Revision as of 11:44, 17 September 2015

NOTEBOOK

December

9.12.-13.12. We filled a survey to become next generation of ATOMS members.

Waiting in excitement and wondering who will be the members of this year’s team.

22.12. Aaaaand the results of the interviews we made are announced! Now we’re a crowded team of 25 people. Let’s see what’ll happen next.

26.12. Had our first meeting and our first topic was: sponsorship.

January

We had training classes at 08.01-10.01. January. Now it is time to learn what iGEM wants from us.

10.01.-23.01. We made researches about previous iGEM teams, wondering who did what.

23.01.-28.01. Hooray! It’s holiday! Home sweet home.

It’s time to find our own project. After now, we started to have meetings every Monday and Thursday, becase we need to work a lot for finding a new project. Also, still trying to find sponsors.

February

01.02. As we are ATOMS, those Sundays needed to be filled too! We made subgroups in our team and started to search previous Grand Prized-Teams. Now every group will present a team at the meetings.

We have just built ATOMS gene library.

02.02. We decided to attend some competitions due to the lack of sponsors. We attended ‘illnesses with imagery’. Talented people is a must in a team.

13.02. Drawings were done and sent. We believe we will be successful. We are still doing researches in full swing.

March

05.03. Today they filmed our school, and our laboratory so. We had so much fun while they were shooting us!

11.03. The art competiton’s results are just announced. Disappointment. There was not even a winner of first place. We convinced ourselves with thinking they don’t have a sense of art.

14.03. We made a biobrcik design workshop till we see the sunlight! At the late times of night, every group explained their biobrick designs. Now everyone knows what a promoter is :)

17.03. Lab-cleaning party! We don’t wanna be contaminated.

April

05.04. We bid farewell to our teammate Furkan Beştepe. He went to USA.

10.04. Happy birthday Gülnihal! By the way your birthday cake was yummy.

12.04. Daytime wasn’t enough so we started to have meetings in the nights! After working a lot, we deserved eating a delicious meal. Today we also started to search about Toehold.

13.04. We are still learnig about Toehold. It has a potential to be used.

27.04. Fun at the lab.

30.04. ATOMS Ladieas worked on a universal blood idea till the morning.

May

03.05. We must hurry up to find a project. Camp time at Asya Thermal Hotel.

04.05. Why there isn’t anyone in the lab?

06.05. Finally found our project idea! ULCER AND CANCER

09.05. Perfecting our cancer switch system.

15.05. Presented our project to the dean Mehmet Gündüz and the whole genetic department of our faculty! He treated us with Turkish tea and snacks.

24.05. We held a meet-up with other Turksih iGEM teams! Time to make some presentations.

June

This month we designed our genes and studied for our exams at the same time. In short it was a tough week.

Week 1

Gradient PCR of „pCAG with CMV-Enhancer FWD/Cβ-Actin REV. Primers” (29.06.2015)

Gradient PCR from pCAGGS
	MgCl₂	(NH₄)2SO₄	VR fwd	VR rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	16.3 ul	2.0 ul	25.0 ul
9X	22.5 ul	22.5 ul	4.5 ul	4.5 ul	4.5 ul	1.8 ul	146.7 ul	18.0 ul	225.0 ul

57-64˚C

Results weren’t matching with expected results, experiment will be repeated.

(30.06.2015)

Gradient PCR from pCAGGS
	MgCl₂	(NH₄)2SO₄	VR fwd	VR rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	16.3 ul	2.0 ul	25.0 ul
9X	22.5 ul	22.5 ul	4.5 ul	4.5 ul	4.5 ul	1.8 ul	146.7 ul	18.0 ul	225.0 ul

52-59˚C

Results weren’t matching with expected results, experiment will be repeated.

July

01.07. Some preparetions were made for experiments.

05.07. Today is the first day of shooting. We just learned picking costumes isn’t as easy as we think.

06.07. If there is a film, then there is After Effects work to do. Good luck with this, dear teammate Şahika.

08.07. We made a presentation to the pre-med students which came from USA for intership and they loved our project.

21.07. Drawing pictures for wiki began. Thus we discovered our teammate Kevser’s hidden talents.

22.07. Our gene blocks has just arrived. Let the experiments begin! We are all ready now.

29.07. We released our first video of Virtual Hospital. Also arm’s design is finished.

Week 2

Gradient PCR of „pCAG with CAG FWD/CAG REV. Primers/pCMV REV.” (01.07.2015) {| border="1" class="wikitable" !Gradient PCR from pCAGGS (CAG FWD – CAG REVERSE) |- |||MgCl₂||(NH₄)2SO₄||VR fwd||VR rv||dNTP||Tag||ddH₂O||DNA||Total |- |1x||2.5 ul||2.5 ul||0.5 ul||0.5 ul||0.5 ul||0.2 ul||16.3 ul||2.0 ul||25.0 ul |- |9X||22.5 ul||22.5 ul||4.5 ul||4.5 ul||4.5 ul||1.8 ul||146.7 ul||18.0 ul||225.0 ul |}

60-68˚C

Results weren’t matching with expected results, experiment will be repeated.

Gradient PCR from pCAGGS (CAG FWD – Chicken β Aktin REVERSE)
	MgCl₂	(NH₄)2SO₄	VR fwd	VR rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	16.3 ul	2.0 ul	25.0 ul
9X	22.5 ul	22.5 ul	4.5 ul	4.5 ul	4.5 ul	1.8 ul	146.7 ul	18.0 ul	225.0 ul

60-68˚C

Results weren’t matching with expected results, experiment will be repeated.

GEL GÖRÜNTÜSÜ

Protocols of „Phusion Pol, and Q5 Polymerase” (02.07.2015)

Phusion DNA Polymerase
	dNTP	Fwd primer	Rev primer	Buffer	Phusion Pol.	ddH₂O	DNA	Total
1x	0.4 ul	2.0 ul	2.0 ul	4.0 ul	0.2 ul	10.4 ul	1.0 ul	20.0 ul

Cycling
	98˚C	98˚C	56˚C	72˚C	72˚C	Cycle
Time	2’	10’’	30’’	1’	5’	35x

Q5 DNA Polymerase
	dNTP	Fwd primer	Rev primer	Buffer	Q5 Pol.	ddH₂O	DNA	Total
1x	0.5 ul	2.5 ul	2.5 ul	5.0 ul	0.25 ul	8.25 ul	1.0 ul	20.0 ul

Cycling
	98˚C	98˚C	56˚C	72˚C	72˚C	Cycle
Time	2’	10’’	30’’	1’	5’	35x

Defterde jel görüntüsü yok.

Week 3

Gradient PCR of „pCAG with CAG-FWD/CAG REV. Primers and Phusion Pol.” (07.07.2015)

Gradient PCR from pCAGGS
	dNTP	Fwd primer	Rev primer	Buffer	Phusion Pol.	ddH₂O	DNA	Total
1x	0.4 ul	2.0 ul	2.0 ul	4.0 ul	0.2 ul	10.4 ul	1.0 ul	20.0 ul

62-64˚C

Result: Gel extraction was performed. PCR (+): 680 bp

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	eb	biospec	7/8/2015 1:56:43 AM	0.1	ng/ul	0.002	-0.009	-0.25	-0.19	DNA	50.00
2	pCAG	biospec	7/8/2015 1:58:14 AM	13.7	ng/ul	0.275	0.138	1.98	0.15	DNA	50.00

Creating “Plasmid pCAG” via “pTRE” and “Promoter pCAG” (09.07.2015)

Digestion of “pTRE” and “Promoter pCAG”
	pTRE (1536 ng/ul)	pCAG (promoter) (13.7 ng/ul)	EcoRI	XhoI	Neb 3.1 Buffer	ddH₂O	Total
1	3.2 ul	-	0.5 ul	0.5 ul	2.0 ul	13.8 ul	20.0 ul
2	-	10.0 ul	0.5 ul	0.5 ul	2.0 ul	7.0 ul	20.0 ul

pTRE-delta-TRE was made after digestion.

Concentration: 99.9 ng/ul

The final concentration of pCAG is 6.855 ng/ul.

Ligation of „pTRE TRE“ and „Digested promoter pCAG“

	pTRE TRE
pCAG	T4 DNA Ligase	Buffer	ddH₂O	Total
1:1	3.0 ul	7.0 ul	0.5 ul	2.0 ul	7.5 ul	20.0 ul

Ligation products were transformed into E.Coli/BL321 strain.

Result: No colonies were observed.

Digestion of “pTEToff and pET45 Vectors” (10.07.2015)

Digestion of “pTEToff and pET45 Vectors”
	pTEToff (1141 ng/ul)	pET45 (485 ng/ul)	XhoI (Neb)	BamHI (Neb)	SalI (Thermo)	HindIII (Thermo)	Cut Smart Buffer	Fast Digest Buffer	ddH₂O	Total
1	3.1 ul	-	-	-	0.5 ul	0.5 ul	-	2.0 ul	13.9 ul	20.0 ul	37˚C 1h
2	-	4.1 ul	0.5 ul	0.5 ul	-	-	2.0 ul	-	12.9 ul	20.0 ul	37˚C 2h

Result: Bands were at the expected section. Gel extraction was made.

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	eb	biospec	7/10/2015 11:37:54 PM	-0.4	ng/ul	-0.008	-0.015	0.58	-0.39	DNA	50.00
2	pET45 x+b	biospec	7/10/2015 11:40:59 PM	59.0	ng/ul	1.180	0.612	1.93	0.74	DNA	50.00
3	pTEToff s+h	biospec	7/10/2015 11:41:58 PM	55.5	ng/ul	1.110	0.581	1.91	0.25	DNA	50.00

Creating “Plasmid pCAG” via “pTRE” and “Promoter pCAG” – Repeat (08.07.2015)

Digestion of “pTRE with EcoRI/XhoI”
	pTRE	XhoI	EcoRI	Neb 2.1 Buffer	ddH₂O	Total
1	3.2 ul	0.5 ul	0.5 ul	2.0 ul	13,8 ul	20.0 ul	37˚C 2h
2	3.2 ul	0.5 ul	0.5 ul	2.0 ul	13,8 ul	20.0 ul	37˚C 2h/0.5 ul CIP/37˚C 30’/50˚C 30’

Result: Gel extraction was made.

GEL GÖRÜNTÜSÜ

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	eb	biospec	7/9/2015 6:32:17 PM	-0.7	ng/ul	-0.015	-0.022	0.66	0.21	DNA	50.00
2	hre cmv mini	biospec	7/9/2015 6:34:10 PM	13.8	ng/ul	0.277	0.141	1.97	0.03	DNA	50.00
3	ptre delta tre cip -	biospec	7/9/2015 6:34:54 PM	88.7	ng/ul	1.774	0.941	1.88	0.24	DNA	50.00
4	ptre delta tre cip +	biospec	7/9/2015 6:35:35 PM	86.0	ng/ul	1.721	0.947	1.82	0.25	DNA	50.00

Creating “Plasmid pCAG” – Continue (12.07.2015)

Ligation of „pTRE TRE“ and „Digested promoter pCAG“

	pTRE TRE CIP (+)	pTRE TRE CIP (-)	pCAG (6.85 ng/ul)	T4 DNA Ligase	Buffer	ddH₂O	Total
1	3.0 ul	-	7.0 ul	0.5 ul	2.0 ul	7.5 ul	20.0 ul
2	-	3.0 ul	7.0 ul	0.5 ul	2.0 ul	7.5 ul	20.0 ul

Room Temperature 1h

Sonuc: Transformation was made. No colonies were observed at first plate. At the second plate there was five colonies. Colony PCR will be made.

Week 4

Creating “Plasmid pCAG” – Continue (13.07.2015)

Colony PCR from “pCAG” with “pTRE Luc fwd/SV40 polyA re. primers”
	MgCl₂	(NH₄)2SO₄	pTRE Luc fwd	SV40 rev	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	1.0 ul	1.0 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	25.0 ul
6X	15.0 ul	15.0 ul	6.0 ul	6.0 ul	3.0 ul	1.2 ul	73.8 ul		120.0 ul

Cycling
	95˚C	95˚C	55˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Result: All bands were observed around 700 bp, results were negative. Ligation will be repeated.

(+) bant: 923 bp

(-) bant: 705 bp

GEL GÖRÜNTÜSÜ
Creating “Plasmid pCAG” – Repeat (19.07.2015)

Ligation of „pTRE TRE“ and „Digested Promoter pCAG“

	pTRE TRE CIP (+)	pTRE TRE CIP (-)	pCAG (6.85 ng/ul)	T4 DNA Ligase	Buffer	ddH₂O	Total
1	3.0 ul	-	2.5 ul	0.5 ul	2.0 ul	12.0 ul	20.0 ul
2	-	3.0 ul	2.5 ul	0.5 ul	2.0 ul	12.0 ul	20.0 ul

Vector:Insert

3:1

RT 2h

Transformation at BL21.

CIP (+): No colonies were absorved.

CIP (-): Colony PCR will be made.

Week 5

Creating “Plasmid pCAG” – Continue (20.07.2015)

Colony PCR from “pCAG” with “pTRE Luc fwd/SV40 polyA re. primers”
	MgCl₂	(NH₄)2SO₄	pTRE Luc fwd	SV40 rev	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	1.0 ul	1.0 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	25.0 ul
6X	15.0 ul	15.0 ul	6.0 ul	6.0 ul	3.0 ul	1.2 ul	73.8 ul		120.0 ul

Cycling
	95˚C	95˚C	55˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Result: All bands were observed around 700 bp, results were negative. Ligation will be repeated.

(+) bant: 923 bp

(-) bant: 705 bp

GEL GÖRÜNTÜSÜ
Creating “pCAG (Plasmid) – Repeat (23.07.2015)

PCR from “pCAGGS”
	dNTP	CAG fwd	CAG rev	Chicken β Akt. Rev	pCAGGS	Phusion Pol	Buffer	ddH₂O	Total
1	2.0 ul	10.0 ul	10.0 ul	-	5.0 ul	1.0 ul	20.0 ul	52.0 ul	100.0 ul
2	2.0 ul	10.0 ul	-	10.0 ul	5.0 ul	1.0 ul	20.0 ul	52.0 ul	100.0 ul

Cycling
	98˚C	98˚C	64/68˚C	72˚C	72˚C	Cycle
Time	2’	10’’	30’’	1’	5’	35x

Gel Extraction will made.

GEL GÖRÜNTÜSÜ

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	eb	biospec	7/23/2015 6:56:38 PM	0.2	ng/ul	0.005	0.005	0.92	0.14	DNA	50.00
2	pcag e	biospec	7/23/2015 6:58:03 PM	42.9	ng/ul	0.858	0.450	1.91	1.97	DNA	50.00
3	pcag y	biospec	7/23/2015 6:58:53 PM	23.3	ng/ul	0.466	0.233	2.00	1.94	DNA	50.00

Resuspension of “Newly Arrived G-Blocks from IDT” (S. 23/23.7.2015)

100 ul TE for all tubes.

		ng	fmol	TE ul	fmol/ul	ul of inserts for 75 fmol
1	Toehold for cola	1000	1523	100	15.23	4.92449
2	TnrA-pTnrA-RFP	1000	1032	100	10.32	7.26744
3	ColA-KanR-dTer	1000	816	100	8.16	9.19118
4	HNS for PET	500	1578	100	15.78	4.75285
5	HNS-T108I for PET	500	1578	100	15.78	4.75285
6	potB59-pomA for PET	1000	892	100	8.92	8.40807
7	Gad E – for PET	500	1291	100	12.91	5.80945
8	TlpB for PET	1000	901	100	9.01	8.32408
9	DAMP-Pex for PET/pcolA	1000	2089	100	20.89	3.59023
10	Tev Protease for PET	1000	1948	100	19.48	3.8501
11	miRNA switch- miR373- BS for pTET	500	2212	100	22.12	3.3906
12	LacO- DsRed- miR26a-375 pC	1000	1709	100	17.09	4.38853
13	mLacI-miR373 BS for pTRE	1000	1280	100	12.8	5.85938
14	miRNA switch- miR 21 BS- miR 223	1000	1902	100	19.02	3.94322
15	mLacI-miR223 BS miR 21 BS for pTRE	1000	1272	100	12.72	5.89623
16	Trigger RNA for pSB1C3	250	1910	100	19.1	3.9267
17	PsicA for pSB1C3	1000	1546	100	15.46	4.86
18	MVF-sicA for ColA	1000	1042	100	10.42	7.20

Not: 100ng pSB1C3 (2050 bp) ≈ 75 fmol
Digestion of „G-Blocks from IDT and pSB1C3“ (23.07.2015)

Digestion
	Insert	EcoRI-HF	PstI	NEB 2.1 Buffer	ddH₂O	Total
1x	10.0 ul	1.0 ul	1.0 ul	2.0 ul	6.0 ul	20.0 ul
17x	10.0 ul	17.0 ul	17.0 ul	34.0 ul	102.0 ul	20.0 ul

Digestion
	Vector	EcoRI-HF	PstI	NEB 2.1 Buffer	ddH₂O	Total
2x	17.0 ul	1.0 ul	1.0 ul	2.0 ul	-	21.0 ul

Result: Gel extraction was made.

GEL GÖRÜNTÜSÜ
PCR of “G-Blocks from IDT” (24.07.2015)

PCR from G-Bloks
	MgCl₂	(NH₄)2SO₄	CMV fwd	SV40 rev	tetR rev	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	25.0 ul
3x (pTEToff)	7.5 ul	7.5 ul	1.5 ul	-	1.5 ul	1.5 ul	1.6 ul	36.9 ul		58.0 ul
15x	37.5 ul	37.5 ul	7.5 ul	7.5 ul	-	7.5 ul	3.0 ul	184.5 ul		285.0 ul

Cycling for 3x
	95˚C	95˚C	57˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Cycling for 15x
	95˚C	95˚C	60˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Results: Bands were at the expected section.

GEL GÖRÜNTÜSÜ
Gel Extraction (24.07.2015)

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	7/24/2015 12:40:09 PM	-0.8	ng/ul	-0.016	-0.020	0.79	0.24	DNA	50.00
2	pSB1C3	biospec	7/24/2015 12:41:56 PM	42.2	ng/ul	0.848	0.430	1.97	2.05	DNA	50.00

Ligation of „G-Blocks from IDT and pSB1C3“ (24.07.2015)

Ligation
	Insert DNA	Vector (pSB1C3)	T4 DNA Buffer	T4 DNA Ligase	ddH₂O	Total
1	4.9 ul	2.5 ul	2.0 ul	1.0 ul	9.8 ul	20.0 ul
2	7.2 ul	2.5 ul	2.0 ul	1.0 ul	7.3 ul	20.0 ul
3	9.2 ul	2.5 ul	2.0 ul	1.0 ul	5.3 ul	20.0 ul
4	4.8 ul	2.5 ul	2.0 ul	1.0 ul	9.7 ul	20.0 ul
5	4.8 ul	2.5 ul	2.0 ul	1.0 ul	9.7 ul	20.0 ul
6	8.4 ul	2.5 ul	2.0 ul	1.0 ul	6.1 ul	20.0 ul
7	5.8 ul	2.5 ul	2.0 ul	1.0 ul	8.7 ul	20.0 ul
8	4.9 ul	2.5 ul	2.0 ul	1.0 ul	9.6 ul	20.0 ul

RT 1h

Transformation was made.

(The results of psb1c3 gel extraction was lower. So we performed only the first 7 gene ligation.)

1	Toehold for cola
2	TnrA-pTnrA-RFP
3	ColA-KanR-dTer
4	HNS for PET
5	HNS-T108I for PET
6	potB59-pomA for PET
7	Gad E – for PET
8	TlpB for cola (NEB1)

Creating “Plasmid pCAG”

Digestion
	pTRE (1536 ng/ul)	pCAG (promoter) E	pCAG (promoter) Y	EcoRI	XhoI	Cut Smart Buffer	ddH₂O	Total
1	3.2 ul	-	-	0.5 ul	0.5 ul	2.0 ul	13.8 ul	20.0 ul	37˚C 2h
2	-	10 ul	-	0.5 ul	0.5 ul	2.0 ul	7.0 ul	20.0 ul	37˚C 2h
3	-	-	10 ul	0.5 ul	0.5 ul	2.0 ul	7.0 ul	20.0 ul	37˚C overnight

Bands were at the expected section. Gel extraction wil be made.

The Final Concentration

pCAG E: 21.5 ng/ul

pCAG Y: 12 ng/ul

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	eb	biospec	7/25/2015 5:03:57 AM	1.4	ng/ul	0.028	0.006	4.60	0.48	DNA	50.00
2	eb	biospec	7/25/2015 5:05:57 AM	0.0	ng/ul	0.000	-0.012	-0.03	0.06	DNA	50.00
3	ptre delta tre	biospec	7/25/2015 5:07:44 AM	194.0	ng/ul	3.880	2.033	1.91	2.20	DNA	50.00

Colony PCR of “pSB1C3 – GBlocks” (25.07.2015)

PCR from “pCAGGS”
	PCR MM	VR fwd	VR rev	ddH₂O	Tag	DNA	Total
1x	14.0 ul	1.0 ul	1.0 ul	7.5 ul	0.2 ul	5.0 ul	28.7 ul
33x	462.0 ul	33.0 ul	33.0 ul	247.5 ul	6.6 ul	165.0 ul	940.5 ul
33x	462.0 ul	33.0 ul	33.0 ul	247.5 ul	6.6 ul	165.0 ul	940.5 ul

Cycling
	95˚C	95˚C	56˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Sonuc: 8-3 ve 4-9 bands were at the expected section. Liquid Culture was made.

GEL GÖRÜNTÜLERI
Colony PCR of “G-Blocks” (25.07.2015)

Colony PCR of “2,3,6,8”
	MgCl₂	(NH₄)2SO₄	CMV fwd	SV40 rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	24.0 ul
6X	15.0 ul	15.0 ul	3.0 ul	3.0 ul	3.0 ul	1.2 ul	73.8 ul		114.0 ul

Colony PCR of “7,10,12,13”
	MgCl₂	(NH₄)2SO₄	CMV fwd	SV40 rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	24.0 ul
6X	15.0 ul	15.0 ul	3.0 ul	3.0 ul	3.0 ul	1.2 ul	73.8 ul		114.0 ul

Colony PCR of “1,4,9,15”
	MgCl₂	(NH₄)2SO₄	CMV fwd	SV40 rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	13.3 ul	5.0 ul	25.0 ul
6X	15.0 ul	15.0 ul	3.0 ul	3.0 ul	3.0 ul	1.2 ul	79.8 ul		120.0 ul

Colony PCR of “5,16”
	MgCl₂	(NH₄)2SO₄	CMV fwd	SV40 rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	13.3 ul	5.0 ul	25.0 ul
2X	5.0 ul	5.0 ul	1.0 ul	1.0 ul	1.0 ul	0.4 ul	26.6 ul		40.0 ul

Cycling
	95˚C	95˚C	60˚C	72˚C	72˚C	Cycle
Time	5’	30’’	2’	1.5’	5’	35x

G-Blocks PCR / Gel Electrophoresis (25.07.2015)

PCR
	MgCl₂	(NH₄)2SO₄	CMV fwd	TetR rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	13.3 ul	5.0 ul	25.0 ul
6X	15.0 ul	15.0 ul	3.0 ul	3.0 ul	3.0 ul	1.2 ul	79.8 ul		120.0 ul

Cycling
	95˚C	95˚C	60˚C	72˚C	72˚C	Cycle
Time	5’	30’’	2’	1.5’	5’	35x

Result: negative

GEL GÖRÜNTÜSÜ

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	7/26/2015 7:04:13 PM	0.8	ng/ul	0.016	-0.014	-1.13	1.36	DNA	50.00
2	blank	biospec	7/26/2015 7:05:51 PM	-0.4	ng/ul	-0.009	-0.017	0.52	0.17	DNA	50.00
3	colony pcr 8-3	biospec	7/26/2015 7:07:15 PM	87.9	ng/ul	1.758	0.908	1.94	2.09	DNA	50.00
4	colony pcr 4-9	biospec	7/26/2015 7:08:09 PM	101.4	ng/ul	2.027	1.089	1.86	1.74	DNA	50.00
5	colony pcr 4-9	biospec	7/26/2015 7:09:06 PM	71.4	ng/ul	1.429	0.749	1.91	1.96	DNA	50.00
6	colony pcr 8-3	biospec	7/26/2015 7:10:03 PM	87.9	ng/ul	1.758	0.910	1.93	2.10	DNA	50.00
7	colony pcr 4-9	biospec	7/26/2015 7:11:01 PM	57.1	ng/ul	1.142	0.596	1.91	1.77	DNA	50.00
8	colony pcr 4-9	biospec	7/26/2015 7:12:18 PM	77.2	ng/ul	1.543	0.820	1.88	1.76	DNA	50.00

Colony PCR of “pSB1C3- GBlocks” (26.07.2015)

Gradient PCR from pCAGGS
	MgCl₂	(NH₄)2SO₄	VR fwd	VR rv	dNTP	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	1.0 ul	1.0 ul	0.5 ul	12.3 ul	5.0 ul	25.0 ul
41X	102.5 ul	102.5 ul	41.0 ul	41.0 ul	20.5 ul	504.3 ul		881.8 ul

Cycling
	95˚C	95˚C	56˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Result: negative

Digestion of “pTEToff” (26.07.2015)

Digestion
	pTEToff (1141 ng/ul)	SalI (Thermo)	HindIII (Thermo)	Fast Digest Buffer	ddH₂O	Total
Volume	3.1 ul	0.5 ul	0.5 ul	2.0 ul	13.9 ul	20.0 ul

37˚C 1h

Result: Bands were at the expected section. Gel purification was made.

GEL GÖRÜNTÜSÜ

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	7/26/2015 4:18:56 PM	0.3	ng/ul	0.005	-0.010	-0.56	-0.38	DNA	50.00
2	Ptetoff SalI hindIII	biospec	7/26/2015 4:20:23 PM	43.3	ng/ul	0.866	0.452	1.92	0.88	DNA	50.00

Creating “Plasmid pCAG” – Continue (27.07.2015)

Ligation of „pTRE TRE“ and „Digested pCAG“

	pTRE TRE (194 ng/ul)	pCAG E (21.5 ng/ul)	pCAG Y (12.0 ng/ul)	T4 DNA Ligase	Buffer	ddH₂O	Total
1	1.0 ul	2.0 ul	-	0.5 ul	2.0 ul	14.5 ul	20.0 ul
2	1.0 ul	-	3.6 ul	0.5 ul	2.0 ul	12.9 ul	20.0 ul

Result: On the first plate was six colonies. On the second plate was nine colonies.

Colony PCR will be made.
Colony PCR of „pCAG (plasmid)“

PCR
	MgCl₂	(NH₄)2SO₄	pTRE Luc fwd	SV40 rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	1.0 ul	1.0 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	25.0 ul
16X	40.0 ul	40.0 ul	16.0 ul	16.0 ul	8.0 ul	3.2 ul	196.8 ul		320.0 ul

Cycling
	95˚C	95˚C	55˚C	72˚C	72˚C	Cycle
Time	5’	30’’	2’	1.5’	5’	35x

</html>

Result: negative

GEL GÖRÜNTÜSÜ

Colony PCR of “pSB1C3 – Gblocks” (27.07.2015) {| border="1" class="wikitable" !PCR |- |||MgCl₂||(NH₄)2SO₄||VR fwd||VR rv||dNTP||Tag||ddH₂O||DNA||Total |- |1x||2.5 ul||2.5 ul||1.0 ul||1.0 ul||0.5 ul||0.2 ul||12.3 ul||5.0 ul||25.0 ul |- |57X||143.0 ul||143.0 ul||57.0 ul||57.0 ul||29.0 ul||11.4 ul||701.0 ul||||1141.4 ul |- |57X||143.0 ul||143.0 ul||57.0 ul||57.0 ul||29.0 ul||11.4 ul||701.0 ul||||1141.4 ul |} {| border="1" class="wikitable" !Cycling |- |||95˚C||95˚C||56˚C||72˚C||72˚C||Cycle |- |Time||5’||30’’||30’’||1.5’||5’||35x |}

Sonuc: Only 16-9 is positive.

GEL GÖRÜNTÜLERI
Colony PCR of “pSB1C3 – Gblocks” (28.07.2015)

Colony PCR of “2,3,8,9,11,13,14”
	MgCl₂	(NH₄)2SO₄	VR fwd	VR rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	1.0 ul	1.0 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	25.0 ul
66X	165.0 ul	165.0 ul	66.0 ul	66.0 ul	33.0 ul	13.2 ul	811.8 ul		1650.0 ul

Cycling
	95˚C	95˚C	56˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Result: negative

GEL GÖRÜNTÜLERI
Digestion of “HNS, HNS-T108I, potB59-pomA, GadE, TlpB, DAMP-Pex, Tev Protease” (27.07.2015)

Inserts from GBlocks were digested to ligate with PET45.

	4	5	6	7	8	9	10
HNS (4)	10.0 ul	-	-	-	-	-	-
HNS-T108I (5)	-	10.0 ul	-	-	-	-	-
potB59-pomA (6)	-	-	10.0 ul	-	-	-	-
GadE (7)	-	-	-	10.0 ul	-	-	-
TlpB (8)	-	-	-	-	10.0 ul	-	-
DAMP-Pex (9)	-	-	-	-	-	10.0 ul	-
Tev Protease (10)	-	-	-	-	-	-	10.0 ul
Cut Smart Buffer	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul
₂XhoI	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul
BamHI-HF	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul
Milli-Q	7.0 ul	7.0 ul	7.0 ul	7.0 ul	7.0 ul	7.0 ul	7.0 ul

Total: 20 ul

37˚C overnight

Ligation will be made.
Ligation of “GBlocks (4,5,6,7,8,10)” and “PET45 (X+B)”

	4	5	6	7	8	10
Insert DNA	4.75 ul	4.75 ul	4.75 ul	4.75 ul	4.75 ul	4.75 ul
Vector (PET45)	2.20 ul	2.20 ul	.,20 ul	2.20 ul	2.20 ul	2.20 ul
Buffer	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul
T4 DNA Ligase	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul	0.5 ul
ddH₂O	10.55 ul	10.55 ul	10.55 ul	10.55 ul	10.55 ul	10.55 ul
Total	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul

Room Temperature 2h

	11	14
Insert DNA	3.4 ul	3.95 ul
Vector (PET45)	2.20 ul	2.20 ul
Buffer	2.0 ul	2.0 ul
T4 DNA Ligase	0.5 ul	0.5 ul
ddH₂O	11.9 ul	11.35 ul
Total	20.0 ul	20.0 ul

</html> Room Temperature 2h

Creating of “pTRE – mLacI miRNA-BS” (27.07.2015) </html>

Digestion of “pTRE” and G-Blocks”
	pTRE	EcoRI-HF	BamHI-HF	mLacI-miR 373 BS	mLacI-miR (21-223) BS	Cut Smart	ddH₂O	Total
1	3.1 ul	0.5 ul	0.5 ul	-	-	2.0 ul	13.9 ul	20.0 ul	37˚C-3h Gel Elect.
2	-	0.5 ul	0.5 ul	10.0 ul	-	2.0 ul	7.0 ul	20.0 ul	37˚C overnight/80˚C-10’ heat inactivation
3	-	0.5 ul	0.5 ul	-	10.0 ul	2.0 ul	7.0 ul	20.0 ul	37˚C overnight/80˚C-10’ heat inactivation

Gel purification was made.

GEL GÖRÜNTÜSÜ

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	7/27/2015 2:26:05 PM	0.3	ng/ul	0.007	-0.004	-1.71	0.20	DNA	50.00
2	pTRE e+b	biospec	7/27/2015 2:27:08 PM	92.9	ng/ul	1.859	1.015	1.83	1.24	DNA	50.00

Creating of “pTRE – mLacI miRBS” (27.07.2015)

Ligation of „pTRE” and “mLacI miRBS”
	Digested pTRE	D. mLacI miR373 BS	D. mLacI miR(21-223) BS	T4 DNA Ligase	T4 DNA Buffer	ddH₂O	Total
1	1.0 ul	5.9 ul	-	2.0 ul	0.5 ul	10.6 ul	20.0 ul
2	1.0 ul	-	5.9 ul	2.0 ul	0.5 ul	10.6 ul	20.0 ul

Room Temperature 2h

Transformation was made with TOP10.
Creating of “pTEToff – miRBS” (27.07.2015)

Digestion
	pTEToff (2.5 ng/ul)	miRNA switch miR373 BS	miRNA switch miR(223-21) BS	SalI (FD)	HindIII (FD)	Fast Digest Buffer	ddH₂O	Total
1	2.0 ul	-	-	0.5 ul	0.5 ul	5.0 ul	42.0 ul	50.0 ul	37˚C-3h Gel Elect.
2	-	10.0 ul	-	0.5 ul	0.5 ul	2.0 ul	7.0 ul	20.0 ul	37˚C overnight/80˚C-10’ heat inactivation
3	-	-	10.0 ul	0.5 ul	0.5 ul	2.0 ul	7.0 ul	20.0 ul	37˚C overnight/80˚C-10’ heat inactivation

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	7/27/2015 8:35:05 PM	0.0	ng/ul	0.000	-0.013	-0.01	0.01	DNA	50.00
2	pTRE s+h	biospec	7/27/2015 8:36:16 PM	76.7	ng/ul	1.534	0.810	1.89	1.05	DNA	50.00

Creating of “pTEToff – miRNA Switch miR BS” (28.07.2015)

Ligation of „pTRE” and “mLacI miRBS”
	Digested pTEToff	D. mLacI miR373 BS	D. mLacI miR(21-223) BS	T4 DNA Ligase	T4 DNA Buffer	ddH₂O	Total
1	2.2 ul	3.4 ul	-	2.0 ul	0.5 ul	10.9 ul	20.0 ul
2	2.2 ul	-	4.0 ul	2.0 ul	0.5 ul	11.3 ul	20.0 ul

Room Tempretare 2h

Transformation was made.
Creating of “pCAG”

Digestion of “pCAG (Promotor)”
	pCAG (promoter) E	pCAG (promoter) Y	EcoRI-HF	XhoI-HF	Cut Smart Buffer	ddH₂O	Total
1	10.0 ul	-	0.5 ul	0.5 ul	2.0 ul	7.0 ul	20.0 ul	37˚C overnight
2	-	10.0 ul	0.5 ul	0.5 ul	2.0 ul	7.0 ul	20.0 ul	37˚C overnight

Mini Prep of “Colony PCR 16-9” {| border="1" class="wikitable" !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor |- |1||blank||biospec||7/28/2015 12:11:17 PM||-1.9||ng/ul||-0.038||-0.049||0.77||0.19||DNA||50.00 |- |2||blank||biospec||7/28/2015 12:12:22 PM||-0.4||ng/ul||-0.007||-0.014||0.53||0.30||DNA||50.00 |- |3||colony pcr 16-9||biospec||7/28/2015 12:13:33 PM||84.9||ng/ul||1.698||0.881||1.93||2.02||DNA||50.00 |- |4||colony pcr 16-9||biospec||7/28/2015 12:14:24 PM||76.3||ng/ul||1.527||0.797||1.92||1.95||DNA||50.00 |}
Mini Prep of “pTEToff”

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	7/30/2015 4:44:01 PM	0.4	ng/ul	0.008	-0.005	-1.55	1.11	DNA	50.00
2	ptetoff neb	biospec	7/30/2015 4:45:00 PM	442.2	ng/ul	8.884	4.683	1.89	2.20	DNA	50.00
3	ptetoff bl21	biospec	7/30/2015 4:46:08 PM	314.3	ng/ul	6.286	3.317	1.90	2.22	DNA	50.00

Cut Check of “HNS toehold and Trigger RNA” (30.07.2015) {| border="1" class="wikitable" !!!HNS (70 ng/ul)!!TlpB (87 ng/ul)!!Trigger RNA (80 ng/ul)!!EcoRI (Thermo)!!PstI (Thermo)!!Fast Digest Buffer!!ddH₂O!!Total!! |- |1||3.5 ul||-||-||1.0 ul||1.0 ul||2.0 ul||12.5 ul||20.0 ul||37˚C 20min |- |2||-||3.0 ul||-||1.0 ul||1.0 ul||2.0 ul||13.0 ul||20.0 ul||37˚C 20min |- |3||-||-||3.0 ul||1.0 ul||1.0 ul||2.0 ul||13.0 ul||20.0 ul||37˚C 20min |}

Gel Electropheres was made.

Result: Bands were at the expected section.

HNS: 480 bp

tgRNA:˞ 100bp

Toehold: ˃1000bp

GEL GÖRÜNTÜSÜ
Colony PCR of „9-10 GBlocks“ (31.07.2015)

Result: negative

Expected: ˞1100 bp

Observed: ˞300 bp

Gel extraction 1-6

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	8/2/2015 12:01:41 AM	0.2	ng/ul	0.004	-0.002	-2.02	17.14	DNA	50.00
2	psb1c3	biospec	8/2/2015 12:31:14 AM	43.0	ng/ul	0.861	0.462	1.87	0.94	DNA	50.00

Gel extraction 8-9

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	8/2/2015 12:27:36 AM	-0.4	ng/ul	-0.009	-0.012	0.74	-0.09	DNA	50.00
2	psb1c3 atoms	biospec	8/2/2015 12:34:11 AM	10.4	ng/ul	0.208	0.111	1.87	0.03	DNA	50.00

Colony PCR of „pSB1C3 – Gblocks“

Colony PCR
	MgCl₂	(NH₄)2SO₄	VR fwd	VR rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	0.5 ul	0.5 ul	0.5 ul	0.2 ul	13.3 ul	5.0 ul	25.0 ul
17X	42.5 ul	42.5 ul	8.5 ul	8.5 ul	8.5 ul	3.4 ul	226.1 ul		340.0 ul

Cycling
	95˚C	95˚C	56˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Result: negative

GEL GÖRÜNTÜLERI

August

11.08. We started designing our wiki.

18.08.2015 We got a little tired of doing experiments, so treated ourselves with an awesome team dinner at a fish restaurant.

22.08.2015 A team dinner again, but this time our dear professors Mehmet and Esra Gündüz hosted us at their house.

29.08.2015 Wiki’s tour part is drawn, now it’s time to color these drawings!

Week 6

Mini Prep of “pSB1C3-RFP”

#	Sample ID	User name	Date and Time	Nucleic Acid Conc.	Unit	A260	A280	260/280	260/230	Sample Type	Factor
1	blank	biospec	8/1/2015 6:03:37 PM	-0.1	ng/ul	-0.003	-0.009	0.30	0.12	DNA	50.00
2	psb1c3-A	biospec	8/1/2015 6:06:00 PM	207.0	ng/ul	4.140	2.184	1.90	2.11	DNA	50.00
3	psb1c3-B	biospec	8/1/2015 6:07:07 PM	209.0	ng/ul	4.179	2.210	1.89	2.19	DNA	50.00
4	psb1c3-C	biospec	8/1/2015 6:08:05 PM	157.3	ng/ul	3.147	1.664	1.89	2.09	DNA	50.00
5	psb1c3-D	biospec	8/1/2015 6:08:58 PM	242.5	ng/ul	4.851	2.548	1.90	2.11	DNA	50.00
6	psb1c3-E	biospec	8/1/2015 6:09:42 PM	116.4	ng/ul	2.329	1.215	1.92	2.17	DNA	50.00
7	psb1c3-F	biospec	8/1/2015 6:10:28 PM	236.4	ng/ul	4.729	2.503	1.89	2.17	DNA	50.00
8	psb1c3-71	biospec	8/1/2015 6:11:33 PM	111.7	ng/ul	2.233	1.175	1.90	2.10	DNA	50.00
9	psb1c3-72	biospec	8/1/2015 6:12:14 PM	106.4	ng/ul	2.127	1.100	1.93	2.23	DNA	50.00
10	psb1c3-8	biospec	8/1/2015 6:12:51 PM	90.7	ng/ul	1.814	0.959	1.89	1.98	DNA	50.00

Ligation of „pSB1C3 – Gblocks“ (02.08.2015)

	2	3	5	6	7	8	9	10	11	12	13	14	15
Insert	7.3 ul	7.0 ul	4.8 ul	8.4 ul	5.8 ul	8.3 ul	3.6 ul	3.9 ul	3.4 ul	4.4 ul	5.9 ul	3.9 ul	5.9 ul
Vector	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul
Buffer	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul	2.0 ul
Enzyme	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul	1.0 ul
ddH₂O	7.7 ul	8.0 ul	10.2 ul	6.6 ul	9.2 ul	6.7 ul	11.4 ul	11.1 ul	11.6 ul	10.6 ul	9.1 ul	11.1 ul	9.1 ul
Total	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul	20.0 ul

Week 6 Colony PCR of „pSB1C3 – Gblocks“ (03.08.2015)

Colony PCR
	MgCl₂	(NH₄)2SO₄	VR fwd	VR rv	dNTP	Tag	ddH₂O	DNA	Total
1x	2.5 ul	2.5 ul	1.0 ul	1.0 ul	0.5 ul	0.2 ul	12.3 ul	5.0 ul	25.0 ul
22X	55.0 ul	55.0 ul	22.0 ul	22.0 ul	11.0 ul	4.4 ul	271.0 ul		440.4 ul

Cycling
	95˚C	95˚C	56˚C	72˚C	72˚C	Cycle
Time	5’	30’’	30’’	1.5’	5’	35x

Difference between revisions of "Team:ATOMS-Turkiye/Extras/Notebook"

Revision as of 11:44, 17 September 2015

Team ATOMS-Turkiye

atoms2015@googlegroups.com

NOTEBOOK

December

January

February

March

April

May

June

July

August

@@ Line 369: / Line 369: @@
-</html>{| border="1" class="wikitable"
+</html>
+{| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
 |-
@@ Line 381: / Line 382: @@
 Creating “Plasmid pCAG” via “pTRE” and “Promoter pCAG” (09.07.2015)
-</html>{| border="1" class="wikitable"
+</html>
+{| border="1" class="wikitable"
 !Digestion of “pTRE” and “Promoter pCAG”
 |-
@@ Line 499: / Line 501: @@
 <p>Sonuc: Transformation was made. No colonies were observed at first plate. At the second plate there was five colonies. Colony PCR will be made.</p>
-</div>
-</section>
-     <a href="week1" class="clickme" id="toggle" onclick="toggle_visibility('1');">Week 4<img src="https://static.igem.org/mediawiki/2014/f/f8/LMU14_arrow_down.png" id="1" class="tiger"></a>
+     <a href="#" class="clickme" id="toggle" onclick="toggle_visibility('4');">Week 4<img src="https://static.igem.org/mediawiki/2014/f/f8/LMU14_arrow_down.png" id="1" class="tiger"></a>
 <div class="box">
@@ Line 556: / Line 556: @@
-</html>
-</div>
-</section>
-<section class="accordion">
+    <a href="#" class="clickme" id="toggle" onclick="toggle_visibility('5');">Week 5<img src="https://static.igem.org/mediawiki/2014/f/f8/LMU14_arrow_down.png" id="1" class="tiger"></a>
-          <div>
-            <input id="july-week4" name="july-week4" type="checkbox" />
+<div class="box">
-            <label for="july-week4">Week 4, 20.07.-26.07.-31.07.</label>
-            <article class="ac-small">
-</html>
 Creating “Plasmid pCAG” – Continue (20.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Colony  PCR from “pCAG” with “pTRE Luc fwd/SV40 polyA re. primers”
@@ Line 585: / Line 582: @@
 |Time||5’||30’’||30’’||1.5’||5’||35x
 |}
+<html>
 <p>Result: All bands were observed around 700 bp, results were negative. Ligation will be repeated.</p>
 	<p>(+) bant: 923 bp</p>
@@ Line 593: / Line 591: @@
 Creating “pCAG (Plasmid) – Repeat (23.07.2015)
-{| border="1" class="sortable"
+</html>
+{| border="1" class="wikitable"
 !PCR from “pCAGGS”
 |-
@@ Line 610: / Line 609: @@
 |Time||2’||10’’||30’’||1’||5’||35x
 |}
+<html>
 <p>Gel Extraction will made.</p>
 GEL GÖRÜNTÜSÜ
@@ Line 615: / Line 615: @@
 <br>
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 624: / Line 625: @@
 |3||pcag y||biospec||7/23/2015 6:58:53 PM||23.3||ng/ul||0.466||0.233||2.00||1.94||DNA||50.00
 |}
+<html>
 <br>
@@ Line 629: / Line 631: @@
 Resuspension of “Newly Arrived G-Blocks from IDT” (S. 23/23.7.2015)
 <p>100 ul TE for all tubes.</p>
+</html>
 {| border="1" class="wikitable"
 !!!!!ng!!fmol!!TE ul!!fmol/ul!!ul of inserts for 75 fmol
@@ Line 668: / Line 671: @@
 |18||MVF-sicA for ColA||1000||1042||100||10.42||7.20
 |}
+<html>
 Not: 100ng pSB1C3 (2050 bp) ≈ 75 fmol
@@ Line 674: / Line 678: @@
 Digestion of „G-Blocks from IDT and pSB1C3“ (23.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Digestion
@@ Line 691: / Line 696: @@
 |2x||17.0 ul||1.0 ul||1.0 ul||2.0 ul||-||21.0 ul
 |}
+<html>
 <p>Result: Gel extraction was made.</p>
 GEL GÖRÜNTÜSÜ
@@ Line 697: / Line 703: @@
 PCR of “G-Blocks from IDT” (24.07.2015)
+</html>
 {| border="1" class="wikitable"
 !PCR from G-Bloks
@@ Line 724: / Line 731: @@
 |Time||5’||30’’||30’’||1.5’||5’||35x
 |}
+<html>
 <p>Results: Bands were at the expected section.</p>
 GEL GÖRÜNTÜSÜ
@@ Line 730: / Line 738: @@
 Gel Extraction (24.07.2015)
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 738: / Line 746: @@
 |2||pSB1C3||biospec||7/24/2015 12:41:56 PM||42.2||ng/ul||0.848||0.430||1.97||2.05||DNA||50.00
 |}
+<html>
 <br>
 Ligation of „G-Blocks from IDT and pSB1C3“ (24.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Ligation
@@ Line 763: / Line 773: @@
 |8||4.9 ul||2.5 ul||2.0 ul||1.0 ul||9.6 ul||20.0 ul
 |}
+<html>
 <p>RT 1h</p>
@@ Line 768: / Line 779: @@
 <p>(The results of psb1c3 gel extraction was lower. So we performed only the first 7 gene ligation.)</p>
+</html>
 {| border="1" class="wikitable"
 !1!!Toehold for cola
@@ Line 785: / Line 797: @@
 |8||TlpB for cola (NEB1)
 |}
+<html>
 <br>
 Creating “Plasmid pCAG”
+</html>
 {| border="1" class="wikitable"
 !Digestion
@@ Line 800: / Line 814: @@
 |3||-||-||10 ul||0.5 ul||0.5 ul||2.0 ul||7.0 ul||20.0 ul||37˚C overnight
 |}
+<html>
 <p>Bands were at the expected section. Gel extraction wil be made.</p>
 <p>The Final Concentration</p>
@@ Line 807: / Line 822: @@
 <br>
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 816: / Line 832: @@
 |3||ptre delta tre ||biospec||7/25/2015 5:07:44 AM||194.0||ng/ul||3.880||2.033||1.91||2.20||DNA||50.00
 |}
+<html>
 <br>
 Colony PCR of “pSB1C3 – GBlocks”  (25.07.2015)
+</html>
 {| border="1" class="wikitable"
 !PCR from “pCAGGS”
@@ Line 839: / Line 857: @@
 |Time||5’||30’’||30’’||1.5’||5’||35x
 |}
+<html>
 <p>Sonuc: 8-3 ve 4-9 bands were at the expected section. Liquid Culture was made.</p>
@@ Line 846: / Line 865: @@
 Colony PCR of “G-Blocks” (25.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Colony PCR of “2,3,6,8”
@@ Line 893: / Line 913: @@
 |Time||5’||30’’||2’||1.5’||5’||35x
 |}
+<html>
 <br>
 G-Blocks PCR / Gel Electrophoresis (25.07.2015)
+</html>
 {| border="1" class="wikitable"
 !PCR
@@ Line 915: / Line 937: @@
 |}
+<html>
 <p>Result: negative</p>
 GEL GÖRÜNTÜSÜ
+</html>
 {| border="1" class="wikitable"
@@ Line 938: / Line 962: @@
 |}
+<html>
 <br>
 Colony PCR of “pSB1C3- GBlocks” (26.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Gradient PCR from pCAGGS
@@ Line 959: / Line 985: @@
 |}
+<html>
 <p>Result: negative</p>
@@ Line 964: / Line 991: @@
 Digestion of “pTEToff” (26.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Digestion
@@ Line 971: / Line 999: @@
 |Volume||3.1 ul||0.5 ul||0.5 ul||2.0 ul||13.9 ul||20.0 ul
 |}
+<html>
 <p>37˚C 1h</p>
 <p>Result: Bands were at the expected section. Gel purification was made.</p>
@@ Line 977: / Line 1,006: @@
 <br>
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 985: / Line 1,015: @@
 |}
+<html>
 <br>
 Creating “Plasmid pCAG” – Continue  (27.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Ligation of „pTRE   TRE“ and „Digested pCAG“
@@ Line 1,000: / Line 1,032: @@
 |}
+<html>
 <p>Result: On the first plate was six colonies. On the second plate was nine colonies.</p>
 Colony PCR will be made.
@@ Line 1,006: / Line 1,039: @@
 Colony PCR of „pCAG (plasmid)“
+</html>
 {| border="1" class="wikitable"
 !PCR
@@ Line 1,024: / Line 1,058: @@
 |}
+</html>
 <p>Result: negative</p>
 GEL GÖRÜNTÜSÜ
@@ Line 1,030: / Line 1,065: @@
 Colony PCR of “pSB1C3 – Gblocks” (27.07.2015)
+<html>
 {| border="1" class="wikitable"
 !PCR
@@ Line 1,050: / Line 1,086: @@
 |}
+<html>
 <p>Sonuc: Only 16-9 is positive.</p>
 GEL GÖRÜNTÜLERI
@@ Line 1,056: / Line 1,093: @@
 Colony PCR of “pSB1C3 – Gblocks” (28.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Colony PCR of “2,3,8,9,11,13,14”
@@ Line 1,074: / Line 1,112: @@
 |}
+<html>
 <p>Result: negative</p>
 GEL GÖRÜNTÜLERI
@@ Line 1,081: / Line 1,120: @@
 Digestion of “HNS, HNS-T108I, potB59-pomA, GadE, TlpB, DAMP-Pex, Tev Protease” (27.07.2015)
 <p>Inserts from GBlocks were digested to ligate with PET45.</p>
-tab2wiki
+</html>
-Tools
-Git
-Talk
-Powered by Wikimedia Labs
-Copy the following into the wiki - done!
 {| border="1" class="wikitable"
 !!!4!!5!!6!!7!!8!!9!!10
@@ Line 1,113: / Line 1,147: @@
 |}
+<html>
 <p>Total: 20 ul</p>
 <p>37˚C overnight</p>
@@ Line 1,120: / Line 1,155: @@
 Ligation of “GBlocks (4,5,6,7,8,10)” and “PET45 (X+B)”
+</html>
 {| border="1" class="wikitable"
 !!!4!!5!!6!!7!!8!!10
@@ Line 1,137: / Line 1,172: @@
 |}
+<html>
 Room Temperature 2h
 <br>
+</html>
 {| border="1" class="wikitable"
 !!!11!!14
@@ Line 1,157: / Line 1,194: @@
 |}
+</html>
 Room Temperature 2h
@@ Line 1,162: / Line 1,200: @@
 Creating of “pTRE – mLacI miRNA-BS” (27.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Digestion of “pTRE” and G-Blocks”
@@ Line 1,174: / Line 1,213: @@
 |}
+<html>
 <p>Gel purification was made.</p>
 GEL GÖRÜNTÜSÜ
@@ Line 1,179: / Line 1,219: @@
 <br>
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 1,187: / Line 1,228: @@
 |}
+<html>
 <br>
 Creating of “pTRE – mLacI miRBS” (27.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Ligation of „pTRE” and “mLacI miRBS”
@@ Line 1,199: / Line 1,242: @@
 |2||1.0 ul||-||5.9 ul||2.0 ul||0.5 ul||10.6 ul||20.0 ul
 |}
+<html>
 <p>Room Temperature 2h</p>
 Transformation was made with TOP10.
@@ Line 1,205: / Line 1,249: @@
 Creating of “pTEToff – miRBS” (27.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Digestion
@@ Line 1,217: / Line 1,262: @@
 |}
+<html>
 <br>
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 1,227: / Line 1,274: @@
 |}
+<html>
 <br>
 Creating of “pTEToff – miRNA Switch miR BS” (28.07.2015)
+</html>
 {| border="1" class="wikitable"
 !Ligation of „pTRE” and “mLacI miRBS”
@@ Line 1,239: / Line 1,288: @@
 |2||2.2 ul||-||4.0 ul||2.0 ul||0.5 ul||11.3 ul||20.0 ul
 |}
+<html>
 <p>Room Tempretare 2h</p>
 Transformation was made.
@@ Line 1,245: / Line 1,295: @@
 Creating of “pCAG”
+</html>
 {| border="1" class="wikitable"
 !Digestion of “pCAG (Promotor)”
@@ Line 1,255: / Line 1,306: @@
 |}
+<html>
 <br>
 Mini Prep of “Colony PCR 16-9”
+<html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 1,270: / Line 1,323: @@
 |}
+<html>
 <br>
 Mini Prep of “pTEToff”
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 1,283: / Line 1,338: @@
 |}
+<html>
 <br>
 Cut Check of “HNS toehold and Trigger RNA” (30.07.2015)
+<html>
 {| border="1" class="wikitable"
 !!!HNS (70 ng/ul)!!TlpB (87 ng/ul)!!Trigger RNA (80 ng/ul)!!EcoRI (Thermo)!!PstI (Thermo)!!Fast Digest Buffer!!ddH₂O!!Total!!
@@ Line 1,296: / Line 1,353: @@
 |}
+<html>
 <p>Gel Electropheres was made.</p>
 <p>Result: Bands were at the expected section.</p>
@@ Line 1,313: / Line 1,371: @@
 Gel extraction 1-6
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 1,321: / Line 1,380: @@
 |}
+<html>
 <br>
 Gel extraction 8-9
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 1,332: / Line 1,393: @@
 |}
+<html>
 <br>
 Colony PCR of „pSB1C3 – Gblocks“
+</html>
 {| border="1" class="wikitable"
 !Colony PCR
@@ Line 1,353: / Line 1,416: @@
 |}
+<html>
 <p>Result: negative</p>
 GEL GÖRÜNTÜLERI
-<html>
 </div>
 </section>
-</div>
@@ Line 1,377: / Line 1,436: @@
 <p>29.08.2015 Wiki’s tour part is drawn, now it’s time to color these drawings!</p>
-<html>
-    <div style="margin-bottom:60px">
+  <a href="#" class="clickme" id="toggle" onclick="toggle_visibility('6');">Week 6<img src="https://static.igem.org/mediawiki/2014/f/f8/LMU14_arrow_down.png" id="1" class="tiger"></a>
-      <section class="accordion">
-          <div>
-            <input id="august-week0" name="august-week0" type="checkbox" />
+<div class="box">
-            <label for="august-week0">Week 1, 01.08.-02.08.</label>
-            <article class="ac-small">
-</html>
 Mini Prep of “pSB1C3-RFP”
+</html>
 {| border="1" class="wikitable"
 !#!!Sample ID!!User name!!Date and Time!!Nucleic Acid Conc.!!Unit!!A260!!A280!!260/280!!260/230!!Sample Type!!Factor
@@ Line 1,411: / Line 1,468: @@
 |}
+<html>
 <br>
 Ligation of „pSB1C3 – Gblocks“ (02.08.2015)
+</html>
 {| border="1" class="wikitable"
 !!!2!!3!!5!!6!!7!!8!!9!!10!!11!!12!!13!!14!!15!!
@@ Line 1,434: / Line 1,493: @@
-</section>
+      <a href="#" class="clickme" id="toggle" onclick="toggle_visibility('6');">Week 6<img src="https://static.igem.org/mediawiki/2014/f/f8/LMU14_arrow_down.png" id="1" class="tiger"></a>
-    <section class="accordion">
-          <div>
-            <input id="august-week1" name="august-week1" type="checkbox" />
-            <label for="august-week1">Week 2, 03.08.-09.08.</label>
-            <article class="ac-small">
-</html>
 Colony PCR of „pSB1C3 – Gblocks“ (03.08.2015)
+</html>
 {| border="1" class="wikitable"
 !Colony PCR
@@ Line 1,462: / Line 1,516: @@
 |}
-<p>Result: negative</p>
+<html>
 <br>
@@ Line 1,472: / Line 1,524: @@
-</section>
 </div>