) Centrifuge the preparations for 3 mins @ 13,000 rpm.
5) Load 20 uL of the supernatant in to the gel.
6) Conduct electrophoresis at a constant voltage (200 V) for one hour.
