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CRISPR System Caroline Vrana Davidson College Synthetic Biology Summer 2012.

Published byAngelica Wade Modified over 9 years ago

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Presentation on theme: "CRISPR System Caroline Vrana Davidson College Synthetic Biology Summer 2012."— Presentation transcript:

1 CRISPR System Caroline Vrana Davidson College Synthetic Biology Summer 2012

2 Big Picture Non-promoter gene regulation Modular Selection Mechanism

3 Full version CRISPR sequence Yellow= BioBrick prefix and suffix Blue= leader sequence Pink= CRISPR repeat Greens= GFP target spacer Reds= AmpR target spacer

4 Simplified synthetic CRISPR sequence BioBrick ends Leader Sequence CRISPR repeat GFP target spacer BamHI recognition site

5 Ligation combinations Reporter Genes GFP – pSB1A8 – pSB4A8 – pSB1C8 – pSB4C8 RFP – pSB1A8 – pSB4A8 – pSB1C8 – pSB4C8 CRISPR – In pSB1K8 All ligations were successful and all in the GCAT-alog

6 Oligo Assembled CRISPR Experiment Results

7 Ratio of GFP fluorescence Expected  no green in CRISPR colonies Results  real green fluorescence

8 Company Synthesized CRISPR experiments

9 CRISPR in pSB1K8 GFP and RFP in pSB4A8 Expected  no growth Results  no growth

10 CRISPR in pSB1K8 GFP and RFP in pSB4C8 Expected  no green fluorescence (only red) Results  real green fluorescence

11 Conclusions/Future Steps Company synthesized CRISPR System  didn’t destroy GFP – Re-do experiment  more colonies to screen Put into modular selection mechanism

12

13 Background CRISPR – Clustered Regularly Interspaced Short Palindromic Repeats Functions as the prokaryotic “immune system” Found first in E.coli in 1987 Found in 90% of archaea and 40% of bacteria tested so far

14 CRISPR process www.wikipedia.org

15 Full version CRISPR sequence Yellow= BioBrick prefix and suffix Blue= leader sequence Pink= CRISPR repeat Greens= GFP target spacer Reds= AmpR target spacer

16 Problems Long turnaround time for synthetic CRISPR sequence Sent off sequence to be synthesized In the meantime… – Simplified the sequence to only 1 target spacer and 2 CRISPR repeats – Assembling sequence on my own from overlapping oligos

17 Simplified synthetic CRISPR sequence BioBrick ends Leader Sequence CRISPR repeat GFP target spacer BamHI recognition site

18 Simplified Sequence Includes: – BioBrick prefix and suffix – Leader sequence (in lieu of promoter) – CRISPR repeats – GFP target spacer – BamHI recognition site  for expanding the sequence in the future

19 End goals Co-transform E.coli cells with 2 plasmids – 1. Synthetic CRISPR sequence in Kan plasmid – 2. A target plasmid (including target spacer of GFP and/or AmpR) Have the CRISPR plasmid destroy the target plasmid  destroying the ampicillin resistance Assess growth (or lack of growth)

20 Non-CRISPR plasmid Ligating different combinations of inserts/plasmids – GFP in non-AmpR plasmid – RFP in AmpR plasmid – GFP in AmpR plasmid

21 Ligations/Transformations GFP RFP GOI OR CRISPR

22 Ligation combinations INSERTS J04450 (RFP) K091131 (GFP) CRISPR sequence PLASMIDS pSB1A8 pSB4A8 pSB1C8 pSB4C8 pSB1K8

23 Parts- Inserts GFP – K091131 – pLacIQ1 + RBS + GFP + TT – Originally in pSB1A2 RFP – J04450 – pLacI + RBS + RFP + TT – Originally in pSB1A2

24 Parts- Plasmids pSB1A8 – J119043 pSB4A8 – J119048 pSB1C8 – J119045 pSB4C8 – J119049 pSB1K8 – J119046 – Cloning CRISPR sequence into here

25 GFP in Amp plasmids GFP and pSB1A8 – Some larger than negative control – Sent off MP DNA of 2 colonies to be sequence verified – Ligation worked GFP and pSB4A8 – Experimental wells larger than negative control – Sent off 2 colonies to be sequence verified – Ligation worked

26 Problems with GFP After sequence verification of ligations- – Found 35 bp spontaneous insertion mutation – Has been documented in the promoter before – Will still work  but not as bright

27 RFP in pSB4A8 Some colonies were visibly red Colony PCR results – Experimental DNA larger than negative control – Sent off DNA from 2 colonies to be sequence verified – Ligation worked

28 RFP in pSB1A8 RFP and pSB1A8 Some colonies glowed visibly red  no need to do colony PCR and sequence verification Ligation worked

29 RFP in pSB1C8 Cells grown from glycerol stocks of RFP and pSB1C8 Ligation worked

30 GFP and RFP in pSB4C8 Colony PCR Most of the colonies are larger than negative control Both red and green fluorescent colonies in later experiments Ligation worked Neg. control GFP RFP

31 Successful Ligations 8 possible combinations successfully ligated Glycerol stocks made and located in GCAT-alog

32 Problems with Cloramphenicol plasmids GFP and RFP in pSB4C8 RFP in pSB1C8

33 CRISPR experiment Oligos arrived on 7/6/12 Assembled by boiling Ligated CRISPR sequence into pSB1K8 plasmid Did colony PCR on 12 colonies

34 Colony PCR of CRISPR sequence One colony seems to be the right length

35 Length verification of CRISPR Length verification of the one colony PCR product Small smear of band seems to be right length (around 240)

36 CRISPR Experiment Cotransformations 4 experimental conditions – Only the CRISPR sequence – Only GFP in pSB4A8 and RFP in pSB4A8 – Empty pSB1K8 plasmid, GFP and RFP in pSB4A8 – CRISPR sequence, GFP and RFP in pSB4A8

37 Co- Transformations GFP RFP CRISPR Selective Media

38 Results

39 Only CRISPR sequence Expected  no growth Result  no growth

40 Only GFP and RFP in pSB4A8 Expected  no growth Results  no growth

41 Empty pSB1K8, GFP in pSB4A8, RFP in pSB4A8 Expected  equal amounts of green and red colonies Results  about equal amounts of green and red colonies

42 CRISPR sequence, GFP in pSB4A8, and RFP in pSB4A8 Expected  only red colonies Results…

43 Ratio of GFP fluorescence

44 Conclusions The CRISPR sequence did not destroy the plasmid containing GFP Reason  1 nucleotide missing in the GFP target spacer when compared to the GFP gene sequence

45 2 nd CRISPR Sequence Synthesized sequence from the company came 7/18 New Experiment – Only GFP and RFP in pSB4A8 – Empty pSB1K8 plasmid, GFP and RFP in pSB4A8 – CRISPR, GFP and RFP in pSB4A8 – CRISPR, GFP and RFP in pSB4C8 The CRISPR should destroy plasmids containing GFP and Ampicillin resistance

46 GFP and RFP Fluorescence

47 GFP and RFP in pSB4A8 A plates only - control

48 Empty pSB1K8 GFP and RFP in pSB4A8 K and A plates

49 Empty pSB1K8 GFP and RFP in pSB4C8 K and C plates

50 CRISPR in pSB1K8 GFP and RFP in pSB4A8

51 CRISPR in pSB1K8 GFP and RFP in pSB4C8

52 Conclusions CRISPR system didn’t work – Minimal GFP fluorescence and no RFP fluorescence

53 Future Steps Continue working on synthetic CRISPR system If/When the sequence works, find applications Put CRISPR plasmid into cells  destroy something bad-ish only if the cell is making a product we want it to

54 Product stress Modular Selection Beneficial E. coli

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