BISC209/S12: Recipes: Difference between revisions
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0.3% Beef extract, 0.5% Peptone- Commercially available and identical to Nutrient agar without the 1.5% solidifying Agar. <BR> | 0.3% Beef extract, 0.5% Peptone- Commercially available and identical to Nutrient agar without the 1.5% solidifying Agar. <BR> | ||
'''Dilute Nutrient Agar''': dilute full strength NA 1:10- 1:300 depending on how much growth reduction you want to achieve | '''Dilute Nutrient Agar''': dilute full strength NA 1:10- 1:300 depending on how much growth reduction you want to achieve. In our experiments we will use a 1:10 dilution of beef extract and peptone= 0.03% beef extract and 0.05% peptone. | ||
'''Gram positive spore forming enrichment:'''<BR> | '''Gram positive spore forming enrichment:'''<BR> | ||
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<UL><LI>'''Glycerol Yeast Extract Agar''' (general enrichment medium for ''Gram positive spore forming bacteria'') | <UL><LI>'''Glycerol Yeast Extract Agar''' (general enrichment medium for ''Gram positive spore forming bacteria'') | ||
0.5% (v/v) Glycerol, 0.2% Yeast Extract, 0.1%Dipotassium phosphate, 1.5% Agar | 0.5% (v/v) Glycerol, 0.2% Yeast Extract, 0.1%Dipotassium phosphate, 1.5% Agar | ||
</LI></UL><BR> | </LI></UL><BR> | ||
'''Nitrogen Cyclers:'''<BR> | '''Nitrogen Cyclers:'''<BR> | ||
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Aseptically combine 1 part of A with 1 part of B (SolutionA:SolutionB=1:1) after autoclaving. Add 0.25 ml filtered multivitamin mix. After autoclaving media will contain some solid material that should be swirled prior to pouring plates.<BR> For solid medium add 2% agar to solution B prior to autoclaving.<BR> | Aseptically combine 1 part of A with 1 part of B (SolutionA:SolutionB=1:1) after autoclaving. Add 0.25 ml filtered multivitamin mix. After autoclaving media will contain some solid material that should be swirled prior to pouring plates.<BR> For solid medium add 2% agar to solution B prior to autoclaving.<BR> | ||
Effective concentrations: 0.08%K<sub>2</sub>HPO<sub>4</sub>; 0.02%KH<sub>2</sub>PO<sub>4</sub>, 0.02% MgSO<sub>4</sub> | Effective concentrations: 0.08%K<sub>2</sub>HPO<sub>4</sub>; 0.02%KH<sub>2</sub>PO<sub>4</sub>, 0.02% MgSO<sub>4</sub> | ||
0.01% CaSO<sub>4</sub>; 0.0015% FeSO<sub>4</sub>/7H<sub>2</sub>O; 0.00025% g MoO<sub>3</sub>; 0.5% mannitol.<BR><BR> | 0.01% CaSO<sub>4</sub>; 0.0015% FeSO<sub>4</sub>/7H<sub>2</sub>O; 0.00025% g MoO<sub>3</sub>; 0.5% mannitol (more selective for ''Azotobacteria''and/or sucrose (less selective).<BR><BR> | ||
</ul> | </ul> | ||
'''Simmons Citrate Medium selects for bacteria (nitrifiers) able extract nitrogen from ammonium (in this case ammonium phosphate) while using citrate as their sole carbon source. The indicator shows a color change from green to blue when an alkaline pH of 7.6 is reached as the ammonium is converted to ammonia.'''<BR> | '''Simmons Citrate Medium selects for bacteria (nitrifiers) able extract nitrogen from ammonium (in this case ammonium phosphate) while using citrate as their sole carbon source. The indicator shows a color change from green to blue when an alkaline pH of 7.6 is reached as the ammonium is converted to ammonia.'''<BR> | ||
0.02% MgSO<sub>4</sub>(Magnesium Sulfate), 0.1% NH<sub>4</sub>H<sub>2</sub>PO<sub>4</sub>(monoammonium phosphate), 0.1% K<sub>2</sub>HPO<sub>4</sub>(dipotassium phosphate), 0.2% C<sub>6</sub>H<sub>5</sub>Na<sub>3</sub>O<sub>7</sub>(sodium citrate), 0.5% NaCl(sodium chloride), 2.5% agar, 0.008% C<sub>27</sub>H<sub>27</sub>Br<sub>2</sub>O<sub>5</sub>SNa(bromothymol blue) at pH6.9 +/-0.2 at 25°C. | 0.02% MgSO<sub>4</sub>(Magnesium Sulfate), 0.1% NH<sub>4</sub>H<sub>2</sub>PO<sub>4</sub>(monoammonium phosphate), 0.1% K<sub>2</sub>HPO<sub>4</sub>(dipotassium phosphate), 0.2% C<sub>6</sub>H<sub>5</sub>Na<sub>3</sub>O<sub>7</sub>(sodium citrate), 0.5% NaCl(sodium chloride), 2.5% agar, 0.008% C<sub>27</sub>H<sub>27</sub>Br<sub>2</sub>O<sub>5</sub>SNa(bromothymol blue) at pH6.9 +/-0.2 at 25°C.<BR> | ||
'''Miscellaneous media and reagents'''<BR><BR> | '''Miscellaneous media and reagents'''<BR><BR> | ||
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'''Cellulose degradation medium''' | '''Cellulose degradation medium''' | ||
<ul><li> | <ul><li> | ||
0.188% ashed, acid washed cellulose powder and 0.02% Congo red in Nutrient Agar (0.3%Beef extract , 0.5% Peptone, 1.5% Agar; at pH 6.6- 7.0 at 25°C. | |||
</LI></UL> | </LI></UL> | ||
<BR> | |||
'''STOCK: Cycloheximide solution (50 mg/ml in 70% ethanol).''' <br> cycloheximide inhibits the growth of eukaryotic cells (e.g. fungi). It inhibits protein biosynthesis by interfering with peptidyl transferase activity of the 60S ribosome, preventing protein elongation. Use caution when working with cycloheximide. | '''STOCK: Cycloheximide solution (50 mg/ml in 70% ethanol).''' <br> cycloheximide inhibits the growth of eukaryotic cells (e.g. fungi). It inhibits protein biosynthesis by interfering with peptidyl transferase activity of the 60S ribosome, preventing protein elongation. Use caution when working with cycloheximide. | ||
Unless otherwise indicated,dilute stock to 1mg/ml final concentration in medium. | Unless otherwise indicated,dilute stock to 1mg/ml final concentration in medium. | ||
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''' | '''Phosphate Buffered Saline (PBS):'''<BR> | ||
0.8% NaCl, 0.2% KCl, 0.143% Na2HPO4, 0.024% KH2PO4<BR><BR> | 0.8% NaCl, 0.2% KCl, 0.143% Na2HPO4, 0.024% KH2PO4<BR><BR> | ||
| Line 73: | Line 68: | ||
<UL><LI> Bacto-tryptone 1%; yeast extract 0.5%; NaCl 1.0% at pH 7.5 </LI></UL> | <UL><LI> Bacto-tryptone 1%; yeast extract 0.5%; NaCl 1.0% at pH 7.5 </LI></UL> | ||
''' | '''Mannitol Nitrate Motility Soft Agar (MNM)'''<BR> | ||
<UL><LI> | <UL><LI> | ||
Casein Peptone (1% wt/vol), Mannitol (0.75%), Potassium Nitrate (KNO<sup>3</sup>) (0.1%), Phenol Red (0.004%), Agar (.035%) Final ph 7.6 +/-0.2 at 25C | |||
</LI></UL> | </LI></UL> | ||
<div class=noprint> | <div class=noprint> | ||
==Links to Labs== | ==Links to Labs== | ||
[[BISC209/S12: Lab1 | Lab 1 ]]<br> | [[BISC209/S12: Lab1 | Lab 1 ]]<br> | ||
Latest revision as of 05:53, 24 January 2012
Media Recipies
Nutrient Agar: A general purpose solid medium
0.3% Beef extract, 0.5% Peptone, 1.5% agar, pH 6.8 at 25°C. This medium is commercially available from BD Difco.
Nutrient Broth: A general purpose liquid medium.
0.3% Beef extract, 0.5% Peptone- Commercially available and identical to Nutrient agar without the 1.5% solidifying Agar.
Dilute Nutrient Agar: dilute full strength NA 1:10- 1:300 depending on how much growth reduction you want to achieve. In our experiments we will use a 1:10 dilution of beef extract and peptone= 0.03% beef extract and 0.05% peptone.
Gram positive spore forming enrichment:
- Glycerol Yeast Extract Agar (general enrichment medium for Gram positive spore forming bacteria) 0.5% (v/v) Glycerol, 0.2% Yeast Extract, 0.1%Dipotassium phosphate, 1.5% Agar
Nitrogen Cyclers:
Azotobacteria enrichment medium (selects for bacteria able to fix nitrogen (ammonifiers) and to use mannitol as their sole carbon source)
- Azotobacter N-Free Media (1 L)
Solution A: 0.16% K2HPO4:0.04% KH2PO4
Solution B: 0.04% MgSO4; 0.02% CaSO4; 0.0006% FeSO4/7H2O; 0.0002% MoO3; 1.0% mannitol.
Aseptically combine 1 part of A with 1 part of B (SolutionA:SolutionB=1:1) after autoclaving. Add 0.25 ml filtered multivitamin mix. After autoclaving media will contain some solid material that should be swirled prior to pouring plates.
For solid medium add 2% agar to solution B prior to autoclaving.
Effective concentrations: 0.08%K2HPO4; 0.02%KH2PO4, 0.02% MgSO4 0.01% CaSO4; 0.0015% FeSO4/7H2O; 0.00025% g MoO3; 0.5% mannitol (more selective for Azotobacteriaand/or sucrose (less selective).
Simmons Citrate Medium selects for bacteria (nitrifiers) able extract nitrogen from ammonium (in this case ammonium phosphate) while using citrate as their sole carbon source. The indicator shows a color change from green to blue when an alkaline pH of 7.6 is reached as the ammonium is converted to ammonia.
0.02% MgSO4(Magnesium Sulfate), 0.1% NH4H2PO4(monoammonium phosphate), 0.1% K2HPO4(dipotassium phosphate), 0.2% C6H5Na3O7(sodium citrate), 0.5% NaCl(sodium chloride), 2.5% agar, 0.008% C27H27Br2O5SNa(bromothymol blue) at pH6.9 +/-0.2 at 25°C.
Miscellaneous media and reagents
Hydrocarbon minimal salts broth
(source: Scott, Christina, C.L., and W.R. Finnerty. 1975. A comparative Analysis of the Ultrastructure of Hydrocarbon-oxidizing Micro-organisms. J. of GEn. Micro. 94, 342-350.)
- 0.2% (NH4)2SO4, 0.4% KH2PO4, 0.4% Na2HPO4 0.02% MgSo47H2, 0.0001%CaCl2, 0.0001% FeSO47H2O, pH 7.8.
- Supplement this medium with the desired hydrocarbons. e.g. 0.5% (v/v) hexadecane for Acinetobacter sp., 1%(v/v) hexadecane Arthrobacter sp, or Corynebacterium.
Cellulose degradation medium
- 0.188% ashed, acid washed cellulose powder and 0.02% Congo red in Nutrient Agar (0.3%Beef extract , 0.5% Peptone, 1.5% Agar; at pH 6.6- 7.0 at 25°C.
STOCK: Cycloheximide solution (50 mg/ml in 70% ethanol).
cycloheximide inhibits the growth of eukaryotic cells (e.g. fungi). It inhibits protein biosynthesis by interfering with peptidyl transferase activity of the 60S ribosome, preventing protein elongation. Use caution when working with cycloheximide.
Unless otherwise indicated,dilute stock to 1mg/ml final concentration in medium.
Phosphate Buffered Saline (PBS):
0.8% NaCl, 0.2% KCl, 0.143% Na2HPO4, 0.024% KH2PO4
Pourite: An antifoaming agent used to prevent bubbles in agar containing media that is not commercially available
This agent helps reduce foaming and bubbles when pouring agar plates. One drop for volumes up to 800 ml and 2 drops up to 1 liter. Purchase this from American Scientific Products.
Additional Misc. Reagents & Media Recipes
Luria Bertoni Broth
- Bacto-tryptone 1%; yeast extract 0.5%; NaCl 1.0% at pH 7.5
Mannitol Nitrate Motility Soft Agar (MNM)
- Casein Peptone (1% wt/vol), Mannitol (0.75%), Potassium Nitrate (KNO3) (0.1%), Phenol Red (0.004%), Agar (.035%) Final ph 7.6 +/-0.2 at 25C
