application of maldi-tof mass spectrometry in post-genomic era
DESCRIPTION
Application of MALDI-TOF Mass Spectrometry in Post-Genomic Era. 99% sequence of human genome published. Genomics: --Identification & characterization of genes & their arrangement in chromosomes Proteomics: --Functional analysis of gene products Bioinformatics: - PowerPoint PPT PresentationTRANSCRIPT
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Application of MALDI-TOF
Mass Spectrometry
in Post-Genomic Era
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99% sequence of human genome published
Genomics:
--Identification & characterization of genes & their arrangement in chromosomes
Proteomics:
--Functional analysis of gene products
Bioinformatics:
--Storage,analysis & manipulation of the information from genomics & proteomics
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DNA
mRNA
t-RNA
t-RNA
t-RNA t-RNA
Ribosome
(....)
Protein
CHOPO4
(....)
Post TranslationalModifications
X
X
Active Protein
mRNAlevel expressed protein level nor does it indicate the nature of the functional protein product
圖一:DNA序列是藍圖決定細胞的表現,蛋白質卻是實際上有功能的工作者;分子階層的蛋白質及DNA分析是瞭解其功能的關鍵
Genomics genes characterization and identification
Proteomics functional analysis of gene products
Bioimformatics
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cDNA microarray:
--measures changes in mRNA
--interface between genomics and proteomics
Two-dimensional gels & Mass spectrometry:
--powerful tools for identifying proteins
--post-translational modifications
--protein-protein interaction
Transgenic & knockout mouse:
--functions of novel proteins in vivo
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99% sequence of human genome published
Age of functional genomics
cDNA microarray core lab
Proteomics core lab
Biological samples (C/E)
ProteinscDNA
Microarray 2-D gels/MS
Protein expression pattern
mRNA expression pattern
Bioinformatics core lab
Function study in Tg/KO mouse core lab
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Strategy for proteomic study in cancer biology
Normal cells
Tumor cells
SD
S-P
AG
E
isoelectrofocusing
MALDI-TOF MS analysis
Laser-captured microdissector
digested by trypsin
Database search/mapping
(?)
Protein identified
Clinical specimens
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Mass Spectrometry for Biotechnology
Gary SiuzdakThe Department of ChemistryThe Scripps Research Institute
La Jolla, California
Academic Press 1996
Reference Book
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What is a mass spectrometer and what does it do?
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Analogy between mass analysis and the dispersion of light
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Components of a mass spectrometer
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First DetectorLaser
Reflector
Second Detector
圖十一:在 MALDI-TOF MS中的反射器設計
MALDI-TOF MS(Matrix-assisted laser desorption/ionization-Time of flight) (基質輔助雷射脫附游離 -飛行時間質譜儀 )
0
40000
40 80 120 160
RPKPQQFFGLMamide
m/z
0
40000
40 80 120 160
RPKPQQFFGLMamide
m/z
M/Z
Time of Flight
Solid probe
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Ion Sources and Sample Introduction
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Sample probes and matrix for MALDI
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MALDI matrix
# A nonvolatile solid material that absorbs the laser radiation resulting in the vaporization of the matrix and sample embedded in the matrix.
#The matrix also serves to minimize sample damage from the laser radiation by absorbing most of the incident energy and the matrix is believed to facilitate the ionization process.
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Matrix-assisted laser desorption/ionization source
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Calibration for MALDI
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Vacuum system in MS
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Mass Analyzer-Time of Flight (TOF)
Kinetic Energy = ½ mv2
v = (2KE/m)1/2
m/z
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Ion Detector
Electron multiplier
Photomultiplier conversion dynodescintillation counting
1 106
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Sensitivity of MALDI-TOF MS
~10 fg
1347.7 g/mole x 5 x 10 -18 mole = 6.74 x 10 –15 g
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Strategy for proteomic study in cancer biology
Normal cells
Tumor cells
SD
S-P
AG
E
isoelectrofocusing
MALDI-TOF MS analysis
Laser-captured microdissector
digested by trypsin
Database search/mapping
(?)
Protein identified
Clinical specimens
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The 2-D gel pattern of human kidney epithelial 293 cells expressed without (A) and with (B) the
Epstein-Barr virus oncoprotein LMP1
(A) (B)
Pick up spots of interest
Digested by trypsin
MALDI-TOF MS analysis
IEF IEF
SD
S-P
AG
E
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170
116.3
66.3
55.4
29
21.5
170
116.3
66.3
55.4
29
21.5
pH 310(A)
pH 310
a
bc
a'
b'c'd
(B)
(A) (B)
1
1
2
1 3
The substrate of GSK-3 purified from pig brain
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(b1)
(d2)
(a'1)
(b'1)
(b'3)
472-480
472-480526-532533-552558-565
472-480526-532533-552558-565
472-480526-532533-552558-565
533-552558-565
MALDI-TOF analysis of tryptic fingerprint from the substrate for kinase FA/GSK-3 in pig brain
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Data base search for the substrate of kinase FA/GSK-3from pig brain
MSYQGKKNIP RITSDRLLIK GGKIVNDDQS FYADIYMEDG LIKQIGENLI VPGGVKTIEA HSRMVIPGGI DVHTRFQMPD QGMTSADDFF QGTKAALAGG TTMIIDHVVP EPGTSLLAAF DQWREWADSK SCCDYSLHVD ISEWHKGIQE EMEALVKDHG VNSFLVYMAF KDRFQLTDCQ IYEVLSVIRD IGAIAQVHAE NGDIIAEEQQ RILDLGITGP EGHVLSRPEE VEAEAVNRAI TIANQTNCPL YITKVMSKSS AEVIAQARKK GTVVYGEPIT ASLGTDGSHY WSKNWAKAAA FVTSPPLSPD PTTPDFLNSL LSCGDLQVTG SAHCTFNTAQ KAVGKDNFTL IPEGTNGTEE RMSVIWDKAV VTGKMDENQF VAVTSTNAAK VFNLYPRKGR IAVGSDADLV IWDPDSVKTI SAKTHNSSLE YNIFEGMECR GSPLVVISQG KIVLEDGTLH VTEGSGRYIP RKPFPDFVYK RIKARSRLAE LRGVPRGLYD GPVCEVSVTP KTVTPASSAK TSPAKQQAPP VRNLHQSGFS LSGAQIDDNI PRRTTQRIVA PPGGRANITS LG
*908.4 da --- 391-397 *2169.1da --- 533-552 *pI~5.95
Collapsin Response Mediator Protein-2 (CRMP-2, human)
(d2)
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(b1)
Amino acid sequence analysis by PSD technique in MALDI-TOF MS
2169
908
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Tandem Mass Spectrometry
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MS/MS with a TOF reflectron mass spectrometer
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Peptide fragmentation postionization [Post Source Decay (PSD)]
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(b1)
Amino acid sequence analysis by PSD technique in MALDI-TOF MS
2169
908
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Amino acid sequencing
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Determination of protein molecular weight
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LC/MS
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ESI Ion Trap LC/MSn
(電噴霧離子井液相層析多重質譜 )
Posttranslational modification (?)
Trypsin digest
nano-LC (check minor difference)
MS-MS(or MSn) analysis for selected peptides
Identification of modifications on protein
Normal Tumor
MALDI-TOF =&
ESI Ion trap LC/MSn MALDI-TOF
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Two-dimensional gel electrophoresis system
Sample purification/preparation
(Laser-captured microdissector)
1o-D Isoelectrophoresis
2o-D SDS-PAGE
2D-gel image
analysis system
Quantitation of spots in 2D-gel
Image comparison between 2D-gels
Automatic spots pick-up
Spot picker and Digester
MALDI-TOF & ESI Ion trap LC/MSn
MS spectrometric
analysis system
Automatic spots digestion/extraction
MS spectrometry database
Bioimformatics
Aim: Set up proteomics core lab
貴儀中心
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Isotope–Coded Affinity TagsICAT™
• Breakthrough approach to quantitative protein expression analysis - 2D gel alternative
reactive group
biotin tag
linker (heavy or light)
heavy reagent: d8-ICAT (X=deuterium)light reagent: d0-ICAT (X=hydrogen)
S
HN NH
O
NH O
ONH
IO OX
X
X
X
X
X
X
XSH
cys
Label&
Quantify
Emerging Technology
Nature Biotechnology 17, 994-999 (1999)
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The End
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Isotope–Coded Affinity TagsICAT™
• Breakthrough approach to quantitative protein expression analysis - 2D gel alternative
reactive group
biotin tag
linker (heavy or light)
heavy reagent: d8-ICAT (X=deuterium)light reagent: d0-ICAT (X=hydrogen)
S
HN NH
O
NH O
ONH
IO OX
X
X
X
X
X
X
XSH
cys
Label&
Quantify
Emerging Technology
ICAT Approachto Quantitative Protein Expression Analysis
Determine differences in protein expression by measuringrelative intensities of light vs. heavy
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ICAT™Protein ID and Quantification Process
ProICAT provides Protein Identification and Quantitation information
ICAT™ Features & Benefits
• Overcomes some of the limitations of 2D Gels.• Ability to quantify membrane proteins.• ID and quantify low abundance proteins.• Broader range of protein MW or pI.
• Allows for greater automated/higher throughput approach in the simultaneous quantification and identification of proteins.
• Reduces complexity of analysis of protein digest -only cysteinecontaining peptides.
• Applied Biosystems ‘Systems Approach’ for ICAT Technology including ICAT reagents, software and support.