Template:SBB-Protocols Assay3: Difference between revisions
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== Procedure == | == Procedure == | ||
===Experimental Group=== | ===Experimental Group=== | ||
<font color="darkturquoise">JCA: Is AgNO3 not AgNO2</font> | <font color="darkturquoise">JCA: Is AgNO3 not AgNO2</font> | ||
| Line 21: | Line 17: | ||
test whether AgNO3 reacts with TBS | test whether AgNO3 reacts with TBS | ||
====Picking and Incubating Colonies==== | ====Picking and Incubating Colonies==== | ||
#Add 4mL of LB media with the appropriate antibiotics | #Add 4mL of LB media with the appropriate antibiotics and arabinose | ||
#Pick a well-isolated, round, and "normal" looking colony | #Pick a well-isolated, round, and "normal" looking colony containing the silver binding peptide with a pipet tip | ||
#Drop it in the test tube | #Drop it in the test tube | ||
#Incubate at 37C overnight | #Incubate at 37C overnight | ||
==== | ====Wash cells and incubate in AgNO3==== | ||
#Pellet 1 mL of saturated culture by spinning full speed, 30 seconds. | #Pellet 1 mL of saturated culture by spinning full speed, 30 seconds. | ||
#Dump supernatant, repeat to pellet another 1 mL (for a total of 2 mL) | #Dump supernatant, repeat to pellet another 1 mL (for a total of 2 mL) | ||
| Line 45: | Line 31: | ||
#Pour out the supernatant | #Pour out the supernatant | ||
#Add 200uL of TBS and resuspend | #Add 200uL of TBS and resuspend | ||
====Treating with Silver==== | ====Treating with Silver==== | ||
| Line 85: | Line 71: | ||
# Wash non-AG4 cells with silver nitrate and look for colour change (tells us if precipitation occurs without AG4)<font color="darkturquoise"> | # Wash non-AG4 cells with silver nitrate and look for colour change (tells us if precipitation occurs without AG4)<font color="darkturquoise"> | ||
# Try growing any functional clones in cultures containing the AgNO3</font> | # Try growing any functional clones in cultures containing the AgNO3</font> | ||
== Procedure carried out on 22 April 2009 == | |||
==== Preparation of Tris buffer solution ==== | |||
* Add 605 mg Tris and 876 mg NaCl to 80 ml H2O | |||
* Adjust pH to 7.4 by adding HCl and bring volume to 100 ml | |||
==== Preparation of AgNO3 solution ==== | |||
* Weigh AgNO3 powder in an Eppendorf tube (weighed 0.013 grams) | |||
* AgNO3 has MW 169.87 g/mol - dilute 0.013g with 0.750ml for ~10 mM solution | |||
* Make 3ml of 1mM solutions by adding 100ul of 10mM AgNO3 into 900ul of H2O | |||
==== Preparation of cells for assay ==== | |||
* Spin down 2ml of cells and throw away supernatant | |||
* Add 200 ul of TBS and resuspend cells | |||
* Spin down the cells and throw away supernatant | |||
==== Preparing cells for growth in LBTAg media ==== | |||
* Dispense 3ml of LB media into 9 chambers in growth rack | |||
* Add 200 ul of Tris buffer solution to the LB media | |||
* Add 32 ul of 10 mM AgNO3 to make 0.1 mM LBTAg media | |||
* Pick cells from each washed pellet (above) and add to corresponding growth chambers | |||
** 11-17 + Control + another one of 11 | |||
* Add 3ul of 1000x Arabinose to the 9th chamber containing a second culture of cells 11 | |||
* Cover the rack and incubate overnight at 37C | |||
==== Running the assay on cells ==== | |||
* Add 180 ul of TBS to each pellet (prepared above) | |||
* Resuspend cells | |||
* Add 20 ul of 1 mM AgNO3 to each TBS/cell-containing tube | |||
* Incubate overnight at room temperature and with agitation | |||
==Procedure 4/30/09== | |||
Follow protocol in yeast paper "Peptide-Mediated Reduction of Silver Ions on Engineered Biological Scaffolds" <br> | |||
<pre> | |||
1. pellet 2ml of cells | |||
2. wash 3X in 1ml water | |||
3. incubate in 1ml aq soln of 1mM AgNO3 for 24-90hrs at room temperature and ambient light with agitation | |||
</pre> | |||
Follow protocol in original (virus) paper <br> | |||
<pre> | |||
1. pellet 2ml of cells | |||
2. wash 2X in 200ul TBS | |||
3. incubate in 900ul of TBS and 100ul 1mM AgNO3 (for constructs 14-17 and control) and in 180ul TBS and 20ul 1mM AgNO3 (for constructs 11-13) for 24-28hrs at room temperature and ambient light with agitation | |||
</pre> | |||
*make new AgNO3 solution (1mM). | |||
*same TBS as before | |||
===Growing Cells in LB and in the presence of arabinose 4/09=== | |||
wash cells with TBS and resuspend it <br> grow a portion of the cells in 4ml LB <br> add 200ul TBS <br> add 0.1mM AgNO3 <br> grow cells overnight <br> hope that AgNO3 does not kill the cells and a color change will occur <br> | |||
one sample (11) also has arabinose in it to test for a difference in expression <br> | |||
Latest revision as of 10:06, 8 May 2009
Silver Biomineralization Assay
Here we present an assay to determine whether the AG4 Silver binding peptide is present in the outer membrane of E.coli.
Procedure
Experimental Group
JCA: Is AgNO3 not AgNO2
pBca9145-Bca1363 as control plasmid.
pBca9145CA- part
test whether AgNO3 reacts with LB test whether AgNO3 reacts with TBS
Picking and Incubating Colonies
- Add 4mL of LB media with the appropriate antibiotics and arabinose
- Pick a well-isolated, round, and "normal" looking colony containing the silver binding peptide with a pipet tip
- Drop it in the test tube
- Incubate at 37C overnight
Wash cells and incubate in AgNO3
- Pellet 1 mL of saturated culture by spinning full speed, 30 seconds.
- Dump supernatant, repeat to pellet another 1 mL (for a total of 2 mL)
- Pour out the supernatant (contains extracellular proteins, unneeded nutrients)
- Add 200uL of TBS (pH 7.4) and resuspend
- Centrifuge the colony solution for 30 seconds
- Pour out the supernatant
- Add 200uL of TBS and resuspend
Treating with Silver
- Make 10mM stock of AgNO3.
- Add 200uL of 0.1 mM silver nitrate and resuspend the cells
- Incubate overnight (24-48 hours) at room temperature
- observe color change and precipitation of colored compound
- Perform same procedure but vary concentration of AgNO3, cell density, and presence of arabinose (see group samples)
Control Group - non-AG4 cells
*note: do controls for each of the sample groups
Picking and Incubating Colonies
- Add 4mL of LB media with the appropriate antibiotics to a clean test tube
- Pick a well-isolated, round, and "normal" looking colony of control E coli with no silver binding peptide with a toothpick
- Drop it in the test tube
- Incubate at 37 overnight
Cleaning
- Pellet 1 mL of saturated culture by spinning full speed, 30 seconds.
- Dump supernatant, repeat to pellet another 1 mL (for a total of 3 mL)
- Pour out the supernatant (contains extracellular proteins, unneeded nutrients)
- Add 1 mL of TBS (pH 7.4) and resuspend
- Centrifuge the colony solution for 30 seconds
- Pour out the supernatant
- Add 200uL of TBS and resuspend
- Dilute an aliquot of the solution 10X. Measure OD of solution using spectrophotometer (at 600nm)
Treating with Silver
- Make 10mM stock of AgNO3
- Add 200uL of 0.1 mM silver nitrate and resuspend the cells JCA: Ammend this step. I think you want to say add 2uL of 10mM AgNO3 stock to 200uL of washed cells and vortext to mix (or something like that).
- Incubate overnight (24-48 hours) at room temperature
- observe color change and precipitation of colored compound
- Perform same procedure but vary concentration of AgNO3, cell density, and presence of arabinose (see group samples)
other controls
- Chemically reduce silver nitrate to precipitate silver (tells us silver nitrate is precipitating)
- Lyse cells over-expressing AG4 and run assay (tells us if AG4 is precipitating silver)
- Wash non-AG4 cells with silver nitrate and look for colour change (tells us if precipitation occurs without AG4)
- Try growing any functional clones in cultures containing the AgNO3
Procedure carried out on 22 April 2009
Preparation of Tris buffer solution
- Add 605 mg Tris and 876 mg NaCl to 80 ml H2O
- Adjust pH to 7.4 by adding HCl and bring volume to 100 ml
Preparation of AgNO3 solution
- Weigh AgNO3 powder in an Eppendorf tube (weighed 0.013 grams)
- AgNO3 has MW 169.87 g/mol - dilute 0.013g with 0.750ml for ~10 mM solution
- Make 3ml of 1mM solutions by adding 100ul of 10mM AgNO3 into 900ul of H2O
Preparation of cells for assay
- Spin down 2ml of cells and throw away supernatant
- Add 200 ul of TBS and resuspend cells
- Spin down the cells and throw away supernatant
Preparing cells for growth in LBTAg media
- Dispense 3ml of LB media into 9 chambers in growth rack
- Add 200 ul of Tris buffer solution to the LB media
- Add 32 ul of 10 mM AgNO3 to make 0.1 mM LBTAg media
- Pick cells from each washed pellet (above) and add to corresponding growth chambers
- 11-17 + Control + another one of 11
- Add 3ul of 1000x Arabinose to the 9th chamber containing a second culture of cells 11
- Cover the rack and incubate overnight at 37C
Running the assay on cells
- Add 180 ul of TBS to each pellet (prepared above)
- Resuspend cells
- Add 20 ul of 1 mM AgNO3 to each TBS/cell-containing tube
- Incubate overnight at room temperature and with agitation
Procedure 4/30/09
Follow protocol in yeast paper "Peptide-Mediated Reduction of Silver Ions on Engineered Biological Scaffolds"
1. pellet 2ml of cells 2. wash 3X in 1ml water 3. incubate in 1ml aq soln of 1mM AgNO3 for 24-90hrs at room temperature and ambient light with agitation
Follow protocol in original (virus) paper
1. pellet 2ml of cells 2. wash 2X in 200ul TBS 3. incubate in 900ul of TBS and 100ul 1mM AgNO3 (for constructs 14-17 and control) and in 180ul TBS and 20ul 1mM AgNO3 (for constructs 11-13) for 24-28hrs at room temperature and ambient light with agitation
- make new AgNO3 solution (1mM).
- same TBS as before
Growing Cells in LB and in the presence of arabinose 4/09
wash cells with TBS and resuspend it
grow a portion of the cells in 4ml LB
add 200ul TBS
add 0.1mM AgNO3
grow cells overnight
hope that AgNO3 does not kill the cells and a color change will occur
one sample (11) also has arabinose in it to test for a difference in expression
