Revision as of 20:56, 27 October 2008

Protocols

1.) Making Agarose Gel (standard 1%)

Time: ~1 hour

Required:

Gel tank, with combs, casting tray and relevant power supply
Agarose powder
TAE buffer, 1x
Ethidium bromide

Method

1. The gel tank we normally use holds 150ml, therefore, take 150ml of 1x TAE Buffer

2. The gel is supposed to be 10% agarose, therefore we need to add 1.5g agarose powder

3. Combine the two in a chemical screw-cap bottle, and, leaving the lid slightly loose

4. Cook on high heat in the microwave for 2 mins, or until ALL the agarose has dissolved (it may stick to the bottom, swirling may be required. *CAUTION* very hot liquid)

5. If it starts to overboil, pause the microwave, allow to calm down, and continue.

6. When all the agarose has dissolved, remove carefully! Its very hot! Oven gloves may be required.

7. Add 10 µl of ethidium bromide per 100ml of buffer. Swirl to mix. Warning! Ethidium bromide is carcinogenic and therefore very dangerous!

8. Leave until touchably cool before pouring into gel tank. Gently bathe bottle in cold water to speed up the process if necessary.

9. Make sure combs are in place in tank, and casting tray is secured on all sides, then pour in the liquid.

10. Leave until cool (~30 mins)

2.) PCR Purification (Using QIAGEN Kit)

Time: ~1 hour

Required:

PCR Purification kit ideally. Instructions and reagents usually provided

Method

1. Add 5 volumes of PBI buffer (provided) for every 1 volume of PCR product in an eppendorf tube. Make sure one eppendorf is large enough – you may need more.

2. Put mixture in a QIAGEN column (purple) and into a 2ml collection tube (clear)(both provided). Remember, these columns only hold 700µl! Again you may need to repeat steps 3 and 4 more than once.

3. Centrifuge at 10000-13000g for 30-60seconds

4. ‘Flow through’ will be found in the collection tube: discard. The DNA has stuck to the column membrane. Repeat if you had more than 700µl of PCR+PBI buffer to start with

5. The wash DNA of impurities further, add 0.75ml (750µl) of PE buffer (provided)(make sure the ethanol HAS been added to it! You have to do this yourself, but previous users of the kit may have done so and should have labelled the bottle so).

6. Centrifuge for 1 min, and discard flow through.

7. Centrifuge for a further 1min, as not all the PE buffer from the last step could fit in the collection tube.

8. Discard flow through and put column into where you want your eluate (usually 1.5ml eppendorfs)

9. To elute DNA, add 50µl of EB buffer (provided). This ‘unsticks’ the DNA allowing it to be washed through.

10. Centrifuge for 1 min

11. KEEP the flow through! This has your DNA in.

1.) Making SOB Medium

Time: ~20 mins, plus autoclaving time

Required:

EITHER

SOB powder, in which case make up as instructions

OR, per litre

950ml dH20
20g Tryptone
5g Yeast Extract
0.5g NaCl
10ml of 250nM KCl
5ml of 2M MgCl2
~0.2ml 5M NaOH (may be required to adjust PH)

Method

1.) Combine dH2O, tryptone, yeats and NaCl, and shake until combined

2.) Add KCl

3.) Adjust to PH 7.0 with the NaOH

4.) Autoclave (20 mins liquid cycle)

5.) Add the MgCl2 just before use

4.) Making SOC Medium

Method

Same as for SOB above, but add 20mM glucose

@@ Line 1: / Line 1: @@
 =Protocols=
 '''1.) Making Agarose Gel (standard 1%)'''
@@ Line 69: / Line 71: @@
 . KEEP the flow through! This has your DNA in.
+----
+'''1.) Making SOB Medium'''
+Time: ~20 mins, plus autoclaving time
+Required:
+EITHER
+*SOB powder, in which case make up as instructions
+OR, per litre
+* 950ml dH20
+* 20g Tryptone
+* 5g Yeast Extract
+* 0.5g NaCl
+* 10ml of 250nM KCl
+* 5ml of 2M MgCl2
+* ~0.2ml 5M NaOH (may be required to adjust PH)
+''Method''
+.) Combine dH2O, tryptone, yeats and NaCl, and shake until combined
+.) Add KCl
+.) Adjust to PH 7.0 with the NaOH
+.) Autoclave (20 mins liquid cycle)
+.) Add the MgCl2 just before use
+----
+'''4.) Making SOC Medium'''
+''Method''
+Same as for SOB above, but add 20mM glucose

Our Protocols

From 2008.igem.org

Revision as of 20:56, 27 October 2008

Protocols