Team:Reading/Protocols

From 2014.igem.org

(Difference between revisions)
Line 4: Line 4:
<table cellpadding=4 cellspacing=0>
<table cellpadding=4 cellspacing=0>
 +
 +
 +
<tr>
 +
<td>
 +
 +
<!--Protocols  -->
 +
<tr><td><h3><font color="#558e2b"> A note on protocols </font></h3></td>
 +
<td></td>
 +
<td> <h3 id="intro"><font color="#558e2b"> Contents </font></h3></td>
 +
</tr>
 +
 +
<!-- Introduction to the Protocols Page -->
 +
<tr>
 +
<td width="45%"  valign="top">
 +
<p><font color="#292929">
 +
A little introduction to our protocols: stuff you need to know, like that we often tweak these protocols in our lab books.
 +
</font></p>
<br>
<br>
-
<br>
+
</td>
-
<br>
+
 
-
<br>
+
<td></td>
-
<h1><b><center><font size="6" color="red">DO NOT EDIT THIS PAGE. GO TO THE GOOGLE DOC</font></b></h1>
+
<td  width="45%"  valign="top">
-
<br>
+
 
-
<br>
+
<!-- Contents - add stuff here to add to the contents page -->
-
<br>
+
<ol>
-
<br>
+
<li><a href="#intro">A Note on Protocols</a></li>
 +
<li><a href="#protocols">The Goods</a></li>
 +
<ul>
 +
    <li><a href="#exampleone">Example one</a></li>
 +
    <li><a href="#exampletwo">Example two</a></li>
 +
</ul>
 +
<li><a href="#acknowledge">Acknowledgements</a></li>
 +
<li><a href="#references">References</a></li>
 +
</ol>
 +
 
 +
</td>
 +
 
 +
</tr>
 +
 
 +
<!-- Spacer line-->
 +
<tr> <td colspan="3"  height="15px"> </td></tr>
 +
<tr><td bgColor="#CCCCCC" colspan="3" height="1px"> </tr>
 +
<tr> <td colspan="3"  height="5px"> </td></tr>
 +
 
 +
<!-- The Protocols -->
 +
<tr>
 +
<td colspan="3"><h3 id="protocols"> <font color="#558e2b">The Goods</font> </h3>
 +
<p bgColor=B2E592><font color="#292929">
 +
Here are all of the protocols.
 +
 
 +
<!-- Miniprep -->
 +
<br />
 +
<br />
 +
<p id="exampleone"><font color="#558e2b"><i>Isolation of plasmid DNA from bacteria (miniprep)</i></font></p>
 +
<p><font color="#292929">
 +
<ol>
 +
  <li>Pellet bacterial cells by centrifuging 1.5 ml of culture in a 1.5 ml microcentrifuge tube at 4000 rpm for 2 minutes
 +
  <li>Discard supernatant by pipetting off ensuring not to disturb the pellet
 +
  <li>Resuspend in 250 µl of resuspension solution by vortexing or pipetting up and down. Do not incubate for more than 5 minutes
 +
  <li>Add 350 µl of neutralisation solution and mix by inverting the tube 4-6 times
 +
  <li>Centrifuge at 13,000 rpm for 5 minutes
 +
  <li>Transfer supernatant to a GeneJET spin column by pipetting. Do not disturb the white precipitate
 +
  <li>Centrifuge the GeneJET spin column for 1 minute at 13,000 rpm
 +
  <li>Discard the flow through
 +
  <li>Add 500 µl of wash solution to the column
 +
  <li>Centrifuge for 1 minute at 13,000 rpm
 +
  <li>Discard flow through
 +
  <li>Add 500 µl of wash solution to the column
 +
  <li>Centrifuge for 1 minute at 13,000 rpm
 +
  <li>Discard flow through
 +
  <li>Centrifuge for 1 minute at 13,000 rpm
 +
  <li>Transfer the GeneJET column to a new 1.5 ml microcentrifuge tube
 +
  <li>Add 35 µl of ultrapure water. Do not touch the membrane with the pipette
 +
  <li>Incubate at room temperature for 2 minutes
 +
  <li>Centrifuge for 2 minutes at 13,000 rpm
 +
</ol>
 +
</font></p>
 +
 
 +
<!-- Glycerol Stock -->
 +
<br />
 +
<p id="exampletwo"><font color="#558e2b"><i>Making glycerol stock</i></font></p>
 +
<p><font color="#292929">
 +
<p>This protocol is adapted from 2 freely available protocols<sup><a href=”#Reference1”>1</a>, <a href=”#Reference2”>2</a></sup>. Ignore steps 2-4 if antibiotic was not present in the overnight broth. Work in a sterile cabinet
 +
<ol>
 +
  <li>Take 0.5 ml from overnight culture and transfer to a centrifuge using sterile DNAase/RNAase free tips
 +
  <li>Centrifuge at 13,000 rpm for 2 minutes
 +
  <li>Discard supernatant
 +
  <li>Add 0.5 ml of 60% glycerol stock
 +
  <ol style="list-style: lower-roman outside">
 +
    <li>240 ml of glycerol
 +
    <li>160 ml nano pure water
 +
    <li>mix together and autoclave
 +
  </ol>
 +
  <li>freeze at -80℃
 +
</ol >
 +
</font></p>
 +
 
 +
<!-- Optical Density -->
 +
<br />
 +
<p id="exampletwo"><font color="#558e2b"><i>Taking optical density of culture</i></font></p>
 +
<p><font color="#292929">
 +
<p>Recommendation for taking OD for monitoring growth is either OD<sub>730</sub><sup><a href=”Reference3”>3</a></sup> or OD<sub>750</sub><sup><a href=”#Reference4”>4</a></sup>. Some recommend taking OD<sub>730</sub> at no higher than 0.4 because of problems with light scattering<sup>REFERENCE</sup>. We chose to measure at growth OD<sub>750</sub> to keep in line with other high-profile papers on Synechocystis<sup>4</sup>.
 +
<ol>
 +
<li>Set spectrophotometer to measure at OD<sub>750</sub>
 +
<li>Blank with 1 ml of BG-11 in a cuvette
 +
<li>Measure 1 ml of culture
 +
<li>If OD is over 1 dilute the 235 ul of culture in 750 ul of BG-11
 +
</ol>
 +
<p>Converting OD<sub>750</sub> to cell density For conversion of cell densities to numbers of cells, we have used the relationship OD750 = 1 (a.u) corresponding to 1.6 x 108 cells mL<sup>-1 5</sup>.
 +
<p>
 +
</font></p>
 +
 
 +
<!-- PCR -->
 +
<br />
 +
<p id=“PCR”><font color="#558e2b"><i>PCR</i></font></p>
 +
<p><font color="#292929">
 +
<p>PCR was used as a means of amplifying each one of our biobrick constructs. Each construct, along with its corresponding flanking sequence of 50-100 bases, was amplified out of each transformed pSB1C3 plasmid.
 +
<p> Prior to PCR, it was ensured that all DNA obtained from miniprep was of a concentration of at least 1ng/ul per 100bp; this was performed using a desktop ThermoScientific NanoDrop machine. All PCR tubes were kept on ice prior to usage.
 +
<p>2μl of each of the VFR (forward) and VR (reverse) primers were added to sterile PCR tubes, along with 2μl of each respective transformed plasmid and 14μl phusion mastermix <sup>REFERENCE</sup>
 +
<p>PCR program program as follows:
 +
<ol>
 +
<li> Start:
 +
<ul>
 +
<il>95℃ for 30 seconds
 +
</ul>
 +
<li>35 cycles:
 +
<ul>
 +
95℃ for 10 seconds
 +
56℃ for 15 seconds
 +
72℃ for 70 seconds
 +
</ul>
 +
<li>Final
 +
<ul>
 +
72℃ for 5 minutes
 +
68℃ for 10 minutes
 +
</ul>
 +
</ol>
 +
<p>All PCR products were cleaned up using a ThermoScientific GeneJET PCR Purification Kit, using the provided protocol<sup>REFERENCE</sup>
 +
 
 +
</font></p>
 +
 
 +
<!-- Transformation into E. coli -->
 +
<br />
 +
<p id="exampletwo"><font color="#558e2b"><i>Transformation into E. coli</i></font></p>
 +
<p><font color="#292929">
 +
<p>
 +
<ol>
 +
<li>Thaw tubes of competent cells on ice and transfer 50 ul to a pre-chilled 1.5 ml Eppendorf
 +
<li>Add 5 ul of DNA using a sterile pipette tip
 +
<li>Flick the tubes to mix and then store on ice for 30 minutes
 +
<li>Heat shock in a water bath at 42℃ for 1 minute
 +
<li>Incubate on ice for 5 minutes
 +
<li>Add 450 ul of SOC (we used LB instead)
 +
<li>Place tubes horizontally at 37℃ for 2 hours on a shaker at 250 rpm
 +
<li>Invert Eppendorfs containing the cells several times
 +
<li>Plate out and incubate overnight at 37℃
 +
</ol>
 +
<p> Notes on transformation efficency
 +
<p>Expected transformation efficiency is 1 x 10<sup>6</sup> cfu/ug of pUC19 DNA, but we should expect a 2-fold decrease in efficiency due to use of LB instead of SOC (a derivative of super optimal broth, SOB). We should also expect a decrease because we thawed the frozen competent cells at a temperature above 0ºC. Ideally they should be thawed on ice, or by hand if needed <sup>REFERENCE</sup>.
 +
</font></p>
 +
 
 +
<!-- Nanodrop -->
 +
<br />
 +
<p id="exampletwo"><font color="#558e2b"><i>Nanodrop</i></font></p>
 +
<p><font color="#292929">
 +
<p>Nanodrop is used to check concentration in DNA often from a miniprep
 +
<ol>
 +
<li>Set the Nanodrop to measure DNA
 +
<li>Blank the Nanodrop by placing 2 ul of PCR water on the stage and pressing blank
 +
<li>Add 2 ul of sample and measure. Measurement should be in ng/ul
 +
</ol>
 +
</font></p>
 +
 
 +
<!-- BG-11 plates -->
 +
<br />
 +
<p id="exampletwo"><font color="#558e2b"><i>Selection plates</i></font></p>
 +
<p><font color="#292929">
 +
<p>BG-11 plates are used to grow Cyanobacteria. Antibiotics are added as needed for selection. 1.5% agar is used.
 +
<ol>
 +
<li>Add 7.55 g of agar to 500 ml BG-11 and autoclave to sterilise
 +
<li>If making kanamycin plates cool to ~55℃ and add 50 ug/ml
 +
<li>Agar melted in steamer and kept at 55℃ until needed for pouring
 +
</ol>
 +
<p> If making a kanamycin cap:
 +
<ol>
 +
<li>0.6% agar w/v
 +
<li>Cool BG-11 to ~55ºC and add 0.5mg/ml kan
 +
<li>Add ~3ml to a plain BG-11 plate with transformed colonies on it
 +
<li>Leave for >1 week for Kan selection to occur
 +
</font></p>
 +
 
 +
<!-- Spacer line-->
 +
<tr> <td colspan="3"  height="15px"> </td></tr>
 +
<tr><td bgColor="#CCCCCC" colspan="3" height="1px"> </tr>
 +
<tr> <td colspan="3"  height="5px"> </td></tr>
 +
 
 +
<!-- Cyanobacteria Transformation -->
 +
<br />
 +
<p id="exampletwo"><font color="#558e2b"><i>Cyanobacteria Transformation</i></font></p>
 +
<p><font color="#292929">
 +
<p>Protocol to transform DNA into cyanobacteria
 +
<ol>
 +
<li>Make a fresh culture to OD<sub>730</sub>=0.2 to 0.3 and grow for 3 days
 +
<li>Centrifuge 1.5 ml of culture at 4000g for 10 min. Remove supernatant
 +
<li>Repeat step 2
 +
<li>Add 1 ml BG-11, resuspend to wash, centrifuge at 4000g for 10 min, remove supernatant
 +
<li>Add 200ml fresh BG-11
 +
<li>4ug plasmid A DNA is added (at a concentration of at least 100ng/ul)
 +
<li>Incubate for 24 under light on a shaker at ~100 rpm
 +
<li>Plate the full 200ml and leave for 1-2 days
 +
<li>Add 3-4ml kan 0.6% agar BG-11
 +
<li>Leave under light for >1 week
 +
</ol>
 +
</font></p>
 +
 
 +
<!-- References Section -->
 +
<tr>
 +
<td colspan="3"><h3 id="references"><font color="#558e2b">References</font></h3>
 +
<p><font color="#292929">
 +
<a href=”Reference1”><p>1. http://www.people.vcu.edu/~pli/Protocols/Plasmid%20Preparation.pdf</a>
 +
<a href=”Reference2”><p>2. http://openwetware.org/wiki/Making_a_long_term_stock_of_bacteria</a>
 +
<a href=”Reference3”><p>3. Eaton-Rye, J. J. in Photosynth. Res. Protoc. 295–312 (Humana Press, 2011). At <http://link.springer.com/protocol/10.1007/978-1-60761-925-3_22>. Accessed 20/08/2014.</a>
 +
<a href=”Reference4”><p>4. Bradley, R. W., Bombelli, P., Lea-Smith, D. J. & Howe, C. J. Terminal oxidase mutants of the cyanobacterium Synechocystis sp. PCC 6803 show increased electrogenic activity in biological photo-voltaic systems. Phys. Chem. Chem. Phys. PCCP 15, 13611–13618 (2013).</a>
 +
<p>5. Pojidaeva E, Zichenko V, Shestakov SV, Sokolenko A (2004) Involvement of the SppA1 peptidase in acclimation to saturating light intensities in Synechocystis sp. strain PCC 6803. J Bacteriol 186: 3991–3999.
 +
</font></p>
 +
</td>
 +
</tr>
 +
 
 +
<!-- Spacer line-->
 +
<tr> <td colspan="3"  height="15px"> </td></tr>
 +
<tr><td bgColor="#CCCCCC" colspan="3" height="1px"> </tr>
 +
<tr> <td colspan="3"  height="5px"> </td></tr>
 +
 
 +
<!-- Acknowledgements section -->
 +
<tr>
 +
<td colspan="3"><h3 id="acknowledge"><font color="#558e2b">Acknowledgements</font></h3>
 +
<p><font color="#292929">
 +
Everyone we need to thank for help with protocols.
 +
</font></p>
 +
</td>
 +
</tr>
 +
 
 +
</table>
 +
</td>
 +
</tr>
 +
 
</html>
</html>
{{Tail}}
{{Tail}}

Revision as of 23:20, 14 October 2014

University of Reading
Home Team Project Fuel Cell Parts Human Practices Lab book Protocols Attributions


Cyanobacteria Transformation

Protocol to transform DNA into cyanobacteria

  1. Make a fresh culture to OD730=0.2 to 0.3 and grow for 3 days
  2. Centrifuge 1.5 ml of culture at 4000g for 10 min. Remove supernatant
  3. Repeat step 2
  4. Add 1 ml BG-11, resuspend to wash, centrifuge at 4000g for 10 min, remove supernatant
  5. Add 200ml fresh BG-11
  6. 4ug plasmid A DNA is added (at a concentration of at least 100ng/ul)
  7. Incubate for 24 under light on a shaker at ~100 rpm
  8. Plate the full 200ml and leave for 1-2 days
  9. Add 3-4ml kan 0.6% agar BG-11
  10. Leave under light for >1 week

A note on protocols

Contents

A little introduction to our protocols: stuff you need to know, like that we often tweak these protocols in our lab books.


  1. A Note on Protocols
  2. The Goods
  3. Acknowledgements
  4. References

The Goods

Here are all of the protocols.

Isolation of plasmid DNA from bacteria (miniprep)

  1. Pellet bacterial cells by centrifuging 1.5 ml of culture in a 1.5 ml microcentrifuge tube at 4000 rpm for 2 minutes
  2. Discard supernatant by pipetting off ensuring not to disturb the pellet
  3. Resuspend in 250 µl of resuspension solution by vortexing or pipetting up and down. Do not incubate for more than 5 minutes
  4. Add 350 µl of neutralisation solution and mix by inverting the tube 4-6 times
  5. Centrifuge at 13,000 rpm for 5 minutes
  6. Transfer supernatant to a GeneJET spin column by pipetting. Do not disturb the white precipitate
  7. Centrifuge the GeneJET spin column for 1 minute at 13,000 rpm
  8. Discard the flow through
  9. Add 500 µl of wash solution to the column
  10. Centrifuge for 1 minute at 13,000 rpm
  11. Discard flow through
  12. Add 500 µl of wash solution to the column
  13. Centrifuge for 1 minute at 13,000 rpm
  14. Discard flow through
  15. Centrifuge for 1 minute at 13,000 rpm
  16. Transfer the GeneJET column to a new 1.5 ml microcentrifuge tube
  17. Add 35 µl of ultrapure water. Do not touch the membrane with the pipette
  18. Incubate at room temperature for 2 minutes
  19. Centrifuge for 2 minutes at 13,000 rpm


Making glycerol stock

This protocol is adapted from 2 freely available protocols1, 2. Ignore steps 2-4 if antibiotic was not present in the overnight broth. Work in a sterile cabinet

  1. Take 0.5 ml from overnight culture and transfer to a centrifuge using sterile DNAase/RNAase free tips
  2. Centrifuge at 13,000 rpm for 2 minutes
  3. Discard supernatant
  4. Add 0.5 ml of 60% glycerol stock
    1. 240 ml of glycerol
    2. 160 ml nano pure water
    3. mix together and autoclave
  5. freeze at -80℃


Taking optical density of culture

Recommendation for taking OD for monitoring growth is either OD7303 or OD7504. Some recommend taking OD730 at no higher than 0.4 because of problems with light scatteringREFERENCE. We chose to measure at growth OD750 to keep in line with other high-profile papers on Synechocystis4.

  1. Set spectrophotometer to measure at OD750
  2. Blank with 1 ml of BG-11 in a cuvette
  3. Measure 1 ml of culture
  4. If OD is over 1 dilute the 235 ul of culture in 750 ul of BG-11

Converting OD750 to cell density For conversion of cell densities to numbers of cells, we have used the relationship OD750 = 1 (a.u) corresponding to 1.6 x 108 cells mL-1 5.


PCR

PCR was used as a means of amplifying each one of our biobrick constructs. Each construct, along with its corresponding flanking sequence of 50-100 bases, was amplified out of each transformed pSB1C3 plasmid.

Prior to PCR, it was ensured that all DNA obtained from miniprep was of a concentration of at least 1ng/ul per 100bp; this was performed using a desktop ThermoScientific NanoDrop machine. All PCR tubes were kept on ice prior to usage.

2μl of each of the VFR (forward) and VR (reverse) primers were added to sterile PCR tubes, along with 2μl of each respective transformed plasmid and 14μl phusion mastermix REFERENCE

PCR program program as follows:

  1. Start:
      95℃ for 30 seconds
  2. 35 cycles:
      95℃ for 10 seconds 56℃ for 15 seconds 72℃ for 70 seconds
  3. Final
      72℃ for 5 minutes 68℃ for 10 minutes

All PCR products were cleaned up using a ThermoScientific GeneJET PCR Purification Kit, using the provided protocolREFERENCE


Transformation into E. coli

  1. Thaw tubes of competent cells on ice and transfer 50 ul to a pre-chilled 1.5 ml Eppendorf
  2. Add 5 ul of DNA using a sterile pipette tip
  3. Flick the tubes to mix and then store on ice for 30 minutes
  4. Heat shock in a water bath at 42℃ for 1 minute
  5. Incubate on ice for 5 minutes
  6. Add 450 ul of SOC (we used LB instead)
  7. Place tubes horizontally at 37℃ for 2 hours on a shaker at 250 rpm
  8. Invert Eppendorfs containing the cells several times
  9. Plate out and incubate overnight at 37℃

Notes on transformation efficency

Expected transformation efficiency is 1 x 106 cfu/ug of pUC19 DNA, but we should expect a 2-fold decrease in efficiency due to use of LB instead of SOC (a derivative of super optimal broth, SOB). We should also expect a decrease because we thawed the frozen competent cells at a temperature above 0ºC. Ideally they should be thawed on ice, or by hand if needed REFERENCE.


Nanodrop

Nanodrop is used to check concentration in DNA often from a miniprep

  1. Set the Nanodrop to measure DNA
  2. Blank the Nanodrop by placing 2 ul of PCR water on the stage and pressing blank
  3. Add 2 ul of sample and measure. Measurement should be in ng/ul


Selection plates

BG-11 plates are used to grow Cyanobacteria. Antibiotics are added as needed for selection. 1.5% agar is used.

  1. Add 7.55 g of agar to 500 ml BG-11 and autoclave to sterilise
  2. If making kanamycin plates cool to ~55℃ and add 50 ug/ml
  3. Agar melted in steamer and kept at 55℃ until needed for pouring

If making a kanamycin cap:

  1. 0.6% agar w/v
  2. Cool BG-11 to ~55ºC and add 0.5mg/ml kan
  3. Add ~3ml to a plain BG-11 plate with transformed colonies on it
  4. Leave for >1 week for Kan selection to occur

References

1. http://www.people.vcu.edu/~pli/Protocols/Plasmid%20Preparation.pdf

2. http://openwetware.org/wiki/Making_a_long_term_stock_of_bacteria

3. Eaton-Rye, J. J. in Photosynth. Res. Protoc. 295–312 (Humana Press, 2011). At . Accessed 20/08/2014.

4. Bradley, R. W., Bombelli, P., Lea-Smith, D. J. & Howe, C. J. Terminal oxidase mutants of the cyanobacterium Synechocystis sp. PCC 6803 show increased electrogenic activity in biological photo-voltaic systems. Phys. Chem. Chem. Phys. PCCP 15, 13611–13618 (2013).

5. Pojidaeva E, Zichenko V, Shestakov SV, Sokolenko A (2004) Involvement of the SppA1 peptidase in acclimation to saturating light intensities in Synechocystis sp. strain PCC 6803. J Bacteriol 186: 3991–3999.

Acknowledgements

Everyone we need to thank for help with protocols.

Facebook
Twitter
rusynbioigem@gmail.com