Alberta/Calender/October

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October 2007
Su M Tu W Th F Sa
1 2 3 4 5 6
7 8 9 10 11 12 13
14 15 16 17 18 19 20
21 22 23 24 25 26 27
28 29 30 31


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== October 1 ==
JG
Miniprep J61003+Enny and Benny+J61003
Minis are in -20

ML
Brought the tubes labelled "sequencing rxns" up to MBSU
Also brought some XBA 1 from fermentas freezer since we ran out
Digests JG's miniprep with Xbal and PST. Ran out of out of XBA during digests, which meant that EJ 4,5,6only digested with XBA for 35 min
Colony O/N of I0500/ J61003 and Buddy/J61003



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Contents

October 2

VH-1PM
No Kan plates therefore made kan plates
On COuntertop
Miniprepped ML's overnights from OCt 1
Lysis solution is a no go
Started new O/N of previows overnights for tomorrow
No more LB

WM is Wayne Materi (a team advisor) in the following.

WM- Assembling all the individual genes into an operon in order of their role in the butanoate pathway from KEGG. We will start with I725021 (RBS + B-hydroxy butyryl coA dehydrogenase in the B0034 plasmid - pSB1A2)then insert I725022 (RBS + Enoyl-coa hydratase), then I725023 (RBS + Butyryl coa Dehydrogenase), then I725024 (RBS + Butyraldehyde dehydrogenase), and finally I725025 (RBS + Butanol dehydrogenase). After the operon is constructed and verified, we will insert the Arabinose promoter from I0500 5' to all the genes.

Digest I725021/SpeI+PstI and gel purify ~3kb band Digest I725022/SpeI+PstI and gel purify ~1.2kb band

Ligate (Got 16 colonies vs. 10 for negative ctl).

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== October 3 ==

MC - 800hrs
Autoclaved 2 bottosl of Ependorf tupes- to be picked up from G308
Transform THolase into XL10 gold plates
Miniprep of 10500+J61003 O/N

ML
Digest of 10500+J61003 with ECORI and XBA
Housekeeping complete
Note to Justin: Samples to sequence are in -20 labelled "Justin! Sequence me"
CZ - 7:00pm
Ran gel of I0500/J61003
It looks like I05oo is in J61003 but have to confirm with Justin or Michelle or Erin.

NB: please note the lab is unavailable EVERY wednesday from 1400-1700hrs


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October 4

NK - 930
VH - 2pm
Cleaned up 37 degree
Moved 30th plates of I0500+JG and Buddy+j6 to 4 degree fridge
Disposed of really disgusting plates
Got ride of I0500 ovrnights that hve been on shaker for a wek now
CHecke thoolase kan plates
Showing blue dots so far and af we white doets
Left plates in 37 celsious room

JP
Sequencing of 3 primer of DBS
Ligate I0500 eco/spe into J61003 (eco/xba)


WM - Primers for colony PCR and sequencing are as follows:
Primer 1 (3' end of I725021) CTGGTTGGCTGGGTCGTAAATCC
Primer 2 (3' end of I725022) GACGCTATGACCGCTTTCATCG
Primer 3 (3' end of I725023) CTACGAAGGTACCTCCGAAGTTC
Primer 4 (3' end of I725024) CGCTGATCTCCGAACTGAAAGAC
Primer 5 (3' end of I725025) CTGCGTCCGGTTAACGCTTCC
VF and VR as per BioBricks

Performed Colony PCR on 10 candidates for BuOP1 (I725021 + I725022) using Primer1 and VR (expect 1063 bp band if good)

Expect UVP00153annot.jpg

Colonies 1 and 8 look good. Sequence with Primer 1.


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October 5

JG/MC - 800hrs
Ran gel of i0500 and buddy
Digest #4 J61003/I0500 Digest Eco/xba with Pst to drop out of GFP
Ran gel of I0500J61003 eco/xba

ML
Gel completd and took photos
Buddy and I0500 digested
Extracted gel
Labelled I0500 purify Oct5 and Buddy Purify oct 5


CZ - Sorry I can't make it for personal reasons.

WM - BuOP1.1 and BuOP1.8 both sequenced good from nt 1096 to 1816.

Also ran a verifying digest on BuOP1 O/Ns

BuOP1/XbaI + SpeI (expect 2149 and 1709 bp if good)

UVP00157annot.jpg

BuOP1.1 and .8 both look good.

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October 6

ED 9:00
Made a to do list for the day

NK 2pm
Ligations of I0500 purify oct 5 and J61003
Left on bench with green tape labelled "ligations oct6"
Digest Boo34 with s,p
Digests in freezer labelled "digestions B0034 S,P"

WM - Make BuOP2 by inserting I725023 into BuOP1

Digests: BuOP1/SpeI+PstI (gel purify ~3.8kb band)

         I725023/XbaI+PstI (gel purify ~850bp band - already have)

UVP00158annot.jpg

Cutout, bands, quantitated DNA and ligated -> Plate 150 ul on LB+Amp

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October 7

ED 9:00

NG 12:00

WM - did 8 O/Ns and minipreps

Verify with XbaI+SpeI digest (expect 2149+2916bp bands if good)

UVP00160annot.jpg

All but 4 and 8 look good. Sequence BuOP2.1, 2.2, 2.5, 2.6 with Primer 2

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October 8

WM - BuOP2.1, 2.2, 2.5, 2.6 all sequenced good.


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October 9

NK
Loaded gel with digets from october 6, boo34 S,P
Put the ligations from oct6 in the freezer with the tape in tray #3

VH
Gel extrations B0034 sp1 and boo34 sp2


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October 10

JP?
Tholase PCR

MC
Ligated Buddy oct 5 into Boo34 digest oct 6
Left on bench

WM - Make BuOP3 by inserting I725024 into BuOP2

Digests: BuOP2/SpeI+PstI (expect 5047bp -> gel purify)

         I725024/XbaI+PstI (expect 2149bp and 2642bp - gel purify larger band)Not shown

UVP00161annot.jpg

Cutout all four bands and gel purify. I725024 was digested and gel-purified seperately. Quantitation of bands showed ~5pmol/ul for BuOP2/SpeI+PstI digests and ~7pmol/ul for I725024/XbaI+PstI digests.

Ligations (fast tracking construction). Plate 150ul on LB+Amp

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October 11

JP?
PCR thiolase
Transformed Buddy in Boo 1+2 into competentent cells, plated on AMP+ plates

WM - Do Colony PCR on 7 colonies (from very few transformants) with Primer 4 and VR (expect ~240bp if good).

UVP00165annot.jpg

Didn't work very well. Try confirming by digest.

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October 12

MC, JG @ 800hrs
Ran gel of PCR products
No growth on the buddy in Boo transformation
Religations of buddy into boo but couldnt find Buddy therefore religations halted

WM - Verify BuOP3 by digest with XbaI+SpeI (expect 2.1 and 5.6kb bands if good)

UVP00166annot.jpg

Sequence 1, 4, 5, 6 with Primer 3 to confirm

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October 13

ML
Religated buddy and Boo
Note: when free of tasks work on poster, or presentation or wiki or call justin or erin

WM - BuOP3.4 and 3.5 sequenced good. Due to time considerations we will call BuOP3.4 part I725099 and submit this.


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October 14

JG, MC
Retransform Buddy and Boo34
Transform tholase

JP
Restriction of thiolase with ECO/PST
Ran gel
Transform rom Bud "2" oct 12



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October 15

Re-digestions for re-ligations of boo34 and buddy
Digest boo34 s/p
Ran gel
Extract tholase from oct 14 into tube labelled "THiolase band EX"
Updated wiki

To do:
Extract gel
Ligate with buddy
Run ligation on gel
Extract
Transform

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October 16

NK- Digested B0034 with Spe and PST. -Ran a gel of restriction -Extracted Thiolase from gel on previous day.

VH and AL - Took a picture of gel -Cut out and purified four bands of B0034 from previous digestion

JP- Ligate B0034 with Buddy

WM - Verifying I725025 a.k.a. Buddy in Boo) The ligation and transformation already seem to have been done and produced many colonies. So I will do colony PCR with Primer 5 and VR (expect 250 bp) to confirm.

UVP00169annot.jpg

All 16 colonies tested look good. Setup 12 O/Ns to verify by digest.


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October 17

WM verify I725025 by /XbaI+SpeI digest (expect 2149+1.2kb bands)

UVP00170annot.jpg

All looked good. Sequence 1, 2, 9, 10.


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October 18

VH - Transformed B0034, Buddy ligations from yesterday and plated them on Amp plates

WM - I725025 sequences all good. Use #1.

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October 19

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October 20

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October 21

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October 22

I'll be there at 3-NK

ML - Gel purified Boo-Thiolase -Digested B0034 with ECO and PST -Ligated Thiolase with B0034

WM - Add arabinose promoter in front of individual genes so that each protein can be seperately expressed and purified using the His-tags we introduced.

Arabinose promoter (+AraC repressor) comes frmo I0500.

Digests:

        I725021/EcoRI+XbaI
        I725022/EcoRI+XbaI
        I725023/EcoRI+XbaI
        I725024/EcoRI+XbaI
        I725025/EcoRI+XbaI
        I0500/EcoRI+SpeI

UVP00173annot.jpg

Note: I0500 concentration is quite low. Probably need to grow it up O/N then induce O/N with IPTG after that.

Setup ligations anyway.

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October 23

WM - very few colonies from ligation Did 1 O/N from each kind of ligation/transformation for digest verification.


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October 24

WM - Digest O/Ns of arabinose + individual genes for I725021, 022, 024, 025 Digest with /XbaI+SpeI

Expected sizes (in addition to common 2149bp band):

          I725021 - 2100bp
          I725022 - 2400bp
          I725024 - 3839bp
          I725025 - 2435bp

UVP00175annot.jpg

First and last ligation looked like they worked. We will try to do this again.


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October 25

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October 26

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October 27

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October 28

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October 29

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October 30

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