BISC220/S13: Mod 2 Media Recipes: Difference between revisions

Revision as of 10:34, 4 March 2013

Wellesley College BISC 220 Cellular Physiology

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Enzymes Secretory Pathway Apoptosis OWW Basics


Solution	Composition
PBS (Phosphate Buffered Saline) 1X	2.68 mM KCl 1.46 mM KH₂PO₄ 136.9 NaCl 8.1 mM Na₂HPO₄
PBST (PBS with Tween 20)	1X PBS with 0.25% Tween 20
YPD (Yeast Peptone Dextrose	1% Yeast Extract 2% Peptone 2% Glucose 2% Agar (only in solid media)
SD (Sabouraud's Dextrose) -Ura	0.67% Yeast Nitrogen Base 2% Glucose 0.08% -Ura amino acid drop out mix 2% Agar (only in solid media)
SD-Ura-His	0.67% Yeast Nitrogen Base 2% Glucose 0.078% -Ura -His amino acid drop out mix 0.003M Histidinol 2% Agar (only in solid media)
Yeast 5X Protein Sample Buffer	10% SDS 25% Glycerol 250mM Tris (pH = 6.8) 500mM DTT 0.5% BPB
Acrylamide Gel Tank Buffer (Gel Running)	0.92 M Glycine 0.05M Trisma base 0.1% SDS
Western Blotting Buffer (Nitrocellulose Transfer)	25mM Trisma Base 192mM Glycine 20% v/v Methanol
Amersham ECL Western Blotting Analysis System	www.gelifesciences.com catalog #RPN2109
Strain Source	Elizabeth Valen at Swarthmore College is the original source of the 3 plasmids and 3 strains Jennifer Hood-DeGrenier at Worchester State is the source of the Mat a strain

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 [[BISC220/S13: Mod 2 Background  | Background Information]]<br>
-[[BISC220/S13: Mod 2 Lab 5  | Lab 5: Phenotypes of Secretory Mutants]]<br>
+[[BISC220/S13: Mod 2 Lab 5  | Lab 6: Phenotypes of Secretory Mutants]]<br>
-[[BISC220/S13: Mod 2 Lab 6  | Lab 6: Analyzing Secretion Defects by Western Blotting]]<br>
+[[BISC220/S13: Mod 2 Lab 6  | Lab 7: Analyzing Secretion Defects by Western Blotting]]<br>
-[[BISC220/S13: Mod 2 Lab 7  | Lab 7: Probing and Detecting the Western Blot]]<br>
+[[BISC220/S13: Mod 2 Lab 7  | Lab 8: Probing and Detecting the Western Blot]]<br>
 [[BISC220/S13: Mod 2 Media Recipes | Media Recipes]]<br>