Team:HokkaidoU Japan/Protocols
From 2010.igem.org
=Protocols=
==Contents==
* Preparation of Competent cells (''E. coli'' DH5a)
* Bacterial Transformations
* Mini-prep (Alkaline SDS Method)
* PCR
* Restriction Enzyme Digestions
* DNA ligation
* Agarose gel electrophoresis
* Electroporation
==Preparation of Competent cells (''E. coli'' DH5a)==
===Reagents===
'''TB (Transformation Buffer)(at 4C, filtration)'''
{|border="1" class="protocol"
|
|
|Final concentration
|-
|1 M CaCl2 (at RT, autoclaved)
|0.75 mL
|15 mM
|-
|4 M KCl (at RT, autoclaved)
|3.125 mL
|250 mM
|-
|1 M MnCl2 (at 4C, autoclaved)
|2.75 mL
|55 mM
|-
|1 M PIPES (pH 6.7 by NaOH, at 4C, filtration)
|0.5 mL
|10 mM
|-
|'''Total'''
|'''50 mL'''
|
|}
filtration (0.2 um), store at 4C
===Method===
# Single colony isolation on LB plate
# incubate the plate for 15-19 hrs at 37C
# lift a colony into 2 mL of LB
# culture cells at 37C for 12-16 hrs at 180-200 rpm
# transfer 30 uL, 100 uL, 300 uL of the culture into 100 mL SOB medium, respectively
# culture cells at 20C (for 24 hrs over) at 180-200 rpm (to ΔOD550nm = 0.5~0.6)
# leave the 300 mL flask for 10 min on ice
# transfer the culture into two 50 mL Falcon tube
# centrifuge 7500 rpm at 4C for 20 min (TOMY TA-22 rotor), and discard sup
# suspend the pellet in ice-cold 15 mL of TB (Transformation Buffer)(7.5 mL/tube)
# centrifuge 7500 rpm at 4C for 2 min (TOMY TA-22 rotor), and discard sup
# suspend the pellet in ice-cold 3.2 mL of TB
# add 0.24 mL of DMSO (stirring, bit by bit)
# leave the 50 mL Falcon tube for 10 min on ice
# dispense 50 uL into 0.5 mL tube
# freeze the suspension in liquid nitrogen
# store at -80C
==Bacterial Transformations==
==Mini-prep (Alkaline SDS Method)==
==PCR==
==Restriction Enzyme Digestions==
==DNA ligation==
==Agarose gel electrophoresis==
==Electroporation==