Transcript Slide 1

Quantification of low-abundance proteins in complexes and in total cell lysates by mass spectrometry
Bastienne Jaccard and Manfredo Quadroni
Université de Lausanne
Faculté de biologie et de médecine
Department of Biochemistry
INTRODUCTION
Quantification of proteins can be performed in some mass spectrometers by using a particular method called MRM (multiple reaction monitoring). As we aim to quantify
low-abundance proteins (proteins of the Fas Death-Induced Signaling Complex or DISC), it is crucial to determine if they can be relatively well detected by MRM. Here we
show preliminary results that indicate that the low-abundance proteins we are working with are relatively well detected by MRM in an immunoprecipitated complex but
also, for some of them, in a total cell lysate.
METHOD
Sample analysis in the MRM scan mode in a mass spectrometer (triple quadrupole)
SDS-PAGE of the sample
(immunoprecipitation or total
cell lysate) followed by
proteolytic digestion with trypsin
(cleaves after lysine or arginine
residues)
Ion source
Detector
Q1 = First
quadrupole
Q2 = Second
quadrupole
Q1 is set to transmit
only the wanted m/z
(mass to charge ratio),
the m/z of one tryptic
peptide belonging to
the protein we want to
quantify
Q3 = Third
quadrupole
The selected
tryptic peptide
is fragmented
in fragment
ions in Q2
Signal for the transition
parent ion (tryptic peptide)
fragment ion
Q3 is set to transmit
only the wanted m/z,
the m/z of one
fragment ion derived
from fragmentation of
the selected tryptic
peptide
Intensity (cps)
Fractionation of the complex
mixture of tryptic peptides by
liquid chromatography. The
chromatography unit is directly
coupled to the mass
spectrometer.
Elution
time
RESULTS
Ro52
Analysis of an immunoprecipitation sample (Fas Death-Induced Signaling Complex or DISC) by MRM
7500
Several transitions were monitored for proteins known to be in
the Fas DISC (Fas, FasL, FADD, caspase-8, caspase-10, Flip),
for proteins known to be only in the negative control (BAFF,
BAFFR) and for contaminants (EF-1-1, Ro52, Ran, GAPDH,
tubulin, PIMT).
Figure 1
7000
6500
6000
Analysis by MRM
5500
5000
4500
4000
3000
In figure 3 is represented the intensity of the signal (peak area)
obtained in both samples for each transition. A signal was
detected for contaminants in both samples but this was not the
case for proteins known to be specific to one sample
Caspase-8
2000
Fas
Flip
Ef-1-1
PIMT
14-3-3
2500
1500
1000
500
0
5
10
15
20
25
950
MRM of BAFF/FasL pulldown
Contaminants
850
800
35000
750
45
50
55
Negative control :
immunoprecipitation of BAFF
Analysis by MRM
700
30000
650
25000
600
Intensity, cps
500
450
400
10000
tubulin
BAFF
350
5000
300
0
Ran
GAPDH
14-3-3b
PIMT
Tubulin
Ro52
Ef-1-1
BAFFR
BAFF
Fadd
Flip
Flip
Casp-10
Casp-8
Casp-8
Fas
Fas
FasL
FasL
250
200
150
100
protein
50
0
5
Detection of a low-abundance protein (FADD) in a total cell lysate
10
68.04
3800
3400
B 676  765.5
C 451  515.4
D 451  628.4
2600
m/z of
fragment
ions selected
for MRM
2400
451=triply charged tryptic
peptide
2200
2000
676=doubly charged tryptic
peptide
1800
1600
628.41
1400
1200
1000
800
600
200
0
67.2
67.4
67.6
67.8
68.0
68.2
68.4
Time, min
40
45
50
55
Transitions
Transitions
A 676  836.5
3000
35
MRM of total cell lysate
400
CONCLUSION
30
Time, min
68.6
68.8
69.0
69.2
Intensity, cps
836.51
25
Figure 6
3600
3200
Intensity, cps
765.47
20
MRM of recombinant FADD
2800
515.33
15
Figure 5
The peptide ENATVAHLVGALR from FADD (m/z=676 if
doubly charged and 451 if triply charged) was used to
perform MRM. In figure 4, we see the fragmentation pattern
of this tryptic peptide. The fragmentation pattern is
reproducible and the most intense fragment ions were used
to set the transitions to monitor (figure 5 and figure 6).
Figure 4
tubulin
15000
550
14-3-3
BAFF
FasL
20000
PIMT
cps (surface)
40
Ef-1-1
40000
Figure 2
900
35
Ro52
Figure 3
30
Time, min
Caspase-8
3500
tubulin
FasL
Intensity, cps
In figure 1 and 2, we can see two MRM plots (Fas DISC and
negative control). Several transitions were monitored in the same
run. The same transitions were monitored for both samples.
Proteins of the DISC
Immunoprecipitation of the Fas
DISC
68.69
A 676  836.5
168
160
B 676  765.5
150
C 451  515.4
140
D 451  628.4
130
120
110
451=triply charged tryptic
100
peptide
90
676=doubly charged tryptic
80
peptide
70
60
50
40
30
20
10
0 67.0 67.5 68.0 68.5 69.0 69.5 70.0 70.5 71.0 71.5
Time, min
PS For a given tryptic peptide, the intensity of signal depends on the chosen transition. Transition A
gives higher signals than transition D.
We are able to detect relatively well by MRM the low-abundance proteins that we aim to quantify. The higher the intensity of signal is, the better it is for quantification. To
increase the intensity of signal, several parameters were optimized like the choice of the parent ion (tryptic peptide) and of the transition as well as the MRM parameters. A
relatively good detection of FADD in total cell lysates was only possible after optimization. Now, the next step will be quantification. Absolute or relative quantification can be
performed. Absolute quantification could allow us to determine the stoichiometry of the DISC or the number of copies of one protein in a particular cell line for example.
Absolute quantification is performed by using an internal standard (which mimicks a tryptic peptide but is synthesized with a stable heavy isotope of one amino acid) put in the
sample at a known concentration. Relative quantification could allow us to detect changes in the composition of the DISC or in the level of expression of some proteins
between two conditions for example. Relative quantification is performed by differentially modifying (with light and heavy acrylamide for example) the proteins or peptides in the
two conditions.