|
01/25/13
- 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) -- this sample was used for the original ChIP-PCR experiments [1]
Perform End Repair
Note: forgot to dilute Klenow 1:5 with water before use
| Reagent | Volume
|
| Input DNA | 30.0 μL
|
| dH2O | 10.0
|
| T4 DNA ligase buffer | 5.0
|
| dNTP mix | 2.0
|
| T4 DNA Polymerase | 1.0
|
| Klenow DNA polymerase | 1.0
|
| T4 PNK | 1.0
|
| | 50 μL
|
--> 20°C/ 30 min. (PCR machine)
--> QIAquick PCR Purification, elute with 34 μL EB
Add 'A' Bases to the 3' End of the DNA Fragments
| Reagent | Volume
|
| DNA sample | 34.0 μL
|
| Klenow buffer | 5.0
|
| dATP | 10.0
|
| Klenow exo | 1.0
|
| | 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
|
| DNA sample | 10.0 μL
|
| DNA ligase buffer | 15.0
|
| Adapter oligo mix | 1.0
|
| DNA ligase | 4.0
|
| | 30 μL
|
--> Aliquot 20 μL to DNA samples
--> 15 min./ r.t.
--> Zymo clean and concentrator, elute with 10 μL st.dH2O
--> Store at -20°C
Day 2 (1/26/13)
Size Select the Library
> Run all samples (+ loading buffer) in a 2% TAE gel
> Use 100 bp ladder to excise area from 150 - 250
> Purify DNA with a Zymoclean Gel DNA recovery kit
> Elution: 2x 10 μL, add 16 μL st.dH2O to eluate (36 μL total)
Image:KAH012613 gel1.tif
Enrich the Adapter-Modified DNA Fragments by PCR
| Reagent | Volume | Master mix (6x)
|
| DNA | 36.0 μL | ---
|
| 5x Phusion buffer | 10.0 | 60.0
|
| dNTP mix | 1.5 | 9.0
|
| PCR primer 1.1 | 1.0 | 6.0
|
| PCR primer 2.1 | 1.0 | 6.0
|
| Phusion polymerase | 0.5 | 3.0
|
| | 50.0 μL
|
--> PCR machine (heat lid 100°C):
- 98°C, 30 sec
- 18x [98°C, 10 sec/ 65°C, 30 sec/ 72°C, 30 sec]
- 72°C, 5 min
- 4°C, ∞
--> Zymo clean and concentrator, elute with 15 μL st.dH2O
| 
Pc-TF Genomics
Main project page
Previous entry
