Team:Johns Hopkins/Notebook/YVL

(Difference between revisions)

Yeast Vector Library

7/1/11

• Made growth plates for the 12 vectors

-pRS 403: HIS3 Selectable, Integrating -pRS 404: TRP1 Selectable, Integrating -pRS 405: LEU2 Selectable, Integrating -pRS 406: URA3 Selectable, Integrating -pRS 413: HIS3 Selectable, CEN/ARS Episomal -pRS 414: TRP1 Selectable, CEN/ARS Episomal -pRS 415: LEU2 Selectable, CEN/ARS Episomal -pRS 416: URA3 Selectable, CEN/ARS Episomal -pRS 423: HIS3 Selectable, 2micron Episomal -pRS 424: TRP1 Selectable, 2micron Episomal -pRS 425: LEU2 Selectable, 2micron Episomal -pRS 426: URA3 Selectable, 2micron Episomal

• Repipetted primers
• Started PCR experiment design

7/2/11

• Created 2 mL overnight cultures of vectors in E. coli w/ LB + Carbenicillin
• 37C incubation

7/3/11

• Miniprep 12 vectors from 2 mL overnights
• Store in -20C

7/5/11

• Designed the multiple cloning site substitution and QuikChange protocol to run by Dr. Boeke

7/6/11

• Created and consolidated all PCR reagents and DNA for tomorrow's PCR

7/7/11

• Multiple cloning site substitution PCR

7/8/11

• DpnI Digest
• Ligation

7/11/11

• Transformation and plating

7/12/11

• No colonies
• Repeat transformation and plating

7/13/11

• No colonies
• Optimized PCR protocol according to Agilent's Herculase manual

7/14/11

• Regrew original pRS vectors in overnight cultures

7/15/11

• Mini prep vectors
• MCS delete/insert PCR

7/16/11

• PCR Purification

7/18/11

• DpnI digest
• Overnight ligation at 16C

7/19/11

• Transformation of 12 vectors

7/20/11

• No colonies
• Verify original vectors with EcoRI digest
• Verification successful

7/21/11

• Re-do transformation

7/22/11

• Transformation failed
• Change QCPCR protocol to new two-step process
• Create competent cells

7/25/11

• Try new Site Directed Mutagenesis QCPCR protocol on pRS 416 @ various template and primer concentrations

7/26/11

• Yeast spec. assay
• DpnI digest
• 416 Site Directed Mutagenesis Transformation

7/27/11

• Bad competent cells (no colonies on pos. ctrl.)
• Redo QCPCR w/ 9 primer/template concentrations

7/28/11

• DpnI digest of 416 QCPCR
• Transformation using high efficiency TOP10 cells

7/29/11

• 416 SDM QCPCR worked!
• Grow overnight cultures

8/1/11

• Miniprep
• 2nd step QCPCR

8/2/11

• DpnI digest
• Transformation

8/3/11

• Transformation successful: finished 416 biobricked vector
• Grow overnight culture

8/4/11

• Create new competent cells using TSS protocol

8/25/11

• 1st QCPCR on rest of vectors
• DpnI digest
• Transformation

8/26/11

• Colonies for all but 413 and 403
• Grow overnight cultures

8/27/11

• Miniprep successful transformations

8/29/11

• 2nd QCPCR on successful 1st QCPCRs

8/30/11

• DpnI digest

8/31/11

• QCPCR (site directed mutagenesis) on 403, 405, 413, 415, 423

9/1/11

• Digest EcoRI, XbaI, SpeI and PstI on final biobricked vector (416)
• Run Gel: Failed (PstI had 3 products instead of 1)

9/5/11

• DpnI digest 8/31 reactions
• Transform 8/31 reactions

9/6/11

• Colonies for 403, 405, 413, 415, 423, 424, 425

9/7/11

• Redo first second round QCPCR (multiple cloning site swap) 9/6 colonies

9/8/11

• PCR failed: Samples evaporated in PCR machine

9/12/11

• Redo first round (site directed mutagenesis) on all pRS vectors

9/13/11

• DpnI digest
• Transform 9/7 QCPCR

9/14/11

• No colonies
• Problem may be in incompatible PCR buffer (Herculase buffer) and Transformation buffer. Solution is to do PCR purification before transformation.
• Check theory by running PCR purification on PCR products that previously failed transformation and re-transform

9/15/11

• Colonies! Theory confirmed.
• Re-run all QCPCR (site directed mutagenesis) reactions

9/16/11

• DpnI digest
• Transform

9/17/11

• All QCPCR reactions had large amount of colonies
• Miniprep all samples

9/20/11

• Restriction enzyme digest check on all miniprepped vectors