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Latest revision as of 22:09, 29 September 2013

6 August 2013

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Lab 208

Main purpose

Extraction PCR for AMO
PCR for SPL (synthetic promoter library)
PCR for reference promoter
PCR for araBAD biobrick K808000
PCR to extract Nir2 from P. aeruginosa
PCR for araBAD and SPL with DMSO
PCR on Nir1 with MgCl2 gradient
Gel purification of Nir1 (from P. aeruginosa)
Plasmid isolation: HAO in pZA21 from USER cloning.

Who was in the lab

Kristian, Gosia, Natalia, Henrike

Procedure

PCR for AMO

Made four reactions using 1 uL respectively 10 uL of culture from the -20 or from the glycerol stock (-80) as template and adjusted volume of water accordingly.

Primers 10a, 10b.

PCR for SPL (synthetic promoter library)

PCR for reference promoter

PCR for araBAD K808000

PCR to extract Nir2 from P. aeruginosa

PCR for araBAD and SPL with DMSO

Template and primers as previous.

PCR on Nir1 with MgCl2 gradient

Used previous isolation from a gel purification to make PCR for amplification of the strand. Used 5% DMSO as additive. The PCR was done with primer pair 41 and with x7 polymerase at 55C annealing and 5:00 min extension. Also we used 20 sec as denaturing time instead of the normal 10. The magnesium gradient was as follow:

0
1uL MgCl2 2mM per 50uL reaction
5uL MgCl2 2mM per 50uL reaction
20uL MgCl2 2mM per 50uL reaction

Gel purification

of the Nir1 fragment extracted from P. aeruginosa. Nanodrop: 8ng/uL

Plasmid miniprep

HAO in pZA21 from USER cloning was purified for restriction analysis. Nanodrop measurement: 180ng/uL

Results

Gel 1

1% agarose gel

1 kb ladder
Nir1 col. Taq
Nir1 col. Taq
Nir2 col. Taq
Nir2 col. Taq
Nir1 frag. Taq
Nir1 frag. Taq
Nir1 col. x7
Nir1 col. x7
neg
Hi spec. buffer
Hi spec. buffer
DMSO
DMSO
Nir1
Nir1
Nir2
Nir2
1 kb ladder

Nir1 was purified.

Gel 2

1% agarose gel

1 kb ladder
NirW
NirW
araBAD biobrick K808000
araBAD biobrick K808000
SPL in pZA21 containing RFP
SPL in pZA21 containing RFP
reference promoter in pZA21 containing RFP
reference promoter in pZA21 containing RFP
neg
neg
1 kb ladder

Gel 3

1% agarose gel

1 kb ladder
AMO, 1uL of -20 culture as template
AMO, 10uL of -20 culture as template
AMO, 1uL of glycerol stock as template
AMO, 10uL of glycerol stock as template
neg from AMO PCR
1 - SPL, primers 52a, 52b1, template pZA21 with RFP, 50C, 2:30 min extension
2 - SPL, primers 52a, 52b1, template pZA21 with RFP, 50C, 2:30 min extension
3 - ref, primers 52a, 52b2, template pZA21 with RFP, 50C, 2:30 min extension
4 - ref, primers 52a, 52b2, template pZA21 with RFP, 50C, 2:30 min extension
5 - araBAD, primers 12a, 12bn, template K80800, 50C, 2:30 min extension
6 - araBAD, primers 12a, 12bn, template K80800, 50C, 2:30 min extension
1 kb ladder

AMO was gel purified.

Conclusion

Nir was obtained from colony PCR and purified.
AMO was extracted and gel purified.

Navigate to the Previous or the Next Entry

@@ Line 1: / Line 1: @@
 {{:Team:DTU-Denmark/Templates/StartPage|6 August 2013}}
+Navigate to the [[Team:DTU-Denmark/Notebook/5_August_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/7_August_2013|Next]] Entry
-=lab 208=
+=Lab 208=
 <hr/>
 ==Main purpose==
 <hr/>
+* Extraction PCR for AMO
+* PCR for SPL (synthetic promoter library)
+* PCR for reference promoter
+* PCR for araBAD biobrick K808000
+* PCR to extract Nir2 from ''P. aeruginosa''
+* PCR for araBAD and SPL with DMSO
+* PCR on Nir1 with MgCl2 gradient
+* Gel purification of Nir1 (from ''P. aeruginosa'')
+* Plasmid isolation: HAO in pZA21 from USER cloning.
 ==Who was in the lab==
@@ Line 13: / Line 22: @@
 <hr/>
-====PCR for AMO====
+===PCR for AMO===
 Made four reactions using 1 uL respectively 10 uL of culture from the -20 or from the glycerol stock (-80) as template and adjusted volume of water accordingly.
@@ Line 19: / Line 28: @@
 Primers 10a, 10b.
-====PCR for SPL (synthtic promoter library)====
+===PCR for SPL (synthetic promoter library)===
-template: pZa21 with RFP, primers: 52a, 52b1, temperature: 50C, time: 2:30
+template: pZA21 with RFP, primers: 52a, 52b1, temperature: 50C, time: 2:30
-====PCR for reference promoter====
+===PCR for reference promoter===
-template: pZa21 with RFP, primers: 52a, 52b2, temperature: 50C, time: 2:30
+template: pZA21 with RFP, primers: 52a, 52b2, temperature: 50C, time: 2:30
-====PCR for araBAD K808000====
+===PCR for araBAD K808000===
 template: K808000, primers: 12a, 12bn, temperature: 50C, time: 2:30
-===gel purification===
+===PCR to extract Nir2 from P. aeruginosa===
-of the Nir1 fragment extraced from P. aeruginosa
+===PCR for araBAD and SPL with DMSO===
+Template and primers as previous.
-===plasmid miniprep===
+===PCR on Nir1 with MgCl2 gradient===
+Used previous isolation from a gel purification to make PCR for amplification of the strand. Used 5% DMSO as additive. The PCR was done with primer pair 41 and with x7 polymerase at 55C annealing and 5:00 min extension. Also we used 20 sec as denaturing time instead of the normal 10.
+The magnesium gradient was as follow:
+*0
+*1uL MgCl2 2mM per 50uL reaction
+*5uL MgCl2 2mM per 50uL reaction
+*20uL MgCl2 2mM per 50uL reaction
-HAO in pZA21 from USER cloning was purified for restriction analysis
+===Gel purification===
+of the Nir1 fragment extracted from ''P. aeruginosa''. Nanodrop: 8ng/uL
+===Plasmid miniprep===
+HAO in pZA21 from USER cloning was purified for restriction analysis. Nanodrop measurement: 180ng/uL
 ==Results==
 <hr/>
+===Gel 1===
 % agarose gel
 * 1 kb ladder
-* Nir1 col. T
+* Nir1 col. Taq
-* Nir1 col. T
+* Nir1 col. Taq
-* Nir2 col. T
+* Nir2 col. Taq
-* Nir2 col. T
+* Nir2 col. Taq
-* Nir1 frag. T
+* Nir1 frag. Taq
-* Nir1 frag. T
+* Nir1 frag. Taq
-* Nir1 col. X7
+* Nir1 col. x7
-* Nir1 col. X7
+* Nir1 col. x7
 * neg
-* Hi
+* Hi spec. buffer
-* Hi
+* Hi spec. buffer
 * DMSO
 * DMSO
 * Nir1
@@ Line 66: / Line 89: @@
 [[File:2013-08-06 nir.jpg| 600px]]
+Nir1 was purified.
+===Gel 2===
 % agarose gel
@@ Line 81: / Line 107: @@
 * 1 kb ladder
-(pic small gel)
+[[File:2013-08-06 small gel.jpg|600px]]
-===Gel result:===
+===Gel 3===
-* 1 - ladder
+% agarose gel
-* 2 - sample nr 1 - SPL, primers 52a, 52b1, template pZA21 with RFP, 50C, 2:30 min extension
-* 3 - sample nr 2 - SPL, primers 52a, 52b1, template pZA21 with RFP, 50C, 2:30 min extension
+* 1 kb ladder
-* 4 - sample nr 3 - ref, primers 52a, 52b2, template pZA21 with RFP, 50C, 2:30 min extension
+* AMO, 1uL of -20 culture as template
-* 5 - sample nr 4 - ref, primers 52a, 52b2, template pZA21 with RFP, 50C, 2:30 min extension
+* AMO, 10uL of -20 culture as template
-* 6 - sample nr 5 - araBAD, primers 12a, 12bn, template K80800, 50C, 2:30 min extension
+* AMO, 1uL of glycerol stock as template
-* 7 - sample nr 6 - araBAD, primers 12a, 12bn, template K80800, 50C, 2:30 min extension
+* AMO, 10uL of glycerol stock as template
-* 8 - sample nr 7 - Nir2, extraction PCR, primers 42a, 42b, cells in water, Phusion polymerase
+* neg from AMO PCR
-* 9 - sample nr 8 - Nir2, extraction PCR, primers 42a, 42b, cells in water, Phusion polymerase
+* 1 - SPL, primers 52a, 52b1, template pZA21 with RFP, 50C, 2:30 min extension
-* 10 - sample nr 9 - Nir2, extraction PCR, primers 42a, 42b, cells in water, x7 polymerase
+* 2 - SPL, primers 52a, 52b1, template pZA21 with RFP, 50C, 2:30 min extension
-* 11 - sample nr 10 - Nir2, extraction PCR, primers 42a, 42b, cells in water, x7 polymerase
+* 3 - ref, primers 52a, 52b2, template pZA21 with RFP, 50C, 2:30 min extension
-* 12 - sample nr 11 - Nir2, extraction PCR, primers 42a, 42b, cells in water, plus MgCl2 additive, Phusion polymerase
+* 4 - ref, primers 52a, 52b2, template pZA21 with RFP, 50C, 2:30 min extension
-* 13 - sample nr 12 - - Nir2, extraction PCR, primers 42a, 42b, cells in water, plus MgCl2 additive, x7 polymerase
+* 5 - araBAD, primers 12a, 12bn, template K80800, 50C, 2:30 min extension
-* 14 - sample nr 13 - Nir1 with USER primers, primers 39a, 39b, x7, template - Nir purified from gel
+* 6 - araBAD, primers 12a, 12bn, template K80800, 50C, 2:30 min extension
-* 15 - sample nr 14 - Nir1 with USER primers, primers 39a, 39b, x7, template - Nir purified from gel
+* 1 kb ladder
-* 16 - sample nr 15 - check Nir1 with primers for NirM+S, primers 11a, 44, template - Nir purified from gel, Phusion polymerase
-* 17 - sample nr 16 - check Nir1 with primers for NirM+S, primers 11a, 44, template - Nir purified from gel, Phusion polymerase
+[[File:2013-08-06 AMO and spl.jpg| 600px]]
-* 18 - ladder
+AMO was gel purified.
 ==Conclusion==
 <hr/>
+*Nir was obtained from colony PCR and purified.
+*AMO was extracted and gel purified.
 Navigate to the [[Team:DTU-Denmark/Notebook/5_August_2013|Previous]] or the [[Team:DTU-Denmark/Notebook/7_August_2013|Next]] Entry
 {{:Team:DTU-Denmark/Templates/EndPage}}

Team:DTU-Denmark/Notebook/6 August 2013

From 2013.igem.org

Latest revision as of 22:09, 29 September 2013

6 August 2013

Contents

Lab 208

Main purpose

Who was in the lab

Procedure

PCR for AMO

PCR for SPL (synthetic promoter library)

PCR for reference promoter

PCR for araBAD K808000

PCR to extract Nir2 from P. aeruginosa

PCR for araBAD and SPL with DMSO

PCR on Nir1 with MgCl2 gradient

Gel purification

Plasmid miniprep

Results

Gel 1

Gel 2

Gel 3

Conclusion

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