Team:Warsaw/Calendar-Main/3 September 2008

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Revision as of 22:33, 5 October 2008


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Samples were resuspended in PBS, sonicated and centrifuged.
Lysis buffer were added separately to pellet and supernatant, then samples were boiled for 10 minutes.
Lysates loaded on 12% poliacrylamide gel (amount relating to 100 ul of OD=1,0 culture)
Gel stained with Coomassie Blue. Optimal induction conditions chosen
A-alpha, Z-alpha and Z-omega inoculated in the overnight culture (Rosetta strain)

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+<html>
+<h3>Purification of proteins:  A-alpha, Z-alpha and Z-omega<br>Piotr</h3>
+<p><ol><li>Samples were resuspended in PBS, sonicated and centrifuged.</li>
+<li>Lysis buffer were added separately to pellet and supernatant, then samples were boiled for 10 minutes. </li>
+<li>Lysates loaded on 12% poliacrylamide gel (amount relating to 100 ul of OD=1,0 culture)</li>
+<li>Gel stained with Coomassie Blue. Optimal induction conditions chosen</li>
+<li>A-alpha, Z-alpha and Z-omega inoculated in the overnight culture (Rosetta strain)</p>
+</html>
-Oczyszczanie białek: A-alfa, Z-alfa i Z-omega
-Piotr
-zawieszenie próbek w PBS, sonikacja, zwirowanie, do supernatantu i osadu osobno dodanie buforu lizującego (opisać skład gdzieś) gotować przez 10 minut, na żel poliakryl 12% (zrobić protokół) nałożyć  ilość zlizowanych bakterii odpowiadającą 100mikrolitrom chodowli o OD=1, elektroforeza (zrobić protokół), barwienie i odbarwianie qmasim (zrobić protokuł)
-wybranie optymalnych warunków
-zaszczepienie A-alfa, Z-alfa i Z-omega
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