IGEM:Harvard/2006/Lab Intro

Remove plates from 37C
Pick 3-5 colonies from each plate, plus 1 spot away from any colony as a control. I usually use a pipette tip, and just pop the whole thing into a culture tube containing 2 ml LB media (+ antibiotic).
- (see http://openwetware.org/wiki/Bacterial_cell_culture)
Grow on shaker at 37C overnight

June 8

Pour a gel, and let this cool during step 5.
- We can run a 1% gel.
- Weigh out 1 g agarose and add 1x TBE to a total of ~100 g.
- Squirt in a few extra grams of distilled water to allow for evaporation.
- Microwave until agarose is fully dissolved (try 1 minute, followed by 30 second increments.
Qiagen miniprep kit on all samples.
- http://openwetware.org/wiki/Miniprep/Qiagen_kit
Make glycerol stocks at this point. (Add 50 ul cells + 50 ul 30% glycerol to 1.5 ml tube, mix by pipetting and place in -80 freezer)

Construction plasmids
- pSB1A3 - Amp
- pSB1AC3 - Amp/Cm
- pSB1AK3 - Amp/Kan
- pSB1AT3 - Amp/Tet

Hydrate and transform pSB1AT3 into competent cells
Grow overnight 37°C

June 9

Old pages

miniprep pSB1AT3
- Digest - E + P (construction)
R0010
- Digest - E + S (part 1: prefix)
- plasmid pSB1A2 (amp resistance)
E0241
- Digest - X + P (part 2: suffix)
- plasmid: pSB1A2 (amp resistance)

BioBrick Digests

Run samples on gel, cut out bands of proper size. Make sure to weigh empty tubes beforehand, so we will know the weight of the band.
Qiagen gel-extraction kit. Quantitate on nanodrop to determine concentration. (see http://openwetware.org/wiki/Wittrup:_Gel_extraction and Qiagen manual).
(pour a gel at this point)
Ligation (follow protocol that comes with T4 ligase, for example), with proper controls. While ligation runs, figure out what size products you are expecting.
Gel purification of ligated product. Same as steps 4-7.
Transformation (same as Tuesday).

Come in early (e.g. 8 am) and pick colonies so we can miniprep them the same day. Grow at 37C for 6-8 hours.
- Alternatively, come in late and grow cultures overnight and then continue on Saturday
Miniprep & nanodrop quantitation
Gel analysis / purification
Submit samples for sequencing.

June 12

10:00 - lectures + lunch (room 1058)
12:30 - tour, etiquette, wiki notebooks
12:45 - quick intro to folding DNA, prepare folding rxns and start folding, pour gels
13:30 - quick intro to cloning, transformations, PCR, etc
14:00 - transform, plate out bacteria.
16:00 - load and run gels for folding reactions
17:00 - image gels, plan for tomorrow

Folding DNA nanostructures

June 13

Room 1058 is booked from 9 am to 1 pm today
10:00 - pick colonies, start cultures
10:45 - present previous project (1 per student)
14:00 - discussion
16:00 - minipreps

June 14

Room 1079 is booked from 9 am to 1 pm today
10:00 - digest, ligate, gel purify, transform DNA
16:00 - discussion

June 15

Room 1058 is booked from 9 am to 1 pm today
minipreps, digests, run gels, submit samples for sequencing, phenotypic assays, discussion

June 16

Room 1058 is booked from 9 am to 1 pm today

@@ Line 1: / Line 1: @@
+==June 5==
 Parts:
-R0010 - LacI promoter
+[http://parts.mit.edu/registry/index.php/Part:BBa_R0010 R0010] - LacI promoter
 * Plate 1, Well 7K
 * amp resistance
 * Hydrated yellow
-E0241 - GFP reporter
+[http://parts.mit.edu/registry/index.php/Part:BBa_E0241 E0241] - GFP reporter
 * Plate 2, Well 15L
 * amp resistance
 * Hydrated red
-E7104 - GFP reporter behind T7 promoter
+[http://parts.mit.edu/registry/index.php/Part:BBa_E7104 E7104] E7104 - GFP reporter behind T7 promoter
 * Plate 2, Well 13F
 * amp resistance
@@ Line 18: / Line 19: @@
 *Digest R0010 - SpeI + PstI (prefix)
 *Digest E0241 - XbaI + PstI (Suffix)
+'''Standard Assembly Information'''
+[http://parts.mit.edu/wiki/index.php/Standard_Assembly Assembly Overview]
+<b>Restriction Enzymes Used</b>
+*[http://rebase.neb.com/rebase/enz/XbaI.html About XbaI]  [http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Retrieve&db=PubMed&list_uids=592365&dopt=Abstract Origins of XbaI]
+*[http://rebase.neb.com/rebase/enz/SpeI.html About SpeI] [http://home1.gte.net/vsjslsk1/sphaerotilus.htm Origins of SpeI]
+*[http://rebase.neb.com/rebase/enz/EcoRI.html EcoRI] [http://en.wikipedia.org/wiki/EcoRI More info about EcoRI]
+*[http://rebase.neb.com/rebase/enz/PstI.html PstI] [http://www.thelabrat.com/restriction/sources/Providenciastuartii.shtml Origins of Pst1]
 Gel extraction -> Ligation -> Transformation -> Miniprep -> Sequencing
@@ Line 24: / Line 38: @@
 [[Transforming_chemically_competent_cells]]
+==June 6==
+*pick colonies and inoculate overnight cultures
@@ Line 41: / Line 58: @@
 **http://openwetware.org/wiki/Miniprep/Qiagen_kit
 *Make glycerol stocks at this point.  (Add 50 ul cells + 50 ul 30% glycerol to 1.5 ml tube, mix by pipetting and place in -80 freezer)
-*Digest R0010 - SpeI + PstI (prefix)
-*Digest E0241 - XbaI + PstI (Suffix)
+*[http://parts.mit.edu/r/parts/partsdb/pgroup.cgi?pgroup=Plasmid Construction plasmids]
+**[http://parts.mit.edu/registry/index.php/Part:pSB1A3 pSB1A3] - Amp
+**[http://parts.mit.edu/registry/index.php/Part:pSB1AC3 pSB1AC3] - Amp/Cm
+**[http://parts.mit.edu/registry/index.php/Part:pSB1AK3 pSB1AK3] - Amp/Kan
+**[http://parts.mit.edu/registry/index.php/Part:pSB1AT3 pSB1AT3] - Amp/Tet
+*Hydrate and transform pSB1AT3 into competent cells
+*Grow overnight 37°C
+==June 9==
+*[http://parts.mit.edu/r/parts/htdocs/Assembly/index.cgi BioBrick Assembly]
+*[http://parts.mit.edu/r/parts/htdocs/Assembly/standard_assembly.cgi Standard Assembly of 2 Parts]
+'''Old pages'''
+*[http://biobricks.ai.mit.edu/Assembly/BB_Assembly.htm Biobrick Assembly]
+*[http://biobricks.ai.mit.edu/Assembly/Assy_Alternatives.htm Assembly alternatives]
+**[http://biobricks.ai.mit.edu/Assembly/Assy_3A.htm updated 3A]
+**[http://biobricks.ai.mit.edu/Assembly/Assy_Sel_Mix_CcdB.htm CcdB]
+**[http://biobricks.ai.mit.edu/Assembly/Assy_Sel_Mix_Split.htm Split Gene Strategy]
+*miniprep pSB1AT3
+**Digest - E + P (construction)
+*R0010
+**Digest - E + S (part 1: prefix)
+**plasmid pSB1A2 (amp resistance)
+*E0241
+**Digest - X + P (part 2: suffix)
+**plasmid: pSB1A2 (amp resistance)
+*[[Knight:Restriction_Digest|BioBrick Digests]]
 *Run samples on gel, cut out bands of proper size.  Make sure to weigh empty tubes beforehand, so we will know the weight of the band.
 *Qiagen gel-extraction kit.  Quantitate on nanodrop to determine concentration. (see http://openwetware.org/wiki/Wittrup:_Gel_extraction and Qiagen manual).
 *(pour a gel at this point)
-*Ligation (follow protocol that comes with T4 ligase, for example), with proper controls.  While ligation runs, figure out what size products you are expecting.
+*[[Knight:DNA_ligation_using_NEB_Quick_Ligation_Kit|Ligation]] (follow protocol that comes with T4 ligase, for example), with proper controls.  While ligation runs, figure out what size products you are expecting.
 *Gel purification of ligated product. Same as steps 4-7.
 *Transformation (same as Tuesday).
-==June 9==
 *Come in early (e.g. 8 am) and pick colonies so we can miniprep them the same day.  Grow at 37C for 6-8 hours.
 **Alternatively, come in late and grow cultures overnight and then continue on Saturday
@@ Line 56: / Line 104: @@
 *Gel analysis / purification
 *Submit samples for sequencing.
-from 9 am to 1 pm on:
-/13, 6/15, and 6/16.  On 6/14 room 1058 was already booked, I have
-reserved room 1079.
 ==June 12==
@@ Line 66: / Line 109: @@
 *12:30 - tour, etiquette, wiki notebooks
 *12:45 - quick intro to folding DNA, prepare folding rxns and start folding, pour gels
-*13:30 - quick intro to cloning, transformations,
+*13:30 - quick intro to cloning, transformations, PCR, etc
 *14:00 - transform, plate out bacteria.
 *16:00 - load and run gels for folding reactions
 *17:00 - image gels, plan for tomorrow
+[[IGEM:Harvard/2006/Folding_DNA_nanostructures|Folding DNA nanostructures]]
 ==June 13==

IGEM:Harvard/2006/Lab Intro

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