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Detecting Protein-Protein interactions Salman Ul Islam (MS) Cellular Bio Chemistry Lab

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Page 1: Proteins by Salman Ul Islam

DetectingProtein-Protein

interactions

Salman Ul Islam (MS)Cellular Bio Chemistry Lab

Page 2: Proteins by Salman Ul Islam

CONTENTS

Introduction

Types of protein-protein interactions

Methods of detection

Page 3: Proteins by Salman Ul Islam

INTRODUCTION

Importance for cell biology and biochemistry Localization and trafficking posttranslational modifications signaling networks Essential in viral replication Difficult to predict two main patterns: ■ domain-domain interactions ■domain-peptide interactions

Page 4: Proteins by Salman Ul Islam

CHARACTERISTICS OF PROTEINS

• Nitrogenous compounds, contain carbon, hydrogen, oxygen, nitrogen, and sulfur

• Basic building block is the amino acid• Serve as structural components of animals• Serve as control molecules (enzymes)• Serve as transport and messenger molecules

Page 5: Proteins by Salman Ul Islam

AMINO ACID

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FORMATION OF A DIPEPTIDE

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THE MECHANISM OF INTERACTION

Non-covalent so reversible Van del waals forces Hydrophobic interactions Electrostatic bonds Hydrogen bonds For strong couplings very accurate

force field potentials are needed

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POLYPEPTIDE CHAIN STRUCTURE

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WHY ARE PROTEIN-PROTEIN INTERACTIONS SO IMPORTANT?

The binding of one signaling protein to another can have a number of consequences: 

• Such binding can serve to recruit a signaling protein to a location where it is activated and/or where it is needed to carry out its function.

• The binding of one protein to another can induce conformational changes that affect activity or accessibility of additional binding domains, permitting additional protein interactions.

 

Page 10: Proteins by Salman Ul Islam

IMPACT ON OTHER FIELDS

• Cancer Biology The study of protein-protein interactions has

provided important insights into the functions of many of the known oncogenes, tumor suppressors, and DNA repair proteins.

• Pharmacogenetics Pharmacogenetic research has expanded to include

the study of drug transporters, drug receptors, and drug targets.

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THE TYPES OF PROTEIN INTERACTIONS

• Binary protein-protein interactions

• Scaffolding proteins

Page 12: Proteins by Salman Ul Islam

THE TYPES OF PROTEIN INTERACTIONS-ANOTHER CLASSIFICATION

• Metabolic and signaling (genetic)pathways

• Morphogenic pathways in which groups of proteins participate in the same cellular function during a developmental process

• Structural complexes and molecular machines in which numerous macromolecules are brought together

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MORPHOGENIC PATHWAYS

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HOW TO STUDY PROTEIN PROTEIN INTERACTION?

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OVERVIEW OF TECHNIQUES

• Gel filtration• Far western blot• Affinity

chromatography• Co-

immunopercipitation

• Capillary electrophoresis

• Biosensor

• FRET microscopy• Confocal

microscopy• 2 hybrid assay• Protein microarry• Maspec• NMR• Co-crystallization

for crystallography

Page 16: Proteins by Salman Ul Islam

GEL FILTRATION CHROMATOGRAPHY

Also called ”Size exclusion”

Porous made up of cross-linked polymers

Small molecules are trapped by the beads

For self assembling proteins monomers come later

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FAR WESTERN BLOT

Also called ”Blot overlay”

Fractionating proteins on SDS-PAGE

Blotting to nitocellulose or PVDF membrane

Overlaying with a solution of the protein of interest

Binding the added protein to an immobilized protein on the membrane

Detection with antibody against the overlaying protein

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CO-IMMUNOPRECIPITATION

Protein A binds to antibodies

Sepharose beads coated with protein A

Specific antibody binds to the protein of interest

The complex is precipitated by binding to the beads via protein A

Proteins are released from beads by boiling

Western blot

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AFFINITY CHROMATOGRAPHY

In the case of His- tagged proteins

The His-tagged protein binds to nickel or cobalt column

His-tagged protein and it’s associated protein are eluted from the column by adding imidazole

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FLUORESCENCE RESONANCE ENERGY TRANSFER (FRET)

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FRET CONT

Cyan fluorescence protein (CFP) and yellow fluorescence protein (YFP) are spectral variants of GFP

Plasmid constructs to fuse the proteins of interest to CFP and YFP

Co-transfection of plasmids to the cells Fixation of the cells and view by confocal microscopy Disadvantage:False negative results: If the fluorophores are over 200Ǻ apart while the

proteins interact with each other, no signal will be observed

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FRET USING CFP & YFP

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YEAST TWO HYBRID ASSAY

Transcription factor, Gal4p, has DNA binding (BD)(aa1-147) and transcriptional activator(AD)(aa768-881) domains

Stimulates transcription at a promoter reconized by Gal4p (upstream activating sequence,UAS)

Lac Z reporter gene encodes beta-galactosidase which produces blue pigment when the colony is grown in a media containing X-Gal

Disadvantage: time consuming!

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2 HYBRID SYSTEM

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MAMALIAN TWO-HYBRID ASSAY

Is analogous to Y2H assay Plasmids: 1)Gal4pBD-fusion vector 2)VP16AD-fusion vector(viral activator) 3)luciferase reporter plasmid contaning multiple copies of Gal4p binding

sites(UAS)

Co-transfection: in the case of interaction, luciferase activity will be detected

Advantage: good for studying mammalian proteins: they may not fold correctly in yeast or they may require post-tranlational modifications for protein interaction

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WHAT ARE BIOSENSORS?

• Transducer converts physical change(heat, change in charge, light absorbance, mass) into an electrical signal

Page 27: Proteins by Salman Ul Islam

CONFOCAL MICROSCOPY

A good technique to detect intracellular co-localization of proteins

Point scan laser system minimizes overlaps in image (perfect for imaging Co-localization of proteins)

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CONFOCAL MICROSCOPY CONT.

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Thanks