Team:TU-Delft/Protocol 10

From 2013.igem.org

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<h2 align="center">General Peptide Production</h2>
<h2 align="center">General Peptide Production</h2>
<h4 align="left">Procedure</h4>
<h4 align="left">Procedure</h4>
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<li> In morning, dilute the o/n  cultures  1/50 and follow the OD600 till it reaches 0.5-0.6.</li>
<li> In morning, dilute the o/n  cultures  1/50 and follow the OD600 till it reaches 0.5-0.6.</li>
<li> Induce the cultures with 1mM final concentration of IPTG.  </li>
<li> Induce the cultures with 1mM final concentration of IPTG.  </li>
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<li> After 3 hrs of IPTG induction, 0.1 % of arabinose was added .</li>
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<li> After 3 hrs of induction spin down the cultures at 6000 rpm for 10 min, RT.</li>  
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<li> After 3 hrs of induction spin down the cultures at 6000 rpm for 10 min, RT. </li>
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<li> Re-suspend  the pellet in required amount of french press lysis buffer (give the composition)</li>
<li> Re-suspend  the pellet in required amount of french press lysis buffer (give the composition)</li>
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<li> Disrupt the cells using french press at 24000-26000 psi</li>
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<li> Disrupt the cells using french press at 24000-26000 psi.</li>
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<li> Centrifuge the lysates at 45,000 rpm for 30 min to get rid of the cell debris. Collect the clear lysates and the pellet separately. Snap freeze them with liquid nitrogen  and store the samples at  -800C for further use.
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<li> Centrifuge the lysates at 45,000 rpm for 30 min to get rid of the cell debris. Collect the clear lysates and the pellet separately. Snap freeze them with liquid nitrogen  and store the samples at  -800C for further use.</li>
<li> Run the tricine gels (protocol)</li>
<li> Run the tricine gels (protocol)</li>
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Revision as of 13:44, 1 October 2013



Protocols

Our project deals with E.coli cells which sense Auto-inducing peptides (AIPs) from the Staphylococcus aureus and starts producing Antimicrobial peptides in order to kill the Staphylococcus aureus. Different protocols used during the project are described below.


General Peptide Production

Procedure

  1. Inoculate cells from a plate into 5mL of media. Grow overnight (o/n) at 37°C with rotation at 180 rpm.
  2. In morning, dilute the o/n cultures 1/50 and follow the OD600 till it reaches 0.5-0.6.
  3. Induce the cultures with 1mM final concentration of IPTG.
  4. After 3 hrs of induction spin down the cultures at 6000 rpm for 10 min, RT.
  5. Re-suspend the pellet in required amount of french press lysis buffer (give the composition)
  6. Disrupt the cells using french press at 24000-26000 psi.
  7. Centrifuge the lysates at 45,000 rpm for 30 min to get rid of the cell debris. Collect the clear lysates and the pellet separately. Snap freeze them with liquid nitrogen and store the samples at -800C for further use.
  8. Run the tricine gels (protocol)