Team:Heidelberg/Notebook/ViroBytes/October
From 2010.igem.org
(→26/10/2010) |
(→18/10/2010) |
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*~200ng of fragment DNA per reaction | *~200ng of fragment DNA per reaction | ||
*ligation time ~10min | *ligation time ~10min | ||
+ | |||
+ | ==15/10/2010== | ||
+ | |||
+ | *Fragments 1-4; 5-8 assembly. | ||
+ | **ligation time 20-25min @ 16°C | ||
+ | **60ul of beads | ||
+ | **60ul Anchor solution (Nanodrop - 196ng/ul) | ||
+ | **2x wash with 100ul w/b buffer | ||
+ | **1x wash with 100ul 1x T4 ligase buffer | ||
+ | **gentle flicking only to dissolve the bead pellet from the wall | ||
+ | |||
+ | [[Image:Gel_546.jpg|thumb|400px|center|]] | ||
+ | |||
+ | *1 - fragments 1-4 assembly. | ||
+ | *2 - fragments control. | ||
+ | *3 - assembly ligation mix | ||
+ | *M - DNA 1kb ladder | ||
+ | *4 - fragments 5-8 assembly. | ||
+ | *5 - fragments control. | ||
+ | *6 - assembly ligation mix | ||
+ | |||
+ | ---- | ||
+ | |||
+ | ==18/10/2010== | ||
+ | |||
+ | *Fragments 1-4 assembly | ||
+ | |||
+ | |||
+ | Gel map: | ||
+ | |||
+ | *M - DNA 1kb ladder | ||
+ | *1 - control (fragments 1-4 from AAV1). | ||
+ | *2 - fragments 1-4 assembly | ||
+ | *3 - fragments 1-4 assembly (2nd reaction) | ||
+ | *4 - negative control | ||
+ | |||
+ | |||
+ | [[Image:Gel_547.png|thumb|500px|center|]] | ||
+ | |||
+ | ---- | ||
+ | |||
==25/10/2010== | ==25/10/2010== | ||
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................................................ (1x | ................................................ (1x | ||
- | 98 °C/15 s | + | 98 °C/15 s |
+ | |||
72 °C/30 s | 72 °C/30 s | ||
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4 °C/ hold | 4 °C/ hold | ||
+ | |||
+ | |||
[[Image:hot start 25102010 b.png|thumb|350px|center|fragments 5-8 of AAV2 and 1-8 of AAV6]] | [[Image:hot start 25102010 b.png|thumb|350px|center|fragments 5-8 of AAV2 and 1-8 of AAV6]] | ||
+ | |||
+ | <br /> | ||
==26/10/2010== | ==26/10/2010== | ||
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**16ul nuclease free water | **16ul nuclease free water | ||
- | ==27/ | + | ==27/10/2010== |
AAV 1 fragments 1-4; 5-8 and 1-8 (full capsid) assembly | AAV 1 fragments 1-4; 5-8 and 1-8 (full capsid) assembly |
Latest revision as of 03:57, 28 October 2010
October4/10/2010
5/10/2010
15/10/2010
18/10/2010
25/10/2010
PCR was set up as follows: 10 ul Phusion HF Buffer 5x 1ul of dNTP 0.5 ul of 100 um primers 2 ul of AAV template 36 ul of water ................................................ 98 °C/45 s ................................................ (1x 98 °C/15 s 72 °C/30 s ................................................ (35x) 72 °C/10 min ................................................ 4 °C/ hold
26/10/2010
27/10/2010AAV 1 fragments 1-4; 5-8 and 1-8 (full capsid) assembly Touchdown Phusion HiFi PCR was performed according to the following protocol: ................................................ 98 °C/30s ................................................ (1x 98 °C/15 s 72 °C/15 s (- 1.0 °C/cycle) 72 °C/1 min ................................................ (17x) 98 °C/15 s 55 °C/30 s 72 °C/1 min ................................................ (20x) 72 °C/10 min ................................................ (1x) 4 °C/ hold ................................................
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