User:Karmella Haynes/Notebook/BioBrick cloning/2013/01/15

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Revision as of 21:12, 16 January 2013

Karmella's BioBrick Cloning

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01/15/13

Golden gate assembly: test different ligase buffers

Golden Gate Assembly optimization

Test different buffers

Buffer	Tris-HCl	MgCl₂	DTT	ATP
10x Promega	300 mM (pH 7.8)	100 mM	100 mM	10 mM
10x NEB	500 mM (pH 7.5)	100 mM	100 mM	10 mM
2x Roche	?	?	?	?

Make Promega buffer from scratch.

Golden Gate assembly reactions

1, 2. Promega - hPCD+BL01+pSB1A3
3, 4. Promega - pSB1A3
5, 6. NEB - hPCD+BL01+pSB1A3
7, 8. NEB - pSB1A3
9, 10. Roche - hPCD+BL01+pSB1A3
11, 12. Roche - pSB1A3

Reagent	Promega (1,2)	Promega (3, 4)	NEB (5, 6)	NEB (7, 8)	Roche (9, 10)	Roche (11, 12)
gg2 pSB1A3*	1.0	1.0	1.0	1.0	1.0	1.0
gg3 hPCD*	1.0	---	1.0	---	1.0	---
gg4 BL01*	1.0	---	1.0	---	1.0	---
ligase buffer	1.0	1.0	1.0	1.0	5.0	5.0
NEB T4 ligase	0.25	0.25	0.25	0.25	0.25	0.25
NEB BsmBI	0.5	0.5	0.5	0.5	0.5	0.5
dH₂O	5.25	7.25	5.25	7.25	1.25	3.25
	10.0	10.0	10.0	10.0	10.0	10.0

Note: *DNA is 20 fmole/μL

Thermal cycler

[45°C, 2 min.; 16°C, 5 min.] x25
60°C, 20 min.
80°C, 20 min.
4°C, ∞

Transformations
- All odd samples: 50 μL DH5α-Turbo; ice 5 min.; plate on amp agar
- All even samples: 50 μL BL21 in 2.0 mL tubes; ice 2 min.; 42°C 90 sec.; add 800 μL SOC medium; shake @ 37°C 25 min.; pellet @ top speed 3 min.; resuspend in 100 μL amp liq. medium; plate on amp agar

@@ Line 24: / Line 24: @@
 | 10x NEB || 500 mM (pH 7.5) || 100 mM || 100 mM || 10 mM
 |-
-| 2x Roche  || ? || ? || ? || ? || ?
+| 2x Roche  || ? || ? || ? || ?
 |}
-----
+* Make Promega buffer from scratch.
-'''Assemblies'''
-# BioBrick name: 5' part/(a/b)/size + 3' part/(c/d)/size
-# BioBrick name: 5' part/(a/b)/size + 3' part/(c/d)/size
-* Digests (Fermentas FD)
-** Specific notes
-{| {{table}} cellspacing="3" <!-- Digest rxn. table -->
+* Golden Gate assembly reactions
+, 2. Promega - hPCD+BL01+pSB1A3<br>
+, 4. Promega - pSB1A3<br>
+, 6. NEB - hPCD+BL01+pSB1A3<br>
+, 8. NEB - pSB1A3<br>
+, 10. Roche - hPCD+BL01+pSB1A3<br>
+, 12. Roche - pSB1A3<br>
+{| {{table}} border="1" cellspacing="3" <!-- Golden Gate Rxn. table -->
 |- valign="top"
-| bgcolor=#cfcfcf | Reagent
+| Reagent || Promega (1,2)  || Promega (3, 4) || NEB (5, 6) || NEB (7, 8) || Roche (9, 10) || Roche (11, 12)
-| bgcolor=#cfcfcf | Volume
-| rowspan="7" | <!-- [[Image:GelImage.jpg|270px|Hover name]]<br>30 μL/lane, 1% agarose; [http://openwetware.org/wiki/Image:KAH_Fermentas_GeneRuler_1kbplus.jpg Ladder] -->
 |-
-| DNA (plasmid) || up to 25 μL
+| gg2 pSB1A3* || 1.0 || 1.0 || 1.0 || 1.0 || 1.0 || 1.0
 |-
-| 10x buffer || 3.0
+| gg3 hPCD* || 1.0 || --- || 1.0 || --- || 1.0 || ---
 |-
-| enzyme 1 || 1.0
+| gg4 BL01* || 1.0 || --- || 1.0 || --- || 1.0 || ---
 |-
-| enzyme 2 || 1.0
+| ligase buffer || 1.0 || 1.0|| 1.0 || 1.0|| 5.0 || 5.0
 |-
-| dH<sub>2</sub>O || ---
+| NEB T4 ligase || 0.25 || 0.25 || 0.25 || 0.25 || 0.25 || 0.25
 |-
-| &nbsp; || 30 μL --> 37°C/ ~30 min.
+| NEB BsmBI || 0.5 || 0.5 || 0.5 || 0.5 || 0.5 || 0.5
-|}
-* Measure conc.'s
-{| {{table}} cellspacing="3" <!-- [DNA] table -->
-|- bgcolor=#cfcfcf
-| Sample || OD260 || 260/280 || ng/μL
 |-
-| 1. Digested part (a/b) || --- || --- || ---
+| dH<sub>2</sub>O || 5.25 || 7.25 || 5.25 || 7.25 || 1.25 || 3.25
 |-
-| 2. Digested part (c/d) || --- || --- || ---
+| &nbsp; || 10.0 || 10.0 || 10.0 || 10.0 || 10.0 || 10.0
 |}
+Note: *DNA is 20 fmole/μL
+Thermal cycler
+* [45°C, 2 min.; 16°C, 5 min.] x25
+* 60°C, 20 min.
+* 80°C, 20 min.
+* 4°C, ∞
-* Dephosphorylation (Roche)
-{| {{table}} cellspacing="3" <!-- Dephos table -->
-|-
-| bgcolor=#cfcfcf | Reagent
-| bgcolor=#cfcfcf | Volume
-|-
-| DNA (clean digest) || up to 17 μL (500 ng)
-|-
-| 10x buffer d.p. || 2.0
-|-
-| phosphatase || 1.0
-|-
-| dH<sub>2</sub>O || ---
-|-
-| &nbsp; || 20 μL --> 37°C/ 10 min.; 75°C/ 2 min.; [final] = 25 ng/μL
-|}
+* Transformations
+** All odd samples: 50 μL '''DH5α-Turbo'''; ice 5 min.; plate on amp agar
+** All even samples: 50 μL '''BL21''' in 2.0 mL tubes; ice 2 min.; 42°C 90 sec.; add 800 μL SOC medium; shake @ 37°C 25 min.; pellet @ top speed 3 min.; resuspend in 100 μL amp liq. medium; plate on amp agar
-* Ligations
-{| {{table}} cellspacing="3" <!-- Ligations table -->
-|- bgcolor=#cfcfcf
-| Ligation || <font color="blue"><u>Plate results (lig : neg crtl)</u> mm/dd/yy</font>
-|-
-| 1. insert(a/b)/size, ## ng + vector(c/d)/size, ## ng || <font color="blue">new BioBrick #:1 (Pick #)</font>
-|-
-| 2. vector(c/d)/ ## ng || &nbsp;
-|}
-{| {{table}} cellspacing="3" <!-- Ligation rxn table -->
-| &nbsp;             || 1    || 2    ||
-|-
-| Insert DNA         || ###  || ---  ||
-|-
-| Vector DNA         || ###  || ###  ||
-|-
-| 2x lgn buf (Roche) || ###  || ###  ||
-|-
-| T4 ligase (NEB)    || 1.0  || 1.0  ||
-|-
-| dH<sub>2</sub>O    || ###  || ###  ||
-|-
-| &nbsp;             || # μL || # μL ||
-|}
 ----
-'''Oligo annealing'''
-# New BB 1
-# New BB 2
-{| class="wikitable" border="0" cellspacing="3" <!-- Oligo annealing rxn table -->
-| DNA (oligos, 100 μM) || up to 18 μL (3 μL ea.)
-|-
-| 10x annealing buffer || 2.0
-|-
-| dH<sub>2</sub>O || ---
-|-
-| &nbsp; || 20 μL --> 100°C (water bath)/ 5 min.; Cool to R.T. overnight
-|}
 <!-- ##### DO NOT edit below this line unless you know what you are doing. ##### -->

User:Karmella Haynes/Notebook/BioBrick cloning/2013/01/15

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Revision as of 21:12, 16 January 2013

01/15/13

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