Post on 23-Feb-2016
description
MALDI-TOF MSy
Análisis de Proteínas
Alberto Jorge GarcíaLaboratorio de Proteómica
Centro de Biología Molecular Severo OchoaUniversidad Autónoma de Madrid- CSIC
Curso Espectrometría de masas, Electrospray Trampa Iónica y Maldi-Tof
UNIVERSIDAD FRANCISCO DE VITORIA
Proteoma
Proteína
Péptidos
Fragmentos
BASE DEDATOS
BASE DEDATOS
Identificación Proteína
Identificación Péptido
Proteómica:
ESTRATEGIA INTEGRADORA PARA EL ANÁLISIS DEL PROTEOMA
SDS-PAGE
2D-IEF-SDS-PAGEBandas de proteínasDigestión “in situ”
en paralelo
MALDI-TOF mapa de péptidos
m-desalado automático
Electrospray-trampa iónica
aislamiento y fragmentación
Identificación de proteína
Secuenciación “de novo”
Extracto de péptidos
0
20004000
6000
8000
1000012000
14000
1000 1500 2000 2500 3000
Inte
nsid
ad
m/z
Mapa de péptidos (MALDI-TOF)Extracto crudo digestión “en gel”
1. gi|191618 Mass: 223549 Score: 87 (M76598) alpha cardiac myosin heavy chain [Mus musculus]Observed Mr(expt) Mr(calc) Delta Start End Miss Peptide 1061.02 1060.01 1060.13 -0.12 1366 - 1374 0 ANSEVAQWR 1085.02 1084.01 1084.32 -0.31 436 - 443 0 MFNWMVTR 1239.27 1238.26 1238.28 -0.01 1253 - 1262 0 TLEDQANEYR 1346.49 1345.48 1345.52 -0.04 24 - 34 0 LEAQTRPFDIR 1442.63 1441.62 1441.61 0.02 1680 - 1691 0 NNLLQAELEELR 1489.17 1488.16 1488.57 -0.41 1117 - 1128 0 IEELEEELEAER 1602.80 1601.79 1601.82 -0.02 955 - 968 1 DIDDLELTLAKVEK 1703.76 1702.75 1702.90 -0.14 1423 - 1436 0 LQNEIEDLMVDVER 1741.93 1740.92 1740.98 -0.06 726 - 741 0 ILNPAAIPEGQFIDSR 1840.03 1839.02 1838.99 0.03 1179 - 1195 0 DLEEATLQHEATAAALR 1896.08 1895.07 1895.02 0.06 1198 - 1214 0 HADSVAELGEQIDNLQR 1979.38 1978.37 1978.18 0.19 1620 - 1636 0 MEGDLNEMEIQLSQANR 2107.39 2106.38 2106.35 0.03 1619 - 1636 1 KMEGDLNEMEIQLSQANR 2277.72 2276.71 2276.54 0.17 1063 - 1081 1 LTQESIMDLENDKLQLEEK 2343.63 2342.62 2342.42 0.20 887 - 906 0 NDLQLQVQAEQDNLNDAEER 2809.57 2808.56 2809.04 -0.48 1000 - 1024 1 ALQEAHQQALDDLQAEEDKVNTLTK 2837.05 2836.04 2836.07 -0.02 1654 - 1678 1 DTQLQLDDAVHANDDLKENIAIVERNo match to: 1771.94
Identificación de la proteína a partir del mapa de péptidos(“peptide-mass fingerprinting”)
Búsqueda en MASCOT(D.Pappin, ICRF, Londres)
MALDI-TOF/MSTransfer into the gas phase
(desorb) IonizeApply electromagnetic
fields
Analyse ion movementsDetermine m/z
DetectorIon Source
MALDI-TOF/MS
Laser
Sample Target DetectorClock
Time-of-Flight Molecular Mass
matrix analyte sample solution
sample deposition
dry samples
insert target andperform analysis
MALDI-TOF/MS
Sample embedded inlight-absorbing matrix
LASER
LASER-excitation ofmatrix molecules
H+
Sample desorption andprotonation
Matrix for Proteins: sinapinic acid, dihydroxybenzoic acid etc.Matrix for Peptides: 4-hydroxy-a-cyanocinnamic acid, DHB.
it co-crystallizes, absorbs laser energy, evaporates and acts as acid
Ionización/Desorción
++
+
Cationized analyte
Analyte moleculesMatrix
molecules
Laser beam
Matrix molecules
Matrix ions
+
Matrix Assisted Laser Desorption / Ionization (MALDI)
Cortesía de Bruker Daltonics
Tres niveles de preparación de muestras:
– Sensibilidad normal: método estándar. – Alta sensibilidad: método “anchor-chip” con
matriz HCCA y cristalización homogénea de Bruker.
– Muy alta sensibilidad: método “anchor-chip” con matriz DHB y cristalización heterogénea.
Preparación de la muestra: anchor-DHB
Fundamentos del TOF
Laser
ReflectorSource
Lineardetector
Reflector detector
MALDI-TOF
Resolución isotópica
1106 1111 1116 1121 1126 m/z
0
1000
2000
3000
4000
5000
6000
a.i.
Voltaje de extracción
Extracción retardada
Extracción retardada
Laser
ReflectorSource
Lineardetector
Reflector detector
Decay can occur at any point along here
Decomposition occurs in the flight tube
1. PSD refers to a method of detecting and measuring the masses of fragment ions formed from a selected precursor ion during the flight time.
2. Fragment ions are mainly formed by unimolecular decomposition after the precursor ions are fully accelerated (after they exit the source—hence post-source decay)
3. Fragment ions are separated in the reflector.
Fundamentals of PSD
PSD fragment ion velocities are the same as their precursors
+
+All three of these species travel at the same velocity in the flight tube until they reach the mirror.
Why? Velocity is determined by initial acceleration. Initial energy = 20 keV. Bond energies = ~ 10 eV, so breaking a bond has a very minor effect on velocities.
Neutral fragments are not detectedReflector
detector
Reflector +20 kV0 V.
Fragmentedprecursor ion
+
+
Fragment ions take different paths in the reflector
Reflectordetector
Reflector +20 kV0 V.
Fragment ion formed by PSD
Intact precursor ion
++
PSDISD