Introduction of EMSA Electrophoretic Migration Shift Experiment

Experimental principle

Gel Migration or Electrophoretic Mobility Assay (EMSA) is a technique for studying the interaction of DNA-binding proteins with their associated DNA-binding sequences for qualitative and quantitative analysis. This technique was originally used to study DNA binding proteins and has been used to study the interaction of RNA binding proteins with specific RNA sequences.

The purified protein and the crude cell extract are typically incubated with a 32P isotopically labeled DNA or RNA probe, and the complex and unbound probe are separated on non-denaturing polypropylene gel electrophoresis. DNA-complexes or RNA-complexes move slower than unbound probes. Isotopically labeled probes may be double-stranded or single-stranded depending on the binding protein being studied. When detecting a DNA binding protein such as a transcriptional regulatory factor, a purified protein, a partially purified protein, or a nuclear cell extract can be used. In the detection of RNA-binding proteins, purified or partially purified proteins may be used depending on the position of the RNA-binding protein of interest, and nuclear or cytoplasmic cell extracts may also be used. In competition experiments, DNA or RNA fragments and oligonucleotide fragments (specific) containing protein-binding sequences, and other unrelated fragments (non-specific) are used to determine the specificity of DNA or RNA-binding proteins. Specific binding is determined in the presence of competitive specific and non-specific fragments based on the characteristics and strength of the complex.

Experimental reagent
Important reagents:
Boitin-N4-CTP (invitrogen # 15918-18)
TdT (NEB # M0252L)
Poly(dI.dC) (sigma #P4929)
Hybond-N nylon membrane (Amersham #RPN303B)
Luminescent substrate (Ningbo Weiao)

Buffer:
Buffer A (store at 4Â°C)
Hepes (pH7.9) 10mM
KCl 10mM
EDTA 0.1mM
DTT (fresh added) 1mM
PMSF (fresh added) 0.5mM
Buffer B (store at 4Â°C)
0.5M EDTA in PBS (pH 7.4)
Buffer C (store at 4Â°C)
Hepes (pH7.9) 20mM
NaCl 0.4M
EDTA 1mM
DTT (fresh added) 1mM
PMSF (fresh added) 1mM
Buffer I (store at RT)
Tris (pH 7.5) 0.1M
NaCl 1M
MgCl ₂ Â 2mM
Buffer II (pH7.5) (store at RT)
Maleic acid 100mM
NaCl 150mM
Buffer III (store at RT)
Tris (pH 9.5) 100mM
NaCl 100mM
MgCl ₂ 50mM
Blocking Buffer (store at 4Â°C)
0.3% Tween-20, 0.3% Triton X-100, 5% BSA in Buffer I
Wash Buffer
0.3% Tween-20 in Buffer II
20Ã—SSC (1L pH7.0)
NaCl 175.3g
Sodium citrate 88.2g

10Ã—Binding Buffer (store at -20Â°C) [Buy in the company (Biyuntian): 5Ã—binding buffer with Poly(dI.dC)]
Tris (pH 7.5) 0.1M
KCl 0.5M
DTT 10Mm
Poly(dI.dC) (store at -20Â°C)
1mg/ml in TE (pH7.5)
SA-HRP (store stock at -20 Â°C working solution at 4 Â° C)
1mg/ml in 50% PBS (pH7.2) 50% Glycerin
5Ã—TBE (5L)
EDTA 18.612g
Boric acid 139.1175g
Tris 272.565g
5Ã—TdT Reaction Buffer (store at -20Â°C) (pH7.2)
Sodium cacodylate 0.5M
CoCl2 10mM
TCEP 1mM
Biotin-N4-CTP (store at -20Â°C)
Biotin-N4-CTP 50mM
Tris (pH 7.5) 10 mM
EDTA 1mM

Experimental procedure
Biotin Labeling Probe:
1. Add the reactants in the following order, mix gently, do not vortex
Ultrapure water 25Î¼l
5Ã—TdT Reaction Buffer 10Î¼l
Probe (1Î¼M) 5Î¼l
Biotin-N4-CTP 5Î¼l
TdT (2U/Î¼l) 5Î¼l
37 Â° C reaction for 30 minutes
2. Stop the reaction by adding 2.5 Î¼l of 0.2 M EDTA;
3. Add 50 Î¼l of phenol: chloroform, briefly vortex, centrifuge at 15000 g for 2 min, retain the upper aqueous phase, and store at -20 Â° C;
4. Combine the two labeled primers in the same volume before the reaction, anneal the primer at 90 Â°C, and naturally cool to 4 Â°C, stand for use.
Extracting nuclear proteins:
1. 2~3Ã—10 ⁶ density paved 60mm cell culture plate, cultured for about 12h;
2. Remove the cell culture medium and wash the cells once with PBS;
3. Add 1 mL of Buffer B to the plate, scrape the cells and collect in a 1.5 mL centrifuge tube;
4. Centrifuge at 1000g for 2min, aspirate the supernatant;
5. Add 160 Î¼l Buffer A, resuspend the pellet, and incubate for 20 min;
6. Add Buffer A containing 2.5% NP-40, vortex for 10 s, centrifuge at 5 Â°C for 5 min at 4 Â°C;
7. Aspirate the supernatant, add 40 Î¼l Buffer C, vortex at 4 Â° C for 25 min, centrifuge at 18000 g for 4 min at 4 Â° C;
8. Pipette 2 Î¼l of the supernatant to determine the protein concentration using the Bradford method and store the rest at -80 Â°C.
Configure a non-denaturing polyacrylamide gel (take 6% concentration as an example)
5Ã—TBE 1mL
30% Ac-Bi 2mL
40% Glycerin (glycerol) 625Î¼L
DDW (double distilled water) 6.125mL
10% AP 150Î¼L
10% TEMED 100Î¼L
0.5Ã—TBE with pre-cooling at 4Â°C as electrophoresis buffer and 100-60 pre-electrophoresis for 30-60min (time is uncertain, bromophenol blue takes up two-thirds of the whole gel)
EMSA (refer to PIERCE kit)
Proof of specificity
The probe sequence used for the first time needs to prove whether it specifically binds to the protein of interest and determines the position of the target band.
Follow the system in the â€œStepsâ€ and do the following four parallel experiments:
(Based on adding ddw, 10Ã—binding buffer, Poly(dI.dC))
1) Biotinylated probe
2) Protein crude extract
3) crude protein extract + 200-fold concentration of non-labeled homologous probe (ie cold probe)
4) Protein crude extract + 200-fold concentration of non-labeled mutant probes (multiple mutant types of probes can be designed to see if they can compete for binding)
5) The crude protein extract + antibody is reacted at room temperature for 10 min, and then the biotin-labeled probe is added;
The reaction was continued at room temperature for 20 min for EMSA detection.
Analysis of results, if the following experimental results appear
1) Display free probe position
2) Display free probe position and migration belt position
3) Only free belt, no migration belt
4) consistent with 2) belt type
It is then demonstrated that the probe binds specifically to the protein of interest.
step:
1. Add the reactants in the following order and mix gently (20 Î¼l system)
Ddw â€”â€”
10Ã—binding buffer 2Î¼l
Poly(dI.dC) 1Î¼l (the above text has been stated by the company)
Crude nuclear protein extract 4-10Î¼g (mildly mixed)
Biotinylated probe 0.5Î¼l
After reacting for 20 min at room temperature, 4 Î¼l of 6Ã— Loading Buffer (TAKARA) was added, 10-20 Î¼l was applied, and 100 V was electrophoresed to two-thirds of bromophenol blue.
2. Soak the nylon membrane at 0.5Ã—TBE for at least 10 min before electro-rotation.
The pre-cooled 0.5Ã—TBE was electrotranswelled to 100V on a nylon membrane for 45 min.
3. Under UV BOX, face the UV light source on the side close to the film, cross-link with 254nm excitation light for 15min (UV cross-linker 1200 energy, 2 times)
4. Add 25mL Blocking Buffer and close for 30min on a bleaching shaker at approximately 70rpm
5. Dilute SA-HRP at 1 mL in 12 mL Blocking Buffer, decolorize shaker at 70 rpm for 20 min.
(The film washing process is all carried out on a bleaching shaker, about 100-140prm)
6. Buffer II 25ml, 5min
7. wash buffer 25ml 15min
8. Buffer III 25ml 5min Ã— 2 times
9. 0.1% SDS in 2Ã—SSC, 5minÃ—2 times
10. 0.1% SDS in 1Ã—SSC, 10minÃ—2 times
11. 0.1% SDS in 0.5Ã—SSC, 5minÃ—2 times
12. The membrane is slightly blotted on the filter paper, and added to the luminescent reaction solution (Ningbo Aowei) diluted 1:20 for 1-5 min to seal the nylon membrane in the plastic wrap (to avoid wrinkles and bubbles) The darkroom is exposed for 1-5 minutes and the signal is detected.
Precautions
Use this protocol rendering

Figure 1. MEF cells were stimulated with 10 ng/ml mLT-?, stimulated for 0, 15, 30, 60, 120 min, respectively, and the amount of NF-?B was measured. (p:probe only. Only labeled probes were added without nuclear protein extract)
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