Revision as of 03:48, 1 November 2017

Protocols

Grow Pc. denitrificans cultures in liquid media
Dilute 500mL of Pc. denitrificans culture in 500mL SGM17 medium
***Cold Room from here on***
Harvest by centrifuge 250mL samples each in four centrifuge bottles at 5000xg at 4 C. carefully dump out supernatant
Completely resuspend the pellets(shake side to side to avoid liquid loss) in all centrifuge bottles each with 50mL of 0.5 M sucrose solution with 10% glycerol
Combine the liquid(containing resuspended pellets) into one centrifuge bottle, add appropriate amount of water to the other empty centrifuge bottle for counterbalance
Centrifuge the two bottles at 5000xg at 4 C
Dump out supernatant and resuspend the pellets with 100mL of 0.5 M sucrose solution with 10% glycerol. Counter-balance bottle should have 100mL of water
Centrifuge the two bottles at 5000xg at 4 C
Dump out supernatant and resuspend the resulting pellets in 10mL of 0.5 M sucrose solution with 10% glycerol
Aliquot the final 10mL of liquid into 0.25mL(250uL) with 40 microcentrifuge tubes
Flash freeze with liquid nitrogen and store at -80 C

Thaw and mix 50 uL portions cells with 5 uL DNA
Transfer to ice cold electroporation cuvette
Electroporate with single pulse set at 25 uF and 2.0 kV for 4.5 to 5 ms
The electroporator as a Gene-Pulser by BioRad connected to a 200-(-) resistor also by biorad
IMMEDIATELY following electroporation: carefully mix suspension with 0.95 mL ice cold SGM17 containing 20 mM MgCl2, 2 mM CaCl2 and incubate on ice for 5 minutes
Dilutions were made in the SGM17 media
Incubate cells at 30 C for 2 hours
Take 100 uL portions and plate.

Isolate Single colonies

Select glycerol stock cultures from -80 C storage to begin
Thaw on ice for 15 minutes and observe when the cell stock begins to melt
Take a plastic p-loop or other spreading instrument and spread on a selective media agar plate containing the appropriate antibiotics
Incubate both Pc. denitrificans and E. coli overnight at 37 C
Isolate single colonies after overnight incubation and resuspend in 60 mL volumes of liquid selective LB media with appropriate antibiotics

Preculture for Device Testing

Allow the resuspended liquid culture to incubate for 4 to 6 hours in a shaking incubator at 37 C and 220 rpm to reach late- to mid-exponential phase of growth, look for an OD 600 value of ~0.6
Obtain a 1 mL sample and measure the OD600. If at a satisfactory level, then proceed with device testing
Divide the 60 mL pre-cultures into 3.5 mL aliquots in 14 mL falcon RB tubes or comparable sterile culture tube
Start incubation in a shaking incubator at 37 C and 220 rpm

Device Measurements

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@@ Line 62: / Line 62: @@
 <ul>If using untransformed bacteria, equivalent non-selective media should be used</ul></li>
 <li>Incubate both Pc. denitrificans and E. coli overnight at 37 C
-<li>Isolate single colonies after overnight incubation and resuspend in 60 mL volumes of liquid selective LB media with appropriate antibiotics</li>
+<li>Isolate single colonies after overnight incubation and resuspend in 60 mL volumes of liquid selective LB media with appropriate antibiotics</li></ol>
 <br><br>
@@ Line 74: / Line 74: @@
 <li>Start incubation in a shaking incubator at 37 C and 220 rpm
 <ul>Every hour stop the shaking incubator and cover the next tube with parafilm. Repeat this step until all tubes except the last ones are covered</ul>
-<ul>Allow the final set of tubes to incubate unsealed for an hour and stop the incubation</ul></li>
+<ul>Allow the final set of tubes to incubate unsealed for an hour and stop the incubation</ul></li></ol>
 <br><br>