@@ Line 1: / Line 1: @@
-{{Template:HokkaidoU_Japan}}
-=Protocols=
-<ul class="acc" id="acc">
-<li>
-==Preparation of Competent cells (''E. coli'' DH5a)==
-<div class="acc-section">
-<div class="acc-content">
-===Reagents===
-'''TB (Transformation Buffer)(at 4C, filtration)'''
-{|border="1" class="protocol"
-|
-|
-|Final concentration
-|-
-|1 M CaCl<sub>2</sub> (at RT, autoclaved)
-|0.75 mL
-|15 mM
-|-
-|4 M KCl (at RT, autoclaved)
-|3.125 mL
-|250 mM
-|-
-|1 M MnCl<sub>2</sub> (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'''
-|
-|}
-===Procedure===
-# 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 ΔOD<sub>550nm</sub> = 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
-</div></div>
-</li>
-<li>
-==Bacterial Transformations==
-<div class="acc-section">
-<div class="acc-content">
-# add DNA solution to thawed competent cells
-# incubate the cells on ice for 30 min
-# heat shock the cells by immersion in a pre-heated water bath at 42C for 60 sec
-# incubate the cells on ice for 5 min
-# add 200 uL of SOB broth
-# incubate the cells at 37C for 2 hrs while the tubes are shaking
-# plate 200 uL of the transformation onto the dish
-# incubate the plate at 37C for 12-14 hrs
-</div></div>
-</li>
-<li>
-==Mini-prep (Alkaline SDS Method)==
-<div class="acc-section"><div class="acc-content">
-===Reagents===
-'''Solution I'''
-(at RT, filtration 0.2 um, 50 mL)
-{|border="1" class="protocol"
-|-
-|
-|
-|Final concentration
-|-
-|Glucose (at RT)
-|0.45 g
-|50 mM
-|-
-|1 M Tris-HCl (pH8.0, at RT, autoclaved)
-|1.25 mL
-|25 mM
-|-
-|0.5 M EDTA (pH8.0, at RT, autoclaved)
-|1 mL
-|10 mM
-|-
-|'''Total'''
-|'''50 mL'''
-|
-|}
-<br>
-'''Solution II'''
-(at RT, filtration 0.2 um, 20 mL)
-{|border="1" class="protocol"
-|-
-|
-|
-|Final concentration
-|-
-|10 N NaOH (at RT)
-|0.4 mL
-|0.2 N
-|-
-|10% SDS (at RT, filtration)
-|2 mL
-|1%
-|-
-|'''Total'''
-|'''20 mL'''
-|
-|}
-<br>
-'''Solution III'''
-(at RT, filtration 0.2 um, 50 mL)
-{|border="1" class="protocol"
-|-
-|
-|
-|Final concentration
-|-
-|5 M CH<sub>3</sub>COOK
-|30 mL
-|3 M
-|-
-|CH<sub>3</sub>COOH
-|5.75 mL
-|
-|-
-|H<sub>2</sub>O
-|14.25 mL
-|
-|-
-|'''Total'''
-|'''50 mL'''
-|
-|}
-===Procedure===
-# lift colony ''E. coli'' into 2 mL LB contained antibiotics
-# culture cells at 37C for 16-20 hrs at 180-200 rpm
-# transfer 1.2-1.5 mL of culture into 1.5 mL tube
-# centrifuge the culture at 15,000 rpm for 1 min at 4C and discard sup
-# suspend the pellet in ice-cold 100 uL of Solution I
-# add 200 uL of Solution II to the suspension
-# mix by inverting the tube 10-20 times
-# add ice-cold 150 uL of Solution III to the suspension
-# mix by inverting the tube 10-20 times
-# leave the tube for 5 min on ice
-# add 10 uL of Chloroform
-# mix by inverting the tube 5-10 times
-# centrifuge the suspension at 15,000 rpm for 5 min at 4C
-# transfer the supernatant into new 1.5 mL tube↓
-# add equal volume of isopropanol and mix by voltexing
-# leave the tube for 5 min at RT
-# centrifuge the suspension at 15,000 rpm for 10 min at 4C and discard sup
-# rinse the ppt by 70% EtOH and mix by voltexing
-# centrifuge the suspension at 15,000 rpm for 2 min at 4C and discard sup
-# dry up the ppt
-# dissolve the ppt in 50 uL of TE (pH 8.0)
-# add 1 uL of 10 mg/mL RNase A (4C and stock at –20C)
-# incubate for 30 min at 37C
-# PCIAA and CIAA extraction
-# Ethanol precipitation
-# dry up the ppt
-# dissolve the ppt in 50 uL of TE (pH 8.0)
-</div></div></li><li>
-==PCR==
-<div class="acc-section"><div class="acc-content">
-===Vector===
-'''Standard reaction setup'''
-{|class="protocol" style="text-align:center;" border="1"
-|-
-!Component
-!Volume
-|-
-|10x PCR Buffer
-|5 uL
-|-
-|2mM dNTPs
-|5 uL
-|-
-|25mM MgSO<sub>4</sub>
-|3 uL
-|-
-|Suffix-F primer
-|1 uL
-|-
-|Prefix-R primer
-|1 uL
-|-
-|Template DNA
-|1 uL
-|-
-|KOD -Plus- Neo
-|1 uL
-|-
-|DW
-|X uL
-|-
-|'''Total'''
-|'''50 uL'''
-|}
-'''Cycling conditions ''' (2-step cycle)
-{|class="protocol" border="1"
-|-
-| Predenature
-| 94C 2 min
-|-
-| Denature
-| 98C 10 sec
-|-
-| Extension
-| 68C X sec (30 sec/kb)
-|-
-| Hold
-| 4C
-|}
-* 30-40 cycles
-===Insert===
-'''Standard reaction setup'''
-{|class="protocol" style="text-align:center;" border="1"
-|-
-!Component
-!Volume
-|-
-|10x PCR Buffer
-|5 uL
-|-
-|2mM dNTPs
-|5 uL
-|-
-|25mM MgSO<sub>4</sub>
-|3 uL
-|-
-|EX-F primer
-|1 uL
-|-
-|PS-R primer
-|1 uL
-|-
-|Template DNA
-|1 uL
-|-
-|KOD -Plus- Neo
-|1 uL
-|-
-|DW
-|X uL
-|-
-|'''Total'''
-|'''50 uL'''
-|}
-'''Cycling conditions ''' (2-step cycle)
-{|class="protocol" border="1"
-|-
-| Predenature
-| 94C 2 min
-|-
-| Denature
-| 98C 10 sec
-|-
-| Extension
-| 68C X sec (30 sec/kb)
-|-
-| Hold
-| 4C
-|}
-* 30-40 cycles
-===Colony PCR===
-* resuspend a colony into 10 uL of DW (template suspension)
-*
-'''Standard reaction setup'''
-{|class="protocol" style="text-align:center;" border="1"
-|-
-!Component
-!Volume
-|-
-|template suspension
-|4.8 uL
-|-
-|Quick Taq
-|5 uL
-|-
-|Forward primer
-|0.1 uL
-|-
-|Reverse primer
-|0.1 uL
-|-
-|'''Total'''
-|'''10 uL'''
-|}
-'''Cycling conditions ''' (2-step cycle)
-{|class="protocol" border="1"
-|-
-| Predenature
-| 94C 2 min
-|-
-| Denature
-| 94C 10 sec
-|-
-| Extension
-| 68C X sec (60 sec/kb)
-|-
-| Hold
-| 4C
-|}
-* 30-40 cycles
-</div></div></li><li>
-==Restriction Enzyme Digestions==
-<div class="acc-section"><div class="acc-content">c</div></div></li><li>
-==DNA ligation==
-<div class="acc-section"><div class="acc-content">d</div></div></li><li>
-==Agarose gel electrophoresis==
-<div class="acc-section"><div class="acc-content">
-[[Image:HokkaidoU_Pictures_DNA_Marker.png|200px|thumb|right|DNA Weight Markers]]</div></div></li><li>
-==Electroporation==
-<div class="acc-section"><div class="acc-content">
-'''Preparation of electro-competent cells'''
-# cell culture in 400 mL of SOB or LB and grow to ΔOD<sub>600</sub> = 0.5~0.6
-# dispense the medium into 8 Falcon 50 mL tube
-# centrifuge at 3500 rpm for 5 min at 4C and discard sup
-# add 5 mL of DW and suspend the ppt, mix 8 suspensions into single Falcon tube
-# centrifuge at 3500 rpm for 5 min at 4C and discard sup
-# add 40 mL of DW and suspend the ppt
-# centrifuge at 3500 rpm for 5 min at 4C and discard sup
-# add 10 mL of 10% Glycerol and suspend the ppt
-# centrifuge at 3500 rpm for 5 min at 4C and discard sup
-# add 10 mL of 10% Glycerol and suspend the ppt
-# centrifuge at 3500 rpm for 5 min at 4C and discard sup
-# add 5 mL of 10% Glycerol and suspend the ppt
-# dispense 100 uL of the suspensions into 0.5 mL Eppendorf tube, respectively
-# store at -80C freezer
-<br>
-'''Electroporation'''
-</div></div></li><li>
-==PCIAA and CIAA extraction==
-<div class="acc-section"><div class="acc-content">
-'''Reagent'''
-* PCIAA = Phenol : Chloroform : IsoAmyl Alcohol = 25 : 24 : 1
-* CIAA = Chloroform : IsoAmyl Alcohol = 24 : 1
-'''Procedure'''
-# add equal volume of PCIAA and vortex vigorously
-# centrifuge at 15,000 rpm for 2 min at RT
-# transfer the aqueous phase to a new tube, being careful not to transfer the phase interface
-# add equal volume of CIAA and vortex vigorously
-# transfer the aqueous phase to a new tube
-# ethanol precipitation
-</div></div></li><li>
-==Ethanol presipitation==
-<div class="acc-section"><div class="acc-content">
-# add 1/10 volume of 3M CH<sub>3</sub>COONa
-# add 2.5 volume of 100% ethanol (EtOH)
-# incubate on ice for few min
-# centrifuge at 15,000 rpm for 10 min at 4C and discard sup
-# wash precipitation with 100 uL of 70% EtOH (EtOH has to be cold)
-# centrifuge at 15,000 rpm for 5 min at 4C and discard sup
-# dry up the ppt (no EtOH should be left)
-# resuspend ppt in wanted volume of TE
-</div></div></li></ul>
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Team:HokkaidoU Japan/Protocols

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Revision as of 10:17, 25 September 2010