Presentation is loading. Please wait.

Presentation is loading. Please wait.

Electro Mobility Shift Assay EMSA Band Shift Assay Gel Shift Assay

Published byClemence Gray Modified over 8 years ago

Similar presentations

Presentation on theme: "Electro Mobility Shift Assay EMSA Band Shift Assay Gel Shift Assay"— Presentation transcript:

1 Electro Mobility Shift Assay EMSA Band Shift Assay Gel Shift Assay
R. Voll 09/01

2 Gene Regulation by Transcription Factors
Regulatory Region Coding Sequence R. Voll 09/01

3 Application: Detection of DNA-binding factors/proteins
Analysis of DNA sequences (e. g. promoter or enhancer regions) for their potential to bind specifically to proteins/nuclear extracts Analysis of (sub-)cellular extracts for the presence of certain DNA-binding proteins (e. g. a transcription factor with a known recognition sequence) R. Voll 09/01

4 EMSA: Principle Nuclear extract of non-activated cells
Radioaktively labeled oligonucleotide with NF-B - binding site (probe) and bound NF-B NF-B Radioactively labeled oligonucleotide with NF-B - binding site (probe) Free Probe A double-stranded oligonucleotide containig a NF-B- binding site is labeled with a radioactive isotope and incubated with a nuclear extract. During gel-electrophoresis, NF-B bound to the oligonucleotide causes a shift compared to the free probe. R. Voll 09/01

5 Preparation of Nuclear and Cytosolic Extracts
The procedure is carried out on ice rsp at 4°C and in the presence of protease (and phosphatase) inhibitors. 1. Swell cells in hypotonic lysis buffer 2. Add NP-40 and vortex to disrupt cytoplasmic membrane 3. Centrifuge to pellet nuclei 4. Carefully remove supernatant (contains cytosolic and membrane fraction) 4. Wash nuclear pellet once in lysis buffer 5. Add hypertonic extraction buffer to nuclear pellet 6. Agitate vigouresly for 30 minutes 7. Centrifuge at high speed 8. Remove nuclear extract, determine protein concentration and freeze on dry ice until EMSA is performed R. Voll 09/01

6 The Probe Double stranded radiolabeled oligonucleotides containing a transcription factor binding site AP-1 5’-GCT TGA TGA CTC AGC CGG AA C-3’ 3’-CGA ACT ACT GAG TCG GCC TT G-5’ NF-kB 5’-AGT TGA GGG GAC TTT CCC AGG C-3’ 3’-TCA ACT CCC CTC AAA GGG TCC G-5’ Binding motif R. Voll 09/01

7 Annealing the Oligos Heat up an equimolar mixture of the 2 oligos
to 95°C and let them slowly cool down by turning off the heat block. R. Voll 09/01

8 Labeling the Probe (I) A. T4 Polynucleotide Kinase
5’-AGT TGA GGG GAC TTT CCC AGG-3’ 3’-CA ACT CCC CTC AAA GGG TCC G-5’ 5’-P-AGT TGA GGG GAC TTT CCC AGG-3’ 3’-CA ACT CCC CTC AAA GGG TCC G-P-5’ + Adenosin-P-P-P (g-ATP) PNK R. Voll 09/01

9 Labeling the Probe (II)
B. Klenow Fragment of E. coli DNA Polymerase I 5’-ACT TGA GGG GAC TTT CCC AG-3’ 3’-A ACT CCC CTC AAA GGG TCC G-5’ 5’-ACT TGA GGG GAC TTT CCC AGG C-3’ 3’-TGA ACT CCC CTC AAA GGG TCC G-5’ + a-32-P dGTP + dCTP + dTTP Klenow R. Voll 09/01

10 Removal of Unincorporated Nucleotides
Remove not incorporated nucleotides by Sephadex G50 column or non-denaturing PA gel purification repeated ethanol precipitation R. Voll 09/01

11 Reagents Competitor DNA: Competition of unspecific
poly (dI-dC) . poly (dI-dC) binding (e. g. histones) BSA: Protection of nuclear extracts GTP: ? Radiolabeled Probe: Detection of DNA-binding proteins Reaction Buffer Binding conditions R. Voll 09/01

12 Analysis by non-Denaturing Polyacrylamide Gel Electrophoresis
R. Voll 09/01

13 Proof of Specificity Supershift using antibodies against the DNA-binding protein Competition for binding to the radiolabeled probe using unlabeled wildtype and mutated oligos R. Voll 09/01

14 Supershift Nuclear extract of activated cells
cells with anti-p50 antibody Supershift p50/p65 + anti-p50 Radioaktiv labelled oligonucleotide with NF-B - binding site (probe) and bound NF-B p50/p65 Radioactiv labelled oligonucleotide with NF-B - binding site (probe) Free probe A double-stranded oligonucleotide containig a NF-B- binding site is labelled radioactive and incubated with a nuclear extract. During gel-electrophoresis, NF-B bound to the oligonucleotide causes a shift compared to the free probe. R. Voll 09/01

15 Competition with Unlabeled Oligos
p50/p65 p50/p50 Unspecific Free probe GGG GAC TTT CCC GGA GAC TTT CCC Wild type oligo Mutated oligo Increasing amounts of unlabeled oligos containing the NF-kB binding site or unlabeled oligos with a mutated binding site were added to the reaction mix prior to gel electrophoresis. Specific binding is extinguished only by the non-mutated oligo. R. Voll 09/01

Download ppt "Electro Mobility Shift Assay EMSA Band Shift Assay Gel Shift Assay"

Similar presentations

Lecture 8 Transcription Initiation Prokaryotic Eukaryotic Reading: Chapter 4 (115-116) Chapter 11 Molecular Biology syllabus web siteweb site.

Lecture 8 Transcription Initiation Prokaryotic Eukaryotic Reading: Chapter 4 ( ) Chapter 11 Molecular Biology syllabus web siteweb site.
I. Background and Observations CD4 and CD8 cells are essential in immune system function. Both are classified as T- cells and derive from a common precursor,

I. Background and Observations CD4 and CD8 cells are essential in immune system function. Both are classified as T- cells and derive from a common precursor,
PRINCIPLES OF CROP PRODUCTION ABT-320 (3 CREDIT HOURS) LECTURE 14 TECHNIQUES FOR GENETIC ENGINEERING, ISOLATION OF TOTAL CELLULAR DNA NUCLEIC ACID HYBRIDIZATION.

PRINCIPLES OF CROP PRODUCTION ABT-320 (3 CREDIT HOURS) LECTURE 14 TECHNIQUES FOR GENETIC ENGINEERING, ISOLATION OF TOTAL CELLULAR DNA NUCLEIC ACID HYBRIDIZATION.
Online Counseling Resource YCMOU ELearning Drive… School of Architecture, Science and Technology Yashwantrao Chavan Maharashtra Open University, Nashik.

Online Counseling Resource YCMOU ELearning Drive… School of Architecture, Science and Technology Yashwantrao Chavan Maharashtra Open University, Nashik.
ATG GAG GAA GAA GAT GAA GAG ATC TTA TCG TCT TCC GAT TGC GAC GAT TCC AGC GAT AGT TAC AAG GAT GAT TCT CAA GAT TCT GAA GGA GAA AAC GAT AAC CCT GAG TGC GAA.

ATG GAG GAA GAA GAT GAA GAG ATC TTA TCG TCT TCC GAT TGC GAC GAT TCC AGC GAT AGT TAC AAG GAT GAT TCT CAA GAT TCT GAA GGA GAA AAC GAT AAC CCT GAG TGC GAA.
Supplementary Fig.1: oligonucleotide primer sequences.

Supplementary Fig.1: oligonucleotide primer sequences.
Measurement in Science Bioassays and Immunoassays Karim Meeran 23 October 2009.

Measurement in Science Bioassays and Immunoassays Karim Meeran 23 October 2009.
SOUTHERN BLOTTING Presented by: Imran Fakhroni Nurkholis Nugroho Nino Radiansyah Indra Ardi Fauzi Arfita Sari.

SOUTHERN BLOTTING Presented by: Imran Fakhroni Nurkholis Nugroho Nino Radiansyah Indra Ardi Fauzi Arfita Sari.
Protein Purification and Expression MCB 130L, Lecture 2.

Protein Purification and Expression MCB 130L, Lecture 2.
Protein Purification and Expression

Protein Purification and Expression
Chapter 12: DNA-protein interactions. Preparation of nuclear extracts and cytoplasmic (S-100) fraction Use hypotonic solutions and 10 up-and-down strokes.

Chapter 12: DNA-protein interactions. Preparation of nuclear extracts and cytoplasmic (S-100) fraction Use hypotonic solutions and 10 up-and-down strokes.
Genomic DNA purification

Genomic DNA purification
بعض الأجهزه المستخدمة في الوراثة الجزيئية Explanation of some equipment and operation ways.

بعض الأجهزه المستخدمة في الوراثة الجزيئية Explanation of some equipment and operation ways.
Kamila Balušíková.  DNA – sequence of genes, repetitive sequence of noncoding regions  RNA  Proteins gene expression.

Kamila Balušíková.  DNA – sequence of genes, repetitive sequence of noncoding regions  RNA  Proteins gene expression.
Gene Technology Chapters 11 & 13. Gene Expression 0 Genome 0 Our complete genetic information 0 Gene expression 0 Turning parts of a chromosome “on” and.

Gene Technology Chapters 11 & 13. Gene Expression 0 Genome 0 Our complete genetic information 0 Gene expression 0 Turning parts of a chromosome “on” and.
Gene expression *The transcription involves synthesis of an RNA from the DNA template and an enzyme called RNA polymerase. *In prokaryotes there is a single.

Gene expression *The transcription involves synthesis of an RNA from the DNA template and an enzyme called RNA polymerase. *In prokaryotes there is a single.
-The methods section of the course covers chapters 21 and 22, not chapters 20 and 21 -Paper discussion on Tuesday - assignment due at the start of class.

-The methods section of the course covers chapters 21 and 22, not chapters 20 and 21 -Paper discussion on Tuesday - assignment due at the start of class.
PV92 PCR/Informatics Kit

PV92 PCR/Informatics Kit
Proteomics Module Day 1 Tech talk. Experiment: Yeast protein expression changes caused by H 2 O 2 exposure. ► 2 Control groups (A and B): nothing added.

Proteomics Module Day 1 Tech talk. Experiment: Yeast protein expression changes caused by H 2 O 2 exposure. ► 2 Control groups (A and B): nothing added.
DNA Methodologies Sterilization –Clean the workstation with alcohol and bleach. –Autoclaving and ultraviolet light (UV radiation). Consumables and reagents.

DNA Methodologies Sterilization –Clean the workstation with alcohol and bleach. –Autoclaving and ultraviolet light (UV radiation). Consumables and reagents.

Similar presentations

Ads by Google