Team:Heidelberg/Templates/Del week14 FG

From 2013.igem.org

(Difference between revisions)

Latest revision as of 18:41, 3 October 2013

1 29-07-2013
2 30-07-2013
- 2.1 Amplification from FS_21 to FS_26 ; 5.5 kb
3 31-07-2013
- 3.1 Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 29-07-2013) with XmaI
4 02-08-2013
- 4.1 Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 30-07-2013) with ClaI
5 07-08-2013
- 5.1 Amplification from FS_21 to FS_26 ; 5.5 kb

29-07-2013

Amplification from FS_21 to FS_24 ; (WRONG PRIMER!)

Amplifications of DelFG (29.07); run at 100 V, 0.8 % gel (TAE)

Amplifications of DelFG (29.07) cut

Reaction

what	µl
D. acidovorans DSM-39	1
FS_21: (1/10)	2
FS_24: (1/10)	2
Phusion flash Master Mix	10
DMSO	1
dd H₂O	4

Conditions

Biorad MyCycler*
Cycles	temperature [°C]	Time [s]
1	98	10
30	98	1
	55	5
	72	2:30
1	72	8 min
1	12	inf

Results:

PCR product occured, though wrong primers were used, unspecific binding of primers in the genome of D. Acidovorans is the putative reason for this event

Amplification from FS_21 to FS_24; (WRONG PRIMER!)

Amplification of DelFG (FS21 to FS26; 29.07); run at 100 V, 0.8 % gel (TAE)

Amplification of DelFG (FS21 to FS26; 29.07) cut

Reaction

what	µl
D. acidovorans DSM-39	1
FS_21: (1/10)	2
FS_24: (1/10)	2
Phusion flash Master Mix	10
DMSO	1
dd H₂O	4

Conditions

Biorad T100
Cycles	temperature [°C]	Time [s]
1	98	10
30	98	1
	58	5
	72	2:30
1	72	8 min
1	12	inf

Results:

PCR product occured, though wrong primers were used, unspecific binding of primers in the genome of D. Acidovorans is the putative reason for this event

Amplification from FS_21 to FS_24; (WRONG PRIMER!)

Amplification of DelFG (FS21 to FS26; 29.07); run at 100 V, 0.8 % gel (TAE)

Amplification of DelFG (FS21 to FS26; 29.07) cut

Reaction

what	µl
D. acidovorans DSM-39	1
FS_21: (1/10)	2
FS_24: (1/10)	2
Phusion flash Master Mix	10
DMSO	1
dd H₂O	4

Conditions

Biorad T100
Cycles	temperature [°C]	Time [s]
1	98	10
35	98	1
	60	5
	72	2:30
1	72	8 min
1	12	inf

Results:

PCR product occured, though wrong primers were used, unspecific binding of primers in the genome of D. Acidovorans is the putative reason for this event

Amplification from FS_06/FS_20/FS_21 to FS_26 ; 5.5 kb

Amplifications of DelFG (29.07); run at 100 V, 0.8 % gel (TAE)

Amplifications of DelFG (29.07) cut

3x20µl

Reaction

what	µl
D. acidovorans DSM-39	1
FS_06 or FS_20 or FS_21: (1/10)	2
FS_26: (1/10)	2
Phusion flash Master Mix	10
DMSO	1
dd H₂O	4

Conditions

Biorad T100
Cycles	temperature [°C]	Time [s]
1	98	10
30	98	1
	64	5
	72	2:15
1	72	10 min
1	10	inf

Results:

PCR product occured, though wrong primers were used, unspecific binding of primers in the genome of D. Acidovorans is the putative reason for this event
Furthermore, amplification with FS_21 to FS_26 led to the intended product and satisfying specifity
Amplification will be repeated at the same annealing temperature to obtain the amount of PCR product required for Gibson Assembly
Amplfication will be repeated at lower annealing temperature to increase the yield
bands were cut out and DNA purified using QIAquick Gel Extraction Kit

30-07-2013

Amplification from FS_21 to FS_26 ; 5.5 kb

Amplification of DelFG (FS21 to FS26; 30.07) at 60°C and 64°C; run at 100 V, 0.8 % gel (TAE)

Amplification of DelFG (FS21 to FS26; 30.07) cut

3x20µl with conditions I, 2x20µl with conditions II

Reaction

what	µl
D. acidovorans DSM-39	1
FS_21: (1/10)	2
FS_26: (1/10)	2
Phusion flash Master Mix	10
DMSO	1
dd H₂O	4

Conditions I

Biorad T100
Cycles	temperature [°C]	Time [s]
1	98	10
30	98	1
	64	5
	72	2:15
1	72	10 min
1	10	inf

Conditions II

Biometra TProfessional Basic
Cycles	temperature [°C]	Time [s]
1	98	10
30	98	1
	60	5
	72	2:15
1	72	10 min
1	10	inf

Results:

Amplification of DelFG was successful
bands were cut out and DNA purified using QIAquick Gel Extraction Kit
restriction digest with XmaI will be conducted to validate the PCR product

31-07-2013

Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 29-07-2013) with XmaI

Restriction digest of FS21 to FS26 (29.7) with XmaI; run at 100 V, 0.8 % gel (TAE)

Incubation at 37°C for about 3 hours

what	µl
FS_21 to FS_26 (29-07-2013)	17
XmaI	1
Buffer CutSmart	2
Expected fragment lengths [bp]	4268, 1202

Results:

Restriction digest of DelFG with XmaI did not lead to the expected result
digest will be carried out with a different enzyme, as the used one was outdated and digest might therefore not be very reliable

02-08-2013

Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 30-07-2013) with ClaI

Restriction digest of FS21 to FS26 (30.7) with ClaI; run at 100 V, 0.8 % gel (TAE)

Incubation at 37°C for about 3 hours

what	µl
FS_21 to FS_26 (30-07-2013)	~15
ClaI	1
Buffer CutSmart	2
Expected fragment lengths [bp]	2743, 1519, 1208

Results:

Restriction digest of DelFG did not display any product
digest will be repeated with higher amount of DNA after new amplification from the genome of D. Acidovorans

07-08-2013

Amplification from FS_21 to FS_26 ; 5.5 kb

Amplifcation of DelAF(I), DelFG, DelG (07.08); run at 100 V, 0.8 % gel (TAE)

Amplifcation of DelAF(I), DelFG, DelG (07.08), cut

Reaction

what	µl
D. acidovorans SPH-1	1
FS_21: (1/10)	2
FS_26: (1/10)	2
Phusion flash Master Mix	10
DMSO	1
dd H₂O	4

Conditions

Biorad MyCycler
Cycles	temperature [°C]	Time [s]
1	98	10
30	98	1
	60	5
	72	2:15
1	72	10 min
1	10	inf

Results:

Amplification of DelFG was successful, gel displays highly specific product of convincing yield
bands were cut out and DNA purified using QIAquick Gel Extraction Kit
restriction digest with ClaI will be conducted to validate PCR product

@@ Line 270: / Line 270: @@
 ==31-07-2013==
-===Restriction digest of fragment from FS_21 to FS_26; 5.5 kb; [[DelF-G#29-07-2013|29-07-2013]]) with XmaI===
+===Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 29-07-2013) with XmaI===
 [[File:Heidelberg_20130801 2log restrictiondigest.FG.XmaIbesch.png|100px|thumb|Restriction digest of FS21 to FS26 (29.7) with XmaI; run at 100 V, 0.8 % gel (TAE)]]
 Incubation at 37°C for about 3 hours
@@ Line 277: / Line 277: @@
 ! what !! µl
 |-
-| FS_21 to FS_26 ([[DelF-G#29-07-2013|29-07-2013]]) || 17
+| FS_21 to FS_26 (29-07-2013) || 17
 |-
 | XmaI || 1
 |-
 | Buffer CutSmart || 2
+|-
+| Expected fragment lengths [bp]|| 4268, 1202
 |}
@@ Line 293: / Line 295: @@
-===Restriction digest of of fragment from FS_21 to FS_26; 5.5 kb; [[DelF-G#30-07-2013|30-07-2013]]) with ClaI===
+===Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 30-07-2013) with ClaI===
 [[File:Heidelberg_20130802 DelRest Verdau Sophiebesch.png|100px|thumb|Restriction digest of FS21 to FS26 (30.7) with ClaI; run at 100 V, 0.8 % gel (TAE)]]
 Incubation at 37°C for about 3 hours
@@ Line 300: / Line 302: @@
 ! what !! µl
 |-
-| FS_21 to FS_26 ([[DelF-G#30-07-2013|30-07-2013]]) || ~15
+| FS_21 to FS_26 (30-07-2013) || ~15
 |-
 | ClaI || 1
 |-
 | Buffer CutSmart || 2
+|-
+| Expected fragment lengths [bp]|| 2743, 1519, 1208
 |}
 '''Results:'''

Team:Heidelberg/Templates/Del week14 FG

From 2013.igem.org

Latest revision as of 18:41, 3 October 2013

Contents

29-07-2013

Amplification from FS_21 to FS_24 ; (WRONG PRIMER!)

Amplification from FS_21 to FS_24; (WRONG PRIMER!)

Amplification from FS_21 to FS_24; (WRONG PRIMER!)

Amplification from FS_06/FS_20/FS_21 to FS_26 ; 5.5 kb

30-07-2013

Amplification from FS_21 to FS_26 ; 5.5 kb

31-07-2013

Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 29-07-2013) with XmaI

02-08-2013

Restriction digest of fragment FS_21 to FS_26 (5.5 kb; 30-07-2013) with ClaI

07-08-2013

Amplification from FS_21 to FS_26 ; 5.5 kb