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PROTEIN ARRAYS prepared mostly by Ailie

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Proteomics aims to simultaneously characterize all the proteins in biological samples ... Hydrophobic surface (Zeta Grip) Gold array. Printing - Technicalities ... – PowerPoint PPT presentation

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Title: PROTEIN ARRAYS prepared mostly by Ailie


1
PROTEIN ARRAYS(prepared mostly by Ailie)
2
The goals of proteomics
  • Proteomics aims to simultaneously characterize
    all the proteins in biological samples
  • Identify / sequence the proteins and determine
    their relative abundances
  • Characterize their posttranslational
    modifications
  • Determine the three dimensional structure
  • Identify the interactions between the proteins,
    and with other molecules most proteins function
    in complexes
  • Follow all the above during development, in
    response to hormonal stimuli, in health and
    disease, etc.

3
Protein arrays can do the job
  • So far, we talked about using chromatography,
    2D-electrophoresis and tandem mass spectrometry
    to achieve the goal of proteomics
  • However, protein arrays are possible solution to
    the problem and might be able to provide the data
    in a fraction of the cost and a fraction of the
    time.
  • Why not now?

4
What is an array?
  • An array is a high-density arrangement of
    capture agents located at defined positions on a
    slide.
  • Arrays are to detect or measure the presence
    and/or quantity of genes or proteins in a sample.
  • Perform a large number of tests simultaneously

5
Topics for protein arrays
  • Uses
  • Types
  • Binding
  • Fabrication and printing
  • Hurdles
  • Exotic arrays
  • Future directions

6
Emili and Cagney 2000 Nature
7
DNA Microarray Hybridization
Targets hybridize to complementary probes by base
pairing
8
A Good Array
  • Reproducible
  • High density (many spots per slide)
  • Maximal binding efficiency
  • Homogenous signal
  • Minimal background noise

9
Analytical vs. Functional Protein arrays
  • (a) Analytical
  • Identify specific proteins/ expression of
    proteins in a complex mixture
  • (b) Functional
  • Identify biochemical activity
  • such as specific protein-
  • drug, protein-enzyme or
  • protein-protein interactions.

http//www.dojindo.co.jp/letterj/106/reviews_02_su
b-01.html
10
Even more complex protein arrays
http//www.stat.purdue.edu/research/coalesce/bioin
formatics/Center_for_Bioinformatics/protein_array_
analysis.html
11
Reverse Array
  • Cellular extracts are spotted directly onto the
    array surface to analyze entire cell at one time
  • Labeled antibodies used to probe the array for
    analytes of interest in the micro-spots
  • Disadvantage
  • Rare proteins may not be detected
  • Increased chance of unspecific reactions

http//www.zeptosens.com/ZeptoMARK/ZeptoMARK/Zepto
MARK_products.html
12
Membrane Protein Arrays
  • Membrane proteins are an important drug target so
    high throughput ligand affinity screening
    desirable.
  • Need to print protein AND associated lipids on
    the array

Fang Y., Frutos A., and Lahiri J. 2002 Membrane
Protein Microarrays. J. Am. Chem. Soc., 124 (11),
2394 -2395
13
Scope of Protein Array Applications
http//www.bioscience.org/2003/v8/d/1017/figures.h
tm
14
Antibody array
15
Antigen array
16
Immobilizing Capture Agents
  • Protein functionality must be preserved
  • Binding site must remain accessible
  • Proteins with different affinities/ properties
    need to be printed onto a single slide
  • Provide reproducible results

17
Attachment to Slide
  • Glass slide treated with an aldehyde or epoxy
    reagent, which reacts with primary amines
  • Adsorption to charged or hydrophobic surfaces
  • Streptavidin arrayed on slide binds to
    biotinylated molecules
  • His tagged proteins arrayed on nickel coated
    slides

http//arrayit.com/Products/Substrates
18
Immobilizing Capture Agents
  • Covalent interaction with the surface
  • Definite arranged order of molecules
  • Possibility of spacers to prevent specific
    interactions
  • Strong interaction between surface and capture
    agent
  • Non covalent interaction with the surface
  • Hydrophobic, H-bond, van der Waals,
    electrostatic, physical adsorption
  • No modification to capture molecule required
  • Weaker interaction between surface and capture
    agent

http//www.ciphergen.com/MasterPage.aspx?URL/tech
apps/pc/tech/arrays
19
Slide Surface
  • 1-Dimensional
  • Capture agent binds by electrostatic/covalent
    interaction
  • 2-Dimensional
  • Capture agent attached to slide adhering
    molecule (e.g. Self-assembled monolayer -
    spontaneous adsorption of alkanthiols on gold
    surfaces )
  • 3-Dimensional
  • (3D) gel or membrane-coated surfaces such as
    polyacrylamide, agarose and nitrocellulose

Kusnezow, W et al 2003 J. Mol. Recognit. 16
165176
20
Hydrophobic surface (Zeta Grip)
21
Gold array
22
Printing - Technicalities
  • Protein drop cannot dry out (add glycerol)
  • Hydrophilic spots on hydrophobic surfaces
    prevents mixing of aqueous spots
  • Resolution how many drops per unit space
  • Filter arrays drops disperse taking more space
  • 3D arrays more slide surface area gives more
    capacity

http//www.genome.org/content/vol7/issue10
23
Probe Printing - Contact
  • Probes spotted onto the slide by lowering the
    printing tip to just touch the surface of the
    slide.

http//bric.postech.ac.kr/bbs/biostat/2001/2001070
3_2.html
24
Probe Printing - Piezoelectric effect
  • Non contact printing
  • based on ink-jet printing technology
  • Piezoelectric effect
  • Electric current ? Material expands? Drop pushed
    out

http//teched.vt.edu
http//bric.postech.ac.kr/bbs/biostat/2001/2001070
3_2.html
25
Photolithography (AFFYMEX)
  • Photosensitive protection
  • Mask
  • UV light removes the protecting groups in
    unmasked areas
  • Nucleotide added to de-protected areas.
  • Repeat process

http//www.affymetrix.com
26
Developing TechnologyArray Creation by
electrospray
  • IDEA Deposition of proteins onto array surfaces
    after mass spectrometry analysis of sample
  • METHOD Proteins separated and spotted according
    to mass using a soft landing technique after MS
    identification.
  • RESULTS
  • A mixture of cytochrome c, lysozyme, insulin and
    apomyoglobin arrayed by this technique and
    function confirmed by specific substrate binding
  • PROBLEMS
  • Time consuming to deposit enough protein.
  • Loss of activity due to harshness of MS still a
    problem
  • AIM Dramatically increase the complexity of the
    protein mixture applied, deposited and analyzed

Washburn, M. 2003. Soft Landing for Protein
Chips. Nature Biotechnology. 211156-57
27
Protein Array Capture Agents
http//neurolab.fr/Proteo3.gif
  • ANTIBODIES - natural binders of proteins
  • APTAMERS - oligonucleotides with affinity for
    individual protein molecules
  • - easy to synthesis, stable, robust
  • MOLECULES - small molecules are easily
    synthesized and robust
  • PROTEINS - important in functional analysis
  • - easily denatured
  • - hard to isolate large libraries
  • ENZYMES, DNA, MEMBRANE PROTEINS, TOTAL CELLS..

28
Antibodies as Capture Agents
  • Well established ELISA technology applicable in
    array format
  • Monoclonal, polyclonal or recombinant antibodies
    (scFv)
  • Polyclonal antibodies recognize different
    epitopes reducing selectivity
  • Single Chain Antibodies (scFv)
  • The variable regions of the heavy and light
    chains can be fused together with antigen
    specificity maintained
  • Smaller, easier to handle, cheaper

29
Synthesized Molecules as Capture Agents
  • Aptamers and Small Molecules
  • Easily synthesized on large scales
  • Stable and robust
  • non-specific protein stains can be used for
    detection (since targets are the only proteins on
    array)
  • Peptide Aptamers
  • Thioredoxin small stable
  • protein with variable surface
  • loop that can be engineered
  • as binding site to various
  • targets

http//www.docforum.tm.fr/documents/25janv05propin
dusvalsavInterB.Rudkin.pdf
30
Incubation of Sample and Array
  • Plate conditions need to be homogeneous
  • Proteins are sensitive to ambient conditions
  • hard to array many different proteins and keep
    all functional.
  • Biological samples are dynamic
  • Cellular conditions continually changing affect
    interactions. This is hard to simulate in vivo

31
DNA Microarray Signal Detection
http//www.awi-bremerhaven.de/Biomeer/molecular-ge
netics-top08-e.html
  • Fluorescence or luminescence detection
  • The relative intensity of label signals
    correlates to relative abundance of corresponding
    gene.

32
Protein Microarray
Complex protein mixture
Capture Antibodies
Chip surface
Feature I
Feature II
1. Wash array 2. add detection
antibody
3. wash
33
Detection of Protein Target Binding
  • CONSIDERATIONS
  • Accuracy, Efficiency, Sensitivity, Maintain
    integrity of sample
  • METHODS
  • Direct labels - fluorescent dyes
  • Indirect labels - secondary antibodies (sandwich
    assay/ELISA)
  • MALDI-TOF mass spectrometry
  • Surface plasma resonance
  • Rolling circle PCR
  • Atomic Force Microscopy (AFM)

34
Strepavidin-biotin Array based ELISA (Mendoza99)
35
Detection Methods
www.functionalgenomics.org.uk/ sections/resources/
Protein_arrays.htm
36
Mass Spectrometry
  • Idea Detect protein bound to array without need
    for labeling
  • Allows analysis of detected protein
  • Method
  • Add energy absorbing molecules (MATRIX) to array
    spot
  • Analysis of spot by standard MALDI-TOF
  • Problems
  • Low throughput

http//www.evms.edu/vpc/seldi/seldiprocess/
37
Surface Plasma Resonance
  • The refractive index at the surface of a gold
    coated chip is monitored.
  • Binding to the array probes changes this
    refractive index and allows not only for
    detection of binding but for monitoring of
    association/dissociation rates
  • Advantage no labeling necessary within the array

http//www.uni-ulm.de/aktuelles/aktuelles_thema/ak
tuell0207/cast/spr.jpg
38
Rolling Circle PCR
  • Aim
  • To improve sensitivity of detection
  • Idea
  • Reporter antibodies are covalently attached to
    unique oligonucleotide primers.
  • A DNA circle is hybridized for a rolling circle
    amplification of the tag.
  • The tag is labeled by hybridization with
    fluorescently-labeled oligonucleotides (or
    alternatively the fluorescently-labeled
    oligonucleotides can be used in the
    amplification)

Schweitze, B et al. Proc Natl Acad Sci USA
9710113-10119.
39
Luminescence detection Kodadek 01
40
Protein chips (MacBeath2000)
41
Large scale arrays of proteins (MacBeath2000)
42
Protein chips with CBD
Enzymatic one color development
Enzymatic two color development
43
Transfected cell arrayBailey, Wu and Sabatini
DDT 02
44
Membrane protein array Beaumont and Negulescu 99
Nature
45
Bouwman..Hanash, Serological Array, Proteomics
03
46
ScFv antibody array, De Wildt, Nature 2000
47
The effect of multi protein complexes Kodadek 01
48
FACS as array (Nolan 2008)
49
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50
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51
Future directions
  • Proteomics in a drop of blood, saliva, urine,
    sweat, pond, environmental analysis
  • Bedside and clinic assay
  • Rapid answers
  • Screen the entire population for all their future
    diseases
  • Remote medicine
  • Food analysis
  • Single cell assays
  • More idea?
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