Team:Arizona State/Notebook/July

From 2011.igem.org

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(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
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* Got order from IGEM (psb1a3 and agar stab of J04430)
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:* transformed psb1a3 plasmid to make stock
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:* streak plated agar stab of J04430
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== Saturday / Sunday, July 9 / 10 ==
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* Gel of theoretical array (1x, 4x):
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:* plasmid backbone visible, but no inserts
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:* will need to start over from 1x
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* PCR: homerun, EDC, AB, 3
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:* no success
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== Monday, July 11 ==
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* Transformation results from Friday:
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:* PSB1A3: DNA contamination? Red colononies as well as normal growing on plates
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::* will sequence once we get biobrick standard primers
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:* agar stab of part J04430: normal (glowing)
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* made liquid cultures of:
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:* SEQ1, DA, RA (8x) in PSB1k3
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:* PSB1A3 (pink, white colonies)
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:* J04430
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* restriction:
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:* restarting from 1x in PSB1K3
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:* gingko:
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::* seq1: es, xp
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::* da: es, xp
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::* ra: es, xp
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::* e0840: ep to get PSB1A3 backbone
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:* normal:
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::* seq1: es, ex
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::* da: es, ex
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::* ra: es, ex
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* ligation:
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:* 2x seq1, da, ra 2 ways:
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::* psb1k3
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::* psb1a3 (gingko)
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* transformation onto 14 plates:
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:* new promoter (g18 on plate 1) in duplicate
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:* ligation products in duplicate
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* planning:
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:* planned assembly of plasmid construct (cas genes, leader sequence, array) using duet plasmid

Revision as of 16:46, 12 July 2011