Introduction to Proteomics - Metabolomicsmetabolomics.se/sites/default/files/courses_files/Intro to...

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1 Introduction to Proteomics Åsa Wheelock, Ph.D. Division of Respiratory Medicine & Karolinska Biomics Center [email protected] In: Systems Biology and the Omics Cascade, Karolinska Institutet, June 9-13, 2008

Transcript of Introduction to Proteomics - Metabolomicsmetabolomics.se/sites/default/files/courses_files/Intro to...

Page 1: Introduction to Proteomics - Metabolomicsmetabolomics.se/sites/default/files/courses_files/Intro to proteomics... · 1 Introduction to Proteomics Åsa Wheelock, Ph.D. Division of

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Introduction to Proteomics

Åsa Wheelock, Ph.D.Division of Respiratory Medicine &

Karolinska Biomics [email protected]

In: Systems Biology and the Omics Cascade, Karolinska Institutet, June 9-13, 2008

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Focus of course: Tools for data analysis

Your analysis is no better than data you have collected...

The goals of this proteomics overview:• Understand possibilities & limitations • Pros and cons of different method• Sources of variance in proteomics• Take advantage of proteomics core facilities • Perform proteomics collaborations • Write a short research proposal in

proteomics

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Proteomics publications in Pubmed

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1996 1997 1998 1999 2000 2001 2002 2003 2004 2005 2006

First ”proteomics”publication

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Why Proteins?!?• Business end of the cell• Detailed information with limited efforts

– As compared to metabolomics

TRANSCRIPTOMICS

PROTEOME

METABOLOME

Limited info from mRNA

Detailed infoRobust technology

Techincally challenging

• Relatively robust methods available

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Proteomics Methodology• No ”protein PCR”

– 4 nucleotides vs 20+ amino acids– Post-translational modifications (PTM)

3 MAIN PROTEOMICS PLATFORMS• Gel based methods • Shotgun methods (mass spec-based)

”chromatography-based”, ”gel-free”• Array based (antibody based)

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6Klose, J. 1975. Humangenetic 26, 231-43O’Farrel, P. 1975. J. Biol.Chem, 250, 4007-21

Gel based: 2-Dimensional Electrophoresis

Isoelectric point (pI)

Net

cha

rge

3 4 5 6 7 8 9 10 11 pH

+2+1

0-1-2

log

Mw

mobility

Molecular weight

SEPARATION VISUALISATION

QUANTIFICATION

Stoichiometric protein stain => 3rd dimension

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Image acquisition

Image acquisition using fluorescent scanner

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Quantitative image analysis

1. Detect spots

2. Match spots across gels

3. Quantify spot volumes

Pixel intensity => 3rd dimensionSpot volume = protein quantity

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Protein identification

⇒ Mass spectrometry(MALDI-TOF/TOF)

Trypsin digestion

⇒ DATABASE SEARCH => IDENTIFICATION(Swiss-prot, EnSemble) (statistical probability)

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Protein Identification

Protein Trypsine digestion Peptides EXPERIMENTAL Peptide masses

Protein database

DTHKSEIAHRFKDLGEEHFKGLVLIAFSQYLQQCPF DEHVKLVNELTEFAKTCVADESHAGCEKSLHTLFGDELCKVASLRET

Virtual digest

MS analysis

EXPECTED Peptide masses

Statistical matching

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Peptide mass mapping

LHTLFGDR

MS/MS analysis=> sequence information

MS analysis=> peptide masses

Statistical matching

DLGEEHFK database search

DTHKSEIAHRFKDLGEEHFKGLVLIAFSQYLQQCPF DEHVKLVNELTEFAKTCVADESHAGEKSLHTLFGRELCKVASLRET

Homology search Validate statistical hit

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Shotgun vs. Gel-based proteomics

Adapted from Patterson and Aebersold, Nature Genetics 2003, 33:311-23. Fig. 3

extract

Separate Quantify

Separate(LC)

Digest

Digest

MS/MS

MS/MS

(2DE)

ID

Quantify

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Semi-quantitative proteomics

Both 2DE and MS-based methods NOT quantitative by nature

Co-separation: 2 samples => ratiosTags => Semi-quantitative proteomics

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Shotgun isotope-tagging :Isotope coded affinity tag (ICAT)

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Multiplexing in 2DE: DIGEMultiplexing in 2DE: DIGE-- Differential Gel ElectrophoresisDifferential Gel Electrophoresis

Protein abundance = 532/633 signal ratio

Co-separation by 2DE

Direct ratiometric normalization

Spot quantification

Statistical analysis

Protein visualization (super-imposable images)

λex 633nm ⇒ Cy5λex 532nm ⇒ Cy3

Treated sample: Covalently labeled (Cy3)

Control sample: Covalently labeled (Cy5)

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Semi-quantitative proteomics

Both 2DE and MS-based methods NOT quantitative by nature

Co-separation: 2 samples => ratiosTags => Semi-quantitative proteomics

Pooled internal standard + 2-3 samples => Relative quantification

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Internal Standards in 2DE: DIGEInternal Standards in 2DE: DIGE

Protein abundance = relative to IS

Co-separation by 2DE

Direct ratiometric normalization

Spot quantification

Statistical analysis

Protein visualization (super-imposable images)

λex 633nm ⇒ Cy5λex 532nm ⇒ Cy3

Treated Sample: Covalently labeled (Cy3)

Control Sample:Covalently labeled (Cy5)

λex 488nm ⇒ Cy2

Pooled Internal standard (Cy2)

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Proteomics in Pubmed

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500

1000

1500

2000

2500

3000

1996 1997 1998 1999 2000 2001 2002 2003 2004 2005 2006

proteomics 2DE

First ”proteomics”publication

First DIGE-method

published

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Sample A

Trypsin digestion (peptides)

31114

PRG

30

115

PRG

29

116

PRG

28

117

PRG

Multiplexing in MS: iTRAQ- isobaric Tag for Relative and Absolute Quantitation

Sample B Sample C Sample D

a b c diTRAQ labelling

MS/MS m/z

ID

Quantification

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Differential labelling opens up new possibilities

• Cysteine oxidative states

• Identify peptides on plasma membrane surface

• Cellular re-localization

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2D or not 2D?2D or not 2D?Gel-based methods: 2-D electrophoresis

+ soluble proteins

+ post-translational modifications

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Post-translational modifications”Spot trains”

Intact proteins

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2D or not 2D?2D or not 2D?Gel-based methods: 2-D electrophoresis

+ soluble proteins

+ post-translational modifications

- technical variance, time consuming

MS-based (Gel-free) methods: ICAT, iTRAQ

+ membrane proteins

+ low abundance proteins

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Extremes of physiochemical properties: Peptides

• Charge

- pI range from 3-12

• Size

- Mw range of 5 – 500,000 kDa

• Hydrophobicity

- membrane proteins

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2D or not 2D?2D or not 2D?Gel-based methods: 2-D electrophoresis

+ soluble proteins

+ post-translational modifications

- technical variance, time consuming

MS-based (Gel-free) methods: ICAT, iTRAQ

+ membrane proteins

+ low abundance proteins

- expensive, data intense

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Shotgun approcahes and gel-based approaches complementary

No ”true” proteomics technique yet

SHOTGUNGEL-BASED

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日本Japan

103

100 101 102 103 104 105 106 107 108 109 1010 1011 1012

COPIES of each

PROTEIN

Osaka 大阪

Kyoto 京都

Kobe 神戸

104

1012

DYNAMIC RANGE

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- 400 reported PTMs

Protein copy numbers in blood (log10)0 1 2 3 4 5 6 7 8 9 10 11 12

Phos

phor

ylat

ion

site

s

7

6

5

4

3

2

1

Post-translational Modifications (PTMs)

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Variance in 2DE• BIOLOGICAL VARIANCE• Experimental variance

– Pre-fractionation, isolation & labelling of proteins – Protein staining

• Technical variance– Gel-to-gel variation in 2DE– Image acquisition (scanner)

• Post-experimental variance– Software-induced variance– User dependant variance

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Variance in 2DE• BIOLOGICAL VARIANCE•• Experimental varianceExperimental variance

– Pre-fractionation, isolation & labelling of proteins – Protein staining

• Technical variance– Gel-to-gel variation in 2DE– Image acquisition (scanner)

• Post-experimental variance– Software-induced variance– User dependant variance

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Remember that variance adds up:Multiple-step method is not your friend...

10% 40%

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Variance in 2DE• BIOLOGICAL VARIANCE• Experimental variance

– Pre-fractionation, isolation & labelling of proteins – Protein staining

• Technical variance– Gel-to-gel variation in 2DE– Image acquisition (scanner)

• Post-experimental variance– Software-induced variance– User dependant variance

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Technical variance in 2DE

Solubilization Rehydration Isoelectric focusing

SDS-PAGELoad IPG strip Protein visualization

Recovery?

Recovery?

Inhomogenouselectric field?

Gel-to-gel variations?

-SH modifications?

Staining artifacts?

Backgroundfluorescence?

Biological variance

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Tools to reduce variance

Technical variance• Internal standard:

– DIGE

• Software algorithms:– Background subtraction– Normalization

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Dynamic range of scanner

16 bit pixel resolution (216 ∼ 65,000 ~ 105)Make sure you are using the entire range!

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Variance in 2DE• BIOLOGICAL VARIANCE• Experimental variance

– Pre-fractionation, isolation & labelling of proteins – Protein staining

• Technical variance– Gel-to-gel variation in 2DE– Image acquisition (scanner)

• Post-experimental variance– Software-induced variance– User dependant variance

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2DE analysis software

• Main purpose: match and quantify spots• Normalization: reduce gel-to-gel variation• Background subtraction:

– Reduce background noise– Increase signal/noise ratio– Increase sensitivity

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Global Background SubtractionGlobal Background Subtraction

PDQuestPDQuest: Floating/Rolling Ball: Floating/Rolling Ball

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Software induced variance Software induced variance

Expression; No background subtraction

0

25

50

75

100

1 51 101 151 201 251 301 351 401 451

CV

(%) n

=5

Expression; No background subtraction

0

25

50

75

100

1 51 101 151 201 251 301 351 401 451

CV

(%) n

=5

Average CV=4.6%Average CV=10%

PDQuest PG200PD Quest; Power mean

0

25

50

75

100

1 51 101 151 201 251 301 351

CV

(%) n

=5

PD Quest; Power mean

0

25

50

75

100

1 51 101 151 201 251 301 351

CV

(%) n

=5

Software variance up to 30% of technical variance

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Applications of proteomicsApplications of proteomicsBIOMARKER DISCOVERY• Biomarker of disease & susceptibility

CLINICAL APPLICATIONS• Pharmaceutical target identification• Improved diagnostics

MECHANISTIC STUDIES• Protein-protein interactions• Protein adduction /Altered protein expression• Hypothesis generation: avoid local ”maxima”• Systems Biology

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Proteomics in the future

• Improved sensitivity– Currently: scratching the surface– laser capture microdissection

• Protein microarrays– Antibody arrays (e.g. for cytokines)– Tissue microarrays (Peter Nilsson, Friday)

• In vivo subcellular localization assays• Protein amplicifation method?

– i.e. ”protein-PCR”

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Focus on INTERPRETINGINTERPRETING data,not on ACQUIRING ACQUIRING data.

Pathway Analysis• Integrate data from omics cascade• Integrate heatmap with biological pathways

Proteomics in the NEAR future...

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Preview of coming attractionsPreview of coming attractions……KEGG & KEGG & KegArrayKegArray

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Take home messages...

...keep your variance downand your dynamic range up!

...keep your false positives down,and your power up!