http://openwetware.org/index.php?title=Mathies:Culture_in_Broth&action=history Revision history for this page on the wiki en MediaWiki 1.13.2 Wed, 19 Jun 2013 19:29:08 GMT http://openwetware.org/index.php?title=Mathies:Culture_in_Broth&diff=327090&oldid=prev <p>New page: <a href="/wiki/Category:Protocol" title="Category:Protocol">Category:Protocol</a> <a href="/wiki/Category:Microfluidics" title="Category:Microfluidics">Category:Microfluidics</a> &lt;!-- COPY EVERYHING BELOW HERE TO START YOUR OWN PROTOCOL! --&gt; ==E. COLI CULTURE IN BROTH AND QUANTIFICATION== '''Reagents''' Bacteri...</p> <p><b>New page</b></p><div>[[Category:Protocol]]<br /> [[Category:Microfluidics]]<br /> <br /> &lt;!-- COPY EVERYHING BELOW HERE TO START YOUR OWN PROTOCOL! --&gt;<br /> <br /> <br /> ==E. COLI CULTURE IN BROTH AND QUANTIFICATION==<br /> <br /> '''Reagents'''<br /> <br /> Bacteria: E. coli strain K12 and O157<br /> <br /> Broth: Tryptic Soy Broth medium (TSB, Hardy Diagnostics K131); Lewis 310 F3, stored 2ml broth per glass tube<br /> <br /> Antibiotic: stock Ampicillin solution with a concentration of 100mg/ml for E. coli strain K12; (Spectramycin solution for E. coli strain O157 with spec resistance gene or constantly test contamination in O157 cells without spec resistance gene by PCR)<br /> <br /> ==Protocol==<br /> <br /> 1) Thoroughly clean the hood with 70% ethanol<br /> <br /> 2) Place the tube of desired cells in the hood to thaw the solution, slightly spin down the cell solution to the bottom of the 500µl tube.<br /> <br /> 3) Transfer 50µl of the cell solution into a 2ml TSB growing medium<br /> <br /> 4) Add 2µl of 100mg/ml ampicillin solution into the K12 grow medium (or 2µl of 100mg/ml spectramycin into the O157 grow medium)<br /> <br /> 5) Do NOT tightly cap the TSB tube so oxygen exchange can be possible, tape the cap and the tube together before putting into the Bioshaker V.BR-36<br /> <br /> 6) Set the temperature to 37˚C and the speed dial pointing almost vertical<br /> <br /> 7) Grow cells in above conditions over night<br /> <br /> The next day<br /> <br /> 8) Transfer the grown cells into a 15ml/high-clarity polypropylene conical tube<br /> <br /> 9) Centrifuge the cells at 3500rpm for 3 minute in eppendorf Centrifuge 5804<br /> <br /> 10) Discard the supernatant and add 2ml filtered PBS, gently suspend the cell solution<br /> <br /> 11) Repeat step 9) and 10) two more times<br /> <br /> 12) Make 10X dilution from the grown cell solution before UV measurement<br /> <br /> 13) Measure OD600 of the 10X dilution using JASCO V-530 UV/VIS spectrophotometer (Use disposal cuvettes, which are placed at the shelf and purchased from LSA stock room with C# of P2180) Average three OD600 measurement values is highly recommended.<br /> <br /> 14) Calculate the concentration of the cell solution using calibration curves (Please see the section of “CALIBRATION CURVE” for details)<br /> <br /> ==Contact==<br /> *'''[[User:Eric Chu|Eric Chu]] 22:25, 22 July 2009 (PDT)''':<br /> <br /> or instead, [[Talk:{{PAGENAME}}|discuss this protocol]]. <br /> <br /> &lt;!-- You can tag this protocol with various categories. See the [[Categories]] page for more information. --&gt;<br /> <br /> [[Category:Protocol]]<br /> [[Category:Microfluidics]]<br /> <br /> <br /> &lt;!-- Move the relevant categories above this line to tag your protocol with the label<br /> [[Category:Protocol]]<br /> <br /> [[Category:Needs attention]]<br /> <br /> [[Category:In vitro]]<br /> <br /> [[Category:In vivo]]<br /> <br /> [[Category:In silico]]<br /> <br /> [[Category:DNA]]<br /> <br /> [[Category:RNA]]<br /> <br /> [[Category:Protein]]<br /> <br /> [[Category:Chemical]]<br /> <br /> [[Category:Escherichia coli]]<br /> <br /> [[Category:Yeast]]<br /> --&gt;</div> Thu, 23 Jul 2009 05:17:29 GMT Eric Chu http://openwetware.org/wiki/Talk:Mathies:Culture_in_Broth