Revision as of 13:46, 26 November 2012

PcTF Subcloning in E. coli

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11/16/12

---Karmella 13:51, 16 November 2012 (EST): Here is my suggested procedure for trying the PcTF fusion cloning...

Assemblies: Shown as Part/cuts/purified fragment size

KAH109/pT7CFE1-CHis: KAH109/(E/P)/1132 + pT7CFE1-CHis/(E/P)/3600
KAH111/pT7CFE1-CHis: KAH184/(E/S)/1123 + "
KAH112/pT7CFE1-CHis: KAH187/(E/S)/1123 + "
KAH115/pT7CFE1-CHis: KAH188/(E/S)/931 + "
KAH148/pT7CFE1-CHis: KAH189/(E/S)/967 + "
KAH150/pT7CFE1-CHis: KAH190/(E/S)/967 + "
KAH151/pT7CFE1-CHis: KAH191/(E/S)/967 + "

Note: KAH109 is being re-done as an internal control to trouble-shoot the ligation
Note: KAH111-KAH151 are all cut and purified already

Digest (Fermentas FD)

pT7CFE1-CHis, E/P
KAH109 E/P
KAH111 E/P
KAH112 E/P
KAH115 E/P
KAH148 E/P
KAH150 E/P
KAH151 E/P

Reagent	Volume	30 μL/lane, 1% agarose
DNA (plasmid)	25.0 μL
10x buffer	3.0
EcoRI	1.0
PstI	1.0
dH₂O	0
	30 μL --> 37°C/ ~30 min.

Measure concentration(s)

Sample	OD260	260/280	ng/μL
1. pT7CFE1-CHis (E/P)	---	1.829	57.344
2. KAH109 (E/P)	---	2.354	36.072
3. KAH111 (E/P)	---	2.238	15.003
4. KAH112 (E/P)	---	1.862	22.857
5. KAH115 (E/P)	---	2.096	18.312
6. KAH148 (E/P)	---	2.389	23.735
7. KAH150 (E/P)	---	1.99	19.822
8. KAH151 (E/P)	---	1.9	19.701

Ligations (trouble shooting suggestions)

Note: Use 50 ng of vector this time (instead of 20)
Note: Use a 3:1 ratio of insert to vector... x μL insert = 3 * (bp of insert/ bp of vector) * 50 ng vector / (concentration of insert ng/μL)

	1	2	3	4	5	6	7	8
Insert Name	KAH109	KAH111	KAH112	KAH115	KAH148	KAH150	KAH151	N/A
Insert DNA	1.3	3.12	2.05	2.12	1.7	2.03	2.05	0
Vector DNA	0.87	0.87	0.87	0.87	0.87	0.87	0.87	0.87
2x lgn buf (Roche)	5.0	5.0	5.0	5.0	5.0	5.0	5.0	5.0
T4 ligase (NEB)	1.0	1.0	1.0	1.0	1.0	1.0	1.0	1.0
dH₂O	1.83	0.01	1.08	1.01	1.43	1.1	1.08	3.13
	10 μL	10 μL	10 μL	10 μL	10 μL	10 μL	10 μL	10 μL

Plates Nomenclature

BD-116, (KAH109)
BD-117, (KAH111)
BD-118, (KAH112)
BD-119, (KAH115)
BD-120, (KAH148)
BD-121, (KAH150)
BD-122, (KAH151)
CTRL

Add total ligation reaction to 30 μL DH5α-Turbo cells
Follow routine "fast" transformation procedure
Plate onto 100 ug/mL Amp agar plates

@@ Line 27: / Line 27: @@
 '''Digest (Fermentas FD)'''<br>
 # pT7CFE1-CHis, E/P
+# KAH109 E/P
+# KAH111 E/P
+# KAH112 E/P
+# KAH115 E/P
+# KAH148 E/P
+# KAH150 E/P
+# KAH151 E/P
 {| class="wikitable" border="0" cellspacing="3" <!-- Digest rxn. table -->
 |- valign="top"
 | <u>Reagent</u> || <u>Volume</u> || &nbsp;
-| rowspan="9" | <!--- [[Image:image.tif|350px|Cloning digest ]]<br>30 μL/lane, 1% agarose --->
+| rowspan="9" |   [[Image:PcTF_in-vitro_Expression.png‎|350px|Cloning digest ]]<br>30 μL/lane, 1% agarose
 |-
 | DNA (plasmid) || 25.0 μL
@@ Line 70: / Line 77: @@
 |}
-# BD-116, (KAH109)
-# BD-117, (KAH111)
-# BD-118, (KAH112)
-# BD-119, (KAH115)
-# BD-120, (KAH148)
-# BD-121, (KAH150)
-# BD-122, (KAH151)
-# CTRL
 '''Ligations''' (trouble shooting suggestions)
@@ Line 101: / Line 100: @@
 |}
+'''Plates Nomenclature
+# BD-116, (KAH109)
+# BD-117, (KAH111)
+# BD-118, (KAH112)
+# BD-119, (KAH115)
+# BD-120, (KAH148)
+# BD-121, (KAH150)
+# BD-122, (KAH151)
+# CTRL
 * Add total ligation reaction to 30 μL DH5α-Turbo cells
 * Follow routine "fast" transformation procedure
 * Plate onto 100 ug/mL Amp agar plates

User:Behzad Damadzadeh/Notebook/PcTF Subcloning in E-coli/2012/11/16: Difference between revisions

Revision as of 13:46, 26 November 2012

11/16/12

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