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The New Trends of MALDI-
  MS for protein-protein
        complex
            Date: 101-04-17

      Supervisor: Prof. Hui-Fen Wu


   Student: Hani Nasser Abdelhamid
  M.Sc student at NSYSU, Taiwan (ROC)
    Tutor at Assuit university, Egypt.
Introduction
                                 Mass spectrometry components




Figure 1: Douglas A. Skoog, F James Holler, Stanley R. Crouch, Principles of Instrumental Analysis, six edition ,Thomson
                                                                        Higher Education 10 Davis Drivt' Belmont,p564.
Matrix Assisted Laser Desorption
       Ionization MALDI




        Beate Fuchs et.al. Progress in Lipid Research 2010.49 ,450–475




                          Figure 2: MALDI instrument
The matrix
MALDI TOF matrices should be:
1. embed and isolate analytes (e.g., by co-crystallization).
2. be soluble in analyte-compatible solvents.
3. vacuum-stable.
4. absorb the laser wavelength.
5. initiate co-desorption of analyte upon laser irradiation
6. promote analyte ionization .
Challenge




                 Matrixes
                            http://en.wikipedia.org/wiki/Glutathion
                            _S-transferase


GST dimer
rheumatism                   tissue necrosis
α1-antitrypsin




                                             http://trcs.wikispaces.com/Rheumatism      http://veterinaryrecord.bmj.com/


immunoglobulin G (IgG)




http://careers.bmj.com/careers/advice/view-article.html?id=2531



proteins G and A against viruses




                                                                                                          Proteomics 2008, 8, 1809–1818
Solutions

Application I                     Application II

Change the matrix               Stabilize the
                                complex using
   ex) HgTe                     cross linker
Anal. Chem 2012, 84, 1924–1930.
Effects of pH and Salt Concentration.




Figure. Intensities of SALDI-MS signals at m/z 72 160 (α1- antitrypsin and trypsin) and m/z 86 585 (IgG and protein G). (A) Ammonium
citrate solutions (50 mM; pH 4.0−9.0); (B) ammonium citrate solutions (20 mM; pH 4.0−9.0); (C) ammonium citrate solutions (pH 8.0;
20−200 mM); (D) ammonium citrate solutions (pH 5.0; 10−100 mM.
PEG 300, PEG 600, PEG 2000, Tween 20, Brij 30, Brij 35, Br
Effect of Surfactant                       56, and Brij 76 (each concentration: 1%).
                                                                                                 Brij:polyoxyethylenglycol dodecyl ether




                                                                                                                          THAP




  Figure 4. Mass spectra of α1-antitrypsin, trypsin, and their complexes, recorded through SALDI-MS using HgTe nanostructures (A) in the
  absence and (B) in the presence of 1% Brij 76, 1µL Zn(II)
Figure 5. Mass spectra of IgG, protein G, and their complexes, recorded though SALDI-MS using HgTe
nanostructures (A) in the absence and (B,C) in the presence of 0.1% Brij 76. The samples were prepared in
20 mM ammonium citrate (pH 5.0) containing 1 μM Zn(II).
Effect of Nature and Concentration of Metal Ions.

              Zn(II), Fe(III), Co(II), and Cu(II)


                                                four times less than before
Figure 6. Mass spectra of α1-antitrypsin (5 µM) and trypsin (1.7 µM) in the absence
(A) and presence (B) of 1 µM Zn(II) ions through ESI-MS. The samples were
prepared in 50 mM ammonium citrate (pH 8.0).
Stoichiometry of Protein−Protein Interactions.




                             Kf = 2 × 108                                            K f=1011




Figure 7. Molar ratio plots for the protein complexes. Complex signals at m/z 72 160 (α1-antitrypsin and
trypsin) and m/z 86 585 (IgG and protein G) in (A) and (B), respectively. (A) and (B) at a constant
concentration of α1-antitrypsin (5 μM) and IgG (10 μM), respectively. Other conditions for (A) and (B) were
the same as those used to obtain Figures 1B and 2, respectively.
Conclusion
• Simple,
• Reproducible,
• Rapid
1,1′-(suberoyldioxy)bisbenzotriazole




diphtalimide suberate   1,1′-(suberoyldioxy)bisazabenzotriazole
Figure 8. MALDI mass spectra of GST. (A) GST alone, at t ) 0 min of incubation
with a cross-linker. Panels B, C, and D show GST at t) 2 min after incubating with
DSS, SBBT, and SBAT, respectively.
DDS & DPS = 50%,
                 SBBT = 75%,
                 SBAT = 80%




Figure 9. Progression of the formation of the GST dimer vs time for
DSS, DPS, SBBT, and SBAT:, SBAT; , SBBT; , DSS; and , DPS. The
lines are the fitting curves, and the error bars correspond to 1 standard
deviation.
densitometrically
                                              ≈99% for SBAT,
                                               ≈91% for SBBT,
                                              ≈85% for DSS.




Figure 10. 1 dimensional 20% SDS PAGE of GST incubated 10 minutes with
SBBT (A),DSS (B), and SBAT (C). LMW is the low molecular weight marker.
Figure 11. MALDI mass spectra of bPrP with its specific antibody
3E7. Mixture of bPrP + 3E7 at t ) 4 min after incubation with DSS
(A) and with SBAT (B). The  represents impurities.
Figure 12. MALDI mass spectra of the mixture of ubiquitin with GST in presence of DSS
(A) or SBAT (B) after incubation time of 2 h.  corresponds to non-specific clusters of
ubiquitin and  to the nonspecific ubiquitin-GST dimer complex.
K = lysine                                                   Y = Tyrosine




Figure 13. MALDI mass spectra of the peptides Fmoc-EGGGKGGGE and Fmoc-EGGGYGGGE after 15 min of incubation with
DSS and SBAT.
Conclusion
 better efficiency
 a faster stabilization reaction
 specific complexes
Pros and Cons of the two
                         application
                                        Application II
  Application I


                                         Advantages
  Advantages
  •Simple.                               •High Intensity.

  •Rapid                                 • Specific

  •Reproducible                          •High effectiency
Disadvantages                          Disadvantages
  • Highly Toxic (HgTe).
                                     • Active sites.
  • Low intensity.
                                     • Modified protein peaks.
  •Nonspecific
                                     • Sophisticated
Limitation of the technique
• Kf or Ka

• Identification of binding mode and
  binding sites.

• dependant.

• If acidity is the main reason so, what is
  the role of buffer solution in the study???
Acknowledge
*Assuit university, Egypt
*National sun yat sen university NSYSU, ROC.

* Prof. Hui-Fen Wu.
* Prof. Shiea     *Prof. jiang.
* Prof. Tseng.    *Prof. Yang Hsiang Chan

*My colleagues and My lab mate.
A person who never made a
mistake never tried anything
new.
           Albert Einstein

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The new trends of maldi ms in protein-protein interaction

  • 1. The New Trends of MALDI- MS for protein-protein complex Date: 101-04-17 Supervisor: Prof. Hui-Fen Wu Student: Hani Nasser Abdelhamid M.Sc student at NSYSU, Taiwan (ROC) Tutor at Assuit university, Egypt.
  • 2. Introduction Mass spectrometry components Figure 1: Douglas A. Skoog, F James Holler, Stanley R. Crouch, Principles of Instrumental Analysis, six edition ,Thomson Higher Education 10 Davis Drivt' Belmont,p564.
  • 3. Matrix Assisted Laser Desorption Ionization MALDI Beate Fuchs et.al. Progress in Lipid Research 2010.49 ,450–475 Figure 2: MALDI instrument
  • 4. The matrix MALDI TOF matrices should be: 1. embed and isolate analytes (e.g., by co-crystallization). 2. be soluble in analyte-compatible solvents. 3. vacuum-stable. 4. absorb the laser wavelength. 5. initiate co-desorption of analyte upon laser irradiation 6. promote analyte ionization .
  • 5. Challenge Matrixes http://en.wikipedia.org/wiki/Glutathion _S-transferase GST dimer
  • 6. rheumatism tissue necrosis α1-antitrypsin http://trcs.wikispaces.com/Rheumatism http://veterinaryrecord.bmj.com/ immunoglobulin G (IgG) http://careers.bmj.com/careers/advice/view-article.html?id=2531 proteins G and A against viruses Proteomics 2008, 8, 1809–1818
  • 7. Solutions Application I Application II Change the matrix Stabilize the complex using ex) HgTe cross linker
  • 8. Anal. Chem 2012, 84, 1924–1930.
  • 9. Effects of pH and Salt Concentration. Figure. Intensities of SALDI-MS signals at m/z 72 160 (α1- antitrypsin and trypsin) and m/z 86 585 (IgG and protein G). (A) Ammonium citrate solutions (50 mM; pH 4.0−9.0); (B) ammonium citrate solutions (20 mM; pH 4.0−9.0); (C) ammonium citrate solutions (pH 8.0; 20−200 mM); (D) ammonium citrate solutions (pH 5.0; 10−100 mM.
  • 10. PEG 300, PEG 600, PEG 2000, Tween 20, Brij 30, Brij 35, Br Effect of Surfactant 56, and Brij 76 (each concentration: 1%). Brij:polyoxyethylenglycol dodecyl ether THAP Figure 4. Mass spectra of α1-antitrypsin, trypsin, and their complexes, recorded through SALDI-MS using HgTe nanostructures (A) in the absence and (B) in the presence of 1% Brij 76, 1µL Zn(II)
  • 11. Figure 5. Mass spectra of IgG, protein G, and their complexes, recorded though SALDI-MS using HgTe nanostructures (A) in the absence and (B,C) in the presence of 0.1% Brij 76. The samples were prepared in 20 mM ammonium citrate (pH 5.0) containing 1 μM Zn(II).
  • 12. Effect of Nature and Concentration of Metal Ions. Zn(II), Fe(III), Co(II), and Cu(II) four times less than before
  • 13. Figure 6. Mass spectra of α1-antitrypsin (5 µM) and trypsin (1.7 µM) in the absence (A) and presence (B) of 1 µM Zn(II) ions through ESI-MS. The samples were prepared in 50 mM ammonium citrate (pH 8.0).
  • 14. Stoichiometry of Protein−Protein Interactions. Kf = 2 × 108 K f=1011 Figure 7. Molar ratio plots for the protein complexes. Complex signals at m/z 72 160 (α1-antitrypsin and trypsin) and m/z 86 585 (IgG and protein G) in (A) and (B), respectively. (A) and (B) at a constant concentration of α1-antitrypsin (5 μM) and IgG (10 μM), respectively. Other conditions for (A) and (B) were the same as those used to obtain Figures 1B and 2, respectively.
  • 16.
  • 17. 1,1′-(suberoyldioxy)bisbenzotriazole diphtalimide suberate 1,1′-(suberoyldioxy)bisazabenzotriazole
  • 18. Figure 8. MALDI mass spectra of GST. (A) GST alone, at t ) 0 min of incubation with a cross-linker. Panels B, C, and D show GST at t) 2 min after incubating with DSS, SBBT, and SBAT, respectively.
  • 19. DDS & DPS = 50%, SBBT = 75%, SBAT = 80% Figure 9. Progression of the formation of the GST dimer vs time for DSS, DPS, SBBT, and SBAT:, SBAT; , SBBT; , DSS; and , DPS. The lines are the fitting curves, and the error bars correspond to 1 standard deviation.
  • 20. densitometrically ≈99% for SBAT, ≈91% for SBBT, ≈85% for DSS. Figure 10. 1 dimensional 20% SDS PAGE of GST incubated 10 minutes with SBBT (A),DSS (B), and SBAT (C). LMW is the low molecular weight marker.
  • 21. Figure 11. MALDI mass spectra of bPrP with its specific antibody 3E7. Mixture of bPrP + 3E7 at t ) 4 min after incubation with DSS (A) and with SBAT (B). The  represents impurities.
  • 22. Figure 12. MALDI mass spectra of the mixture of ubiquitin with GST in presence of DSS (A) or SBAT (B) after incubation time of 2 h.  corresponds to non-specific clusters of ubiquitin and  to the nonspecific ubiquitin-GST dimer complex.
  • 23. K = lysine Y = Tyrosine Figure 13. MALDI mass spectra of the peptides Fmoc-EGGGKGGGE and Fmoc-EGGGYGGGE after 15 min of incubation with DSS and SBAT.
  • 24.
  • 25. Conclusion  better efficiency  a faster stabilization reaction  specific complexes
  • 26. Pros and Cons of the two application Application II Application I Advantages Advantages •Simple. •High Intensity. •Rapid • Specific •Reproducible •High effectiency Disadvantages Disadvantages • Highly Toxic (HgTe). • Active sites. • Low intensity. • Modified protein peaks. •Nonspecific • Sophisticated
  • 27. Limitation of the technique • Kf or Ka • Identification of binding mode and binding sites. • dependant. • If acidity is the main reason so, what is the role of buffer solution in the study???
  • 28. Acknowledge *Assuit university, Egypt *National sun yat sen university NSYSU, ROC. * Prof. Hui-Fen Wu. * Prof. Shiea *Prof. jiang. * Prof. Tseng. *Prof. Yang Hsiang Chan *My colleagues and My lab mate.
  • 29. A person who never made a mistake never tried anything new. Albert Einstein