Team:Arizona State/Notebook/July
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Ethan ward (Talk | contribs) (Created page with "{{:Team:Arizona_State/Templates/sidebar|title=Notebook: July}} __NOTOC__ == Friday, July 1 == * Ran a gel of PCRed CAS genes from last night * Transformation of NEB cells: :* DA:...") |
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:* GFP streak plate: usable colonies | :* GFP streak plate: usable colonies | ||
:* DAx4, RAx4, seq1 transformation: usable colonies | :* DAx4, RAx4, seq1 transformation: usable colonies | ||
+ | * Got order from IGEM (psb1a3 and agar stab of J04430) | ||
+ | :* transformed psb1a3 plasmid to make stock | ||
+ | :* streak plated agar stab of J04430 | ||
+ | |||
+ | == Saturday / Sunday, July 9 / 10 == | ||
+ | * Gel of theoretical array (1x, 4x): | ||
+ | :* plasmid backbone visible, but no inserts | ||
+ | :* will need to start over from 1x | ||
+ | * PCR: homerun, EDC, AB, 3 | ||
+ | :* no success | ||
+ | |||
+ | == Monday, July 11 == | ||
+ | * Transformation results from Friday: | ||
+ | :* PSB1A3: DNA contamination? Red colononies as well as normal growing on plates | ||
+ | ::* will sequence once we get biobrick standard primers | ||
+ | :* agar stab of part J04430: normal (glowing) | ||
+ | |||
+ | * made liquid cultures of: | ||
+ | :* SEQ1, DA, RA (8x) in PSB1k3 | ||
+ | :* PSB1A3 (pink, white colonies) | ||
+ | :* J04430 | ||
+ | |||
+ | * restriction: | ||
+ | :* restarting from 1x in PSB1K3 | ||
+ | :* gingko: | ||
+ | ::* seq1: es, xp | ||
+ | ::* da: es, xp | ||
+ | ::* ra: es, xp | ||
+ | ::* e0840: ep to get PSB1A3 backbone | ||
+ | :* normal: | ||
+ | ::* seq1: es, ex | ||
+ | ::* da: es, ex | ||
+ | ::* ra: es, ex | ||
+ | |||
+ | * ligation: | ||
+ | :* 2x seq1, da, ra 2 ways: | ||
+ | ::* psb1k3 | ||
+ | ::* psb1a3 (gingko) | ||
+ | |||
+ | * transformation onto 14 plates: | ||
+ | :* new promoter (g18 on plate 1) in duplicate | ||
+ | :* ligation products in duplicate | ||
+ | |||
+ | * planning: | ||
+ | :* planned assembly of plasmid construct (cas genes, leader sequence, array) using duet plasmid |
Revision as of 16:46, 12 July 2011
Notebook: July
Friday, July 1
- Ran a gel of PCRed CAS genes from last night
- Transformation of NEB cells:
- DA: Kan x2, LB
- DB: Kan x2, LB
- Seq1: Kan x2
- CMR: Kan x2, LB
Saturday, July 2
- Plates from Friday: successful transformation for all except CMR
- Need to find a plasmid that can handle such a large insert
- Made overnight cultures of colonies
- Ligation, transformation of RA, RB onto kan plates
- Gels of more PCR products: no usable bands
Tuesday, July 5
- Another PCR attempt with new CAS primers (A, C)
- Miniprep of DA, DB, RA, SEQ1
- Restriction digest of:
- SEQ1, DA, RA, (ES, EX) in PSB1K3
- Tried 2 different ligation protocols:
- Normal protocol:
- seq1 + seq1, da + da, ra + ra
- transformation of ligation products, plated on kan (NEB cells)
- Gingko protocol:
- seq1 (ES, XP) + PSB1A3 (EP)
- transformation, plated on amp (NEB cells)
- glycerol stocks of seq1, da, db, ra, rb in PSB1K3
Wednesday, July 6
- Transformation results:
- Kan plates:
- all successful (?) (seq1 + seq1, da + da, ra + ra), will be sequenced (ordered biobrich forward / reverse primers)
- made liquid culture for miniprep tomorrow
- Amp plates:
- no success
- PCR:
- cas_b, cas_c both unsuccessful (see pictures of gels)
- cas_d run, will visualize tomorrow
- adjusting settings for cas_e_f, cas_3_r: 2 parallel
- touchdown to 70 using builtin touchdown
- constant 70
- probably need new primers
Thursday, July 7
- Miniprep of:
- DADA (kit buffer) in PSB1k3
- RARA (kit buffer) in PSB1k3
- Seq1Seq1 (kit buffer, Dan's buffer) in PSB1k3
- Consensus: Dan's buffer that he created for lysis works
- Nanodrop results: (DADA 48 ng/uL, RARA 68 ng/uL, Seq1Seq1 Dan 73.5 ng/uL, Seq1Seq1 Kit 98 ng/uL)
- Gel of "homerun" attempt from yesterday, Block A touchdown + Block B constant 70 degC
- Unsuccessful, deformed gel near top, nonspecific binding, weird band at ~800bp (see photo)
- Met w/ 3 grad students (Kurt, Jack?, Bo) and had good discussion
- Gel techniques: doing gels in 4 degree room, using X-tracta gel removers for gel band extraction
- Assembly: problems with large insertions (see Infusion)
- Infusion (clonetech)
- Beginning to construct our GFP test plasmid:
- Transformation of biobrick promoter J23101 onto amp (2 plates)
- Streak plated E0840 GFP part onto amp from glycerol stock (3 plates)
- Determined theoretical 3 part PCR (casEDC, casBA, case)
- PCR attempts (see photo):
- CasE forward, Cas3 reverse again but w/varying template DNA concentrations
- 225 ng/uL, 112.5 ng/uL, 56 ng/uL (previous starting conc. was 450, which is too high and could have caused problems)
- started @ 80deg, increment -.3
- Cas3 forward/reverse w/same varying template DNA concentrations
- Restrictions:
- Seq1Seq1 (ES, EX)
- DADA (ES, EX)
- RARA (ES, EX)
- Ligation for theoretical 4-mer:
- 2x Seq1Seq1
- 2x DADA
- 2x RARA
- Plated onto 3 kan plates using NEB cells.
Friday, July 8
- Yesterday's plates:
- promoter transformation: no colonies
- GFP streak plate: usable colonies
- DAx4, RAx4, seq1 transformation: usable colonies
- Got order from IGEM (psb1a3 and agar stab of J04430)
- transformed psb1a3 plasmid to make stock
- streak plated agar stab of J04430
Saturday / Sunday, July 9 / 10
- Gel of theoretical array (1x, 4x):
- plasmid backbone visible, but no inserts
- will need to start over from 1x
- PCR: homerun, EDC, AB, 3
- no success
Monday, July 11
- Transformation results from Friday:
- PSB1A3: DNA contamination? Red colononies as well as normal growing on plates
- will sequence once we get biobrick standard primers
- agar stab of part J04430: normal (glowing)
- made liquid cultures of:
- SEQ1, DA, RA (8x) in PSB1k3
- PSB1A3 (pink, white colonies)
- J04430
- restriction:
- restarting from 1x in PSB1K3
- gingko:
- seq1: es, xp
- da: es, xp
- ra: es, xp
- e0840: ep to get PSB1A3 backbone
- normal:
- seq1: es, ex
- da: es, ex
- ra: es, ex
- ligation:
- 2x seq1, da, ra 2 ways:
- psb1k3
- psb1a3 (gingko)
- transformation onto 14 plates:
- new promoter (g18 on plate 1) in duplicate
- ligation products in duplicate
- planning:
- planned assembly of plasmid construct (cas genes, leader sequence, array) using duet plasmid