User:Karmella Haynes/Notebook/PcTF Genomics/2013/01/25

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Revision as of 17:40, 25 January 2013

Pc-TF Genomics

Main project page

Illumina ChIP-seq prep: input DNA

Illumina ChIP-seq prep
> Follow manufacturer's protocol, with some modifications
> Sample (dated 12/04/10):

"29, FTrx fx Input" (plain cells)

Perform End Repair
Note: forgot to dilute Klenow 1:5 with water before use

Reagent	Volume	Master Mix
Input DNA	30.0 μL	---
dH₂O	10.0	60.0
T4 DNA ligase buffer	5.0	30.0
dNTP mix	2.0	12.0
T4 DNA Polymerase	1.0	6.0
Klenow DNA polymerase	1.0	6.0
T4 PNK	1.0	6.0
	50 μL

--> Aliquot 20 μL master mix, add 30 μL ChIP DNA
--> 20°C/ 30 min. (temp block)
--> QIAquick PCR Purification, elute with 34 μL EB

Add 'A' Bases to the 3' End of the DNA Fragments

Reagent	Volume	Master Mix
DNA sample	34.0 μL	---
Klenow buffer	5.0	30.0
dATP	10.0	60.0
Klenow exo	1.0	6.0
	50 μL

--> Aliquot 16 μL master mix into DNA
--> 37°C/ 30 min. (heat block)
--> Zymo clean and concentrator, elute with 10 μL st.dH₂O

Ligate Adapters to DNA Fragments
Note: Did not dilute the adapter oligo mix

Reagent	Volume	Master Mix
DNA sample	10.0 μL	---
DNA ligase buffer	15.0	90.0
Adapter oligo mix	1.0	6.0
DNA ligase	4.0	24.0
	30 μL

--> Aliquot 20 μL to DNA samples
--> 15 min./ r.t.
--> Zymo clean and concentrator, elute with 10 μL st.dH₂O
--> Store at 4°C o/n

@@ Line 8: / Line 8: @@
-==mm/dd/yy==
+==01/25/13==
 <!-- Precede finished items with a checkmark &#x2713; -->
-* Line item 1
+* Illumina ChIP-seq prep: input DNA
 ----
-'''Line item 1'''<br>
+'''Illumina ChIP-seq prep'''<br>
-> Samples
+> Follow manufacturer's protocol, with some modifications<br>
+> Sample (dated 12/04/10):
+# "29, FTrx fx Input" (plain cells)
+<br>
+<u>Perform End Repair</u><br>
+Note: forgot to dilute Klenow 1:5 with water before use
 {| class="wikitable" border="0" cellspacing="3" <!-- Rxn. table -->
 |-valign="top"
-| <u>Reagent</u> || <u>Volume</u>
+| <u>Reagent</u> || <u>Volume</u> || <u>Master Mix</u>
 |-
-| reagent 1 || # μL
+| Input DNA || 30.0 μL || ---
 |-
-| reagent 2 || #
+| dH<sub>2</sub>O || 10.0 || 60.0
 |-
-| reagent 3 || #
+| T4 DNA ligase buffer || 5.0 || 30.0
 |-
-| reagent 4 || #
+| dNTP mix || 2.0 || 12.0
 |-
-| dH<sub>2</sub>O || #
+| T4 DNA Polymerase || 1.0 || 6.0
 |-
-| &nbsp; || # μL
+| Klenow DNA polymerase || 1.0 || 6.0
+|-
+| T4 PNK || 1.0 || 6.0
+|-
+| &nbsp; || 50 μL
 |}
---> Reaction conditions
+--> Aliquot 20 μL master mix, add 30 μL ChIP DNA<br>
+--> 20°C/ 30 min. (temp block)<br>
+--> QIAquick PCR Purification, elute with 34 μL EB
+<u>Add 'A' Bases to the 3' End of the DNA Fragments</u><br>
+{| class="wikitable" border="0" cellspacing="3" <!-- Rxn. table -->
+|-valign="top"
+| <u>Reagent</u> || <u>Volume</u> || <u>Master Mix</u>
+|-
+| DNA sample || 34.0 μL || ---
+|-
+| Klenow buffer || 5.0 || 30.0
+|-
+| dATP || 10.0 || 60.0
+|-
+| Klenow exo || 1.0 || 6.0
+|-
+| &nbsp; || 50 μL
+|}
+--> Aliquot 16 μL master mix into DNA<br>
+--> 37°C/ 30 min. (heat block)<br>
+--> Zymo clean and concentrator, elute with 10 μL st.dH<sub>2</sub>O
+<u>Ligate Adapters to DNA Fragments</u><br>
+Note: Did not dilute the adapter oligo mix<br>
+{| class="wikitable" border="0" cellspacing="3" <!-- Rxn. table -->
+|-valign="top"
+| <u>Reagent</u> || <u>Volume</u> || <u>Master Mix</u>
+|-
+| DNA sample || 10.0 μL || ---
+|-
+| DNA ligase buffer || 15.0 || 90.0
+|-
+| Adapter oligo mix || 1.0 || 6.0
+|-
+| DNA ligase || 4.0 || 24.0
+|-
+| &nbsp; || 30 μL
+|}
+--> Aliquot 20 μL to DNA samples<br>
+--> 15 min./ r.t.<br>
+--> Zymo clean and concentrator, elute with 10 μL st.dH<sub>2</sub>O<br>
+--> Store at 4°C o/n
 <!-- ##### DO NOT edit below this line unless you know what you are doing. ##### -->

User:Karmella Haynes/Notebook/PcTF Genomics/2013/01/25

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Revision as of 17:40, 25 January 2013

01/25/13

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