Processing of Serum Proteins Underlies the Mass ... - ACS Publications

Jan 20, 2003 - Keywords: mass spectrometry • myocardial infarction • diagnostic • fibrinogen ... in mass spectral diagnosis based on spectral pr...
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Processing of Serum Proteins Underlies the Mass Spectral Fingerprinting of Myocardial Infarction John Marshall,*,† Peter Kupchak, Weimin Zhu, Jason Yantha, Tammy Vrees, Shirley Furesz, Kellie Jacks, Chris Smith, Inga Kireeva, Rulin Zhang, Miyoko Takahashi, Eric Stanton,‡ and George Jackowski§ SYNX PHARMA, 1 Marmac Drive, Toronto, Ontario, Canada, M9W 1E7 Received January 20, 2003

The MALDI-TOF spectra of peptides from the sera of normal and myocardial infarction patients produced patterns that provided an accurate diagnostic of MI. In myocardial infarction, the spectral pattern originated from the cleavage of complement C3 alpha chain to release the C3f peptide and cleavage of fibrinogen to release peptide A. The fibrinogen peptide A and complement C3f peptide were in turn progressively truncated by aminopeptidases to produce two families of fragments that formed the characteristic spectral pattern of MI. Time course and inhibitor studies demonstrated that the peptide patterns in the serum reflect the balance of disease-specific-protease and aminopeptidase activity ex vivo. Keywords: mass spectrometry • myocardial infarction • diagnostic • fibrinogen alpha peptide • complement C3f • sera

Introduction There has been an explosion in interest in the use of mass spectrometry (MS) as a tool to identify patients with a particular disease or other physiological conditions.1-3 To date, the field has focused on the use of highly sensitive but low-resolution MALDI-TOF1 mass spectrometers termed SELDI-TOFs to record spectra of the low molecular mass proteins and polypeptides in sera or biological fluids.4 The Ciphergen Biosystems SELDITOF is a single flight path MALDI-TOF where the sample target may be a selective surface. However, in principle, any type of mass spectrometer or surface could be used to generate a library of analytes5 associated with the control versus diseased states, or with other physiological conditions such as drug interactions. The type of mass spectrometry employed could also be a complex experiment such as an LC-MS or LC-MS/ MS run. The resulting spectral patterns act as fingerprints that are mathematically analyzed to identify the sample as belonging to a certain disease or physiological condition. Consensus is emerging that SELDI peptide profiles have great utility as diagnostics.6 However, because the peptides and small proteins that form these patterns have by and large not been identified there has been to date been little understanding of what mechanisms produce the spectral patterns. Mass spectrometric profiling of the low molecular mass peptides in blood or other * To whom correspondence should be addressed. Department of Chemistry and Biology, Faculty of Engineering and Applied Science, Ryerson University, Toronto, Ontario, Canada. Phone: 416-798-3445. Fax 416-7983447. E-mail: [email protected]. † Department of Chemistry and Biology, Faculty of Applied Arts and Science, Ryerson University. ‡ Department of Cardiology, St. Joseph’s Hospital, McMaster University. § Department of Pathobiology, Hospital for Sick Children, University of Toronto. 10.1021/pr030003l CCC: $25.00

 2003 American Chemical Society

biological fluids may provide a means to diagnose many diseases and physiological conditions in man. The mass spectral diagnostic technique is simple and inexpensive to develop into a working assay, and similar laboratory methods can be used to discriminate between a variety of diseases without specialized reagents for each condition under study. Hence, mass spectrometry may provide methods to detect and discriminate between so-called orphan or rare diseases where traditional diagnostics have not been economical to develop. In contrast to genetic testing for known sequences that may indicate the propensity to develop disease, mass spectral diagnosis may be able to detect the manifestation of the phenotype itself without knowledge of the genetic lesion(s) involved. Computer assisted classification of the mass spectra requires no characterization of genetic materials. This may in turn obviate many ethical concerns regarding genetic diagnostic technologies. Computer assisted analysis of mass spectra as an aid to diagnosis has been reported using a two-step learning algorithm for the comparison of SELDI-TOF-MS spectra of biological fluids.7 Alternatively, quantitative decision tree analysis of mass spectra has been employed.8 The role of the biochemist in this enterprise is to identify the sample preparations that reveal large differences between physiological conditions and thus avoid elaborate mathematical treatments. In this paper, we report the use of a combination of quantitative decision analysis combined with multivariate analysis to provide a statistically appropriate and powerful method of comparing peptide distributions. There is now intense interest in mass spectral diagnosis based on spectral profiling of the families of low molecular mass proteins polypeptides in sera or plasma. However, to date no one has shown the mechanism underlying the presence of the diagnostic peptides in blood. Journal of Proteome Research 2003, 2, 361-372

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research articles Although many papers have now shown the existence of different polypeptides in biological fluids from various disease states, we have not as yet identified most of the peptides. Within the past decade, the Edman degradation method that was typically used for the identification of unknown proteins has been complemented by rapid advances in the use of ESI9and MALDI10 followed by MS/MS fragmentation.11 In this paper, we used two kinds of MS/MS analysis, LC-ESI-ION TRAP and MALDI-Qq-TOF12 to identify some of the peptides in the fingerprint. MS/MS analysis is tandem mass spectrometry, where the first mass analyzer isolates a certain peptide; the peptide is fragmented by acceleration through an electric field in the presence of homonuclear gas molecules producing CID fragmentation, and the fragments are analyzed by a second mass analyzer that records the peptide fragmentation spectra. That spectrum is then compared using a computer to the predicted fragmentation pattern of proteins encoded by the human genome, cDNA banks and EST data. In the case of QqTOF13-16, a quadrupole mass analyzer Q was connected in series to a TOF analyzer via a radio frequency only quadropole q that acts as a trap to fragment the peptide of interest. In the case of the ION-TRAP,1718,19 the same mass analyzer is used to isolate and collect the analyte, fragment the peptide, and then record the fragmentation spectra. Thus, in the ION TRAP, these three functions are separated in time instead of space, as is the case with other tandem mass spectrometers. The large-scale computational identification of proteins based on mass spectrometry is sometimes termed proteomics.20 Myocardial infarction (MI) is a major cause of death in men and women, especially in western society.21,22 However, myocardial necrosis remains difficult to diagnose definitively without specialty reagents and optimized assays.23,24 Present biomarkers often take several hours to appear in the serum. It remains possible that the victims of massive MI have been previously suffering minor events that have gone undiagnosed. Because effective treatment requires instant diagnosis, it is particularly germane to develop rapid diagnostics for MI. Hence, we applied the mass spectral diagnostic technique to produce a rapid and reliable assay for MI. Deeper mass spectral exploration of diagnostic peptide patterns may reveal new insights into the cause of disease or disease symptoms. Pursuit of spectral elements from diseases such as MI may lead to mechanisms of disease. Mounting evidence indicates that an inflammatory reaction following the acute event results in damage to the myocardial tissue that is mediated by a complement driven cellular attack.25 The beginning of the inflammatory response may include the recruitment of the early complement factor C3 to the site of necrotic cells. C3 precursor is cleaved to form the C3 beta chain and the C3 alpha chain. The C3 beta chain remains intact. The C3 alpha chain contains the thioester site that may attach to cellular surface via the thioester link and direct the activation of white blood cells.26,27 Proteolytic processing of the C3 alpha chain may result in the generation of fragments including C3f. To our knowledge, the generation of the C3f fragment has not been previously associated with myocardial infarction. However, myocardial infarction has been associated with the development of blood clots from the proteolytic activation of the fibrinogen clotting cascade upon rupture of unstable atherosclerotic lesions (Fareed et al., 1998). Processing of fibrinogen to produce activated fibrin releases the soluble fibrinogen peptide A (Eisenberg and Sherman et al., 1985). 362

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Material and Methods Materials. Except where indicated, all dry chemicals were obtained from the Sigma-Aldrich chemical company (St. Louis, MO) and were of a fine grade. All solvents were of an optical grade or better. DEAE chromatographic resin was obtained from BIORAD laboratories (Hurcules, CA). Reversed phase resin was obtained from Millipore laboratories (Bedford, MA). The C3b alpha chain antibody was obtained from Research Diagnostics (Flanders, NJ). Blood collection tubes were obtained from Becton, Dickinson (Franklin Lakes, NJ). Blood Samples. Blood samples were obtained under a human ethics protocol. The blood from MI patients was drawn within 2 h of the suspected event, and in each case the presence of heart attack was confirmed by standard methods.23 The protocol ensures that plasma or serum is collected and stored at room temperature for no more than 2 h before freezing at -70 °C. Blood samples were drawn into citrated tubes for plasma and into standard tubes for sera. The samples were thawed, aliquoted, and re-frozen once before being used and discarded. In this study, we demonstrated that processing of serum proteins contributes to MALDI-TOF profiles using the sera of six randomly selected MI and six randomly selected normal patients. MALDI-MS. Sera for MALDI-TOF analysis was diluted 10 fold in 0.1% TFA. Typically, 10 µL of serum was used for the analysis. The peptides were collected in a batch mode by passage over C18 reversed phase resin washed with several column volumes of 0.1% TFA and eluted in one batch with 2 µL of 50% acetonitrile in water with 0.1% TFA and 5% formic acid. The eluted peptides were dried on to gold MALDI targets. After allowing all of the samples to dry evenly, an energy absorbing molecule or matrix was applied. A few milligrams of the matrix CHCA was deposited into a mass spec compatible sample tube, the matrix was washed by re-suspension in 50% acetonitrile in 0.1% TFA in water before the wash solution was discarded and the matrix was covered with fresh 50% acetonitrile 0.1% TFA to form a saturated solution. One µL of saturated matrix solution was applied to each MALDI target spot immediately before sampling. The data were collected using a TOF MS model PBSII provided by Ciphergen Biosystems (Freemount, CA).4 Statistical Analysis of MALDI-MS Spectra. Instead of analyzing all of the MALDI spectra peaks together by multivariate analysis, we broke the spectra into a series of mass windows, analyzed the peaks in each mass window separately, and determined which mass ranges contained peaks that showed a quantitative difference in intensity between normal and MI by one-way ANOVA. Subsequently, the sets of peaks that showed significant differences between normal and MI subjects were reanalyzed by multivariate analysis. Analytes detected in MALDI-MS spectra were categorized into 5 D windows. Raw data was analyzed without noise filtering or other treatments. Within each window, a nested factor design arrangement was assumed, with the type of group (MI vs control) considered a fixed effect, and six random individual subjects nested within each group. The appropriate F statistic associated with the null hypothesis of equality in mean signal strength between the MI group and the control group was computed within each 5 D window, by dividing the mean square associated with the type of group by the mean square associated with subjects nested within a group. Significance levels of R ) 0.005 and R ) 0.001 were considered for the present analysis; with respect to the windows which showed

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Mass Spectral Diagnosis of Heart Attack

extreme differences between the two groups (i.e., where the p-value associated with the F test of interest was smaller than the appropriate significance level), the median signal strength for each subject was computed and retained for subsequent multivariate analysis. Specifically, a linear discriminant analysis was employed using the technique of “leave one out” crossvalidation in order to classify each subject as either a control subject or an MI subject, based on the relative proximity of the vector of signal strengths for that subject to the mean vectors of signal strengths for the two classes of subjects (previously computed by leaving out the vector of signal strengths for the subject in question). In addition, the posterior probability of assigning the subject to each of the two classes was computed using an application of Bayesian methodology.28 All statistical analyses were performed using S-PLUS Version 6 software for Windows (Insightful Corporation, Seattle, WA). Thus, we used a computer to automatically quantify the differences in spectral intensity over a series of peptide mass windows. Where quantified differences in intensity by at least a factor of 2 were observed, their significance was confirmed by ANOVA and the data was copied into a matrix. All the quantifiable, statistically significant differences in the matrix were then subjected as a group to multivariate analysis comparing the features of interest from the control and MI spectra. MS/MS by MALDI-Qq-TOF. Polypeptides from sera samples were prepared for MALDI analysis by reversed phase chromatography as described above but spotted on a neutral target suitable for a Micromass MALDI-Qq-TOF (Micromass, Manchester, UK). MS/MS spectra were collected using CHCA as a matrix. The fragment patterns were searched against a nonredundant library of DNA, cDNA’s EST, and proteins assembled from publicly available data in September 2002. The MS/MS fragmentation patterns were correlated against the databases using MASCOT. Only MS/MS spectra with significant Mowse scores are reported as previously described.29,30 MS/MS by LC-ESI-ION TRAP. Peptides were collected from sera using a single-batch, reversed-phase chromatography by dilution 10-fold in 0.1% TFA in water before collection over C18 resin, washing in at least three column volumes and elution with a final v/v/ of 50% acetonitrile, 0.1% TFA before dilution in 0.1% TFA in water and subsequent re-separation by gradient C18 reversed phase chromatography (Agilent 0.3 mm ID, 15 cm column). The sample was analyzed over a 90 min gradient from 5% to 65% acetonitrile at a flow rate of 1 µL per minute with an Agilent 1100 series capillary pump (Palo Alto CA) through a VYDAK 150 × 0.3 mm C18 column (Hysperia CA) via a metal needle electro-spray head at 3000 V into a Decca XP-100 ION TRAP (Thermo-Finnegan, San Jose, CA). The resulting MS/MS spectra were analyzed by SEQUEST.31 Peptides identified by SEQUEST with significant X-correlations were reported as previously described.32 Alpha fibrinogen and C3f fragments present in the MI samples that were not abundant in the control samples were obtained by subtracting the set of MS/MS found in the controls from that in the MI subjects. DEAE Chromatography, SDS-PAGE, and Western Blot. DEAE columns were equilibrated with binding buffer (100 mM PBS) according to the manufacturer’s protocol. Serum samples from control and MI patients were mixed with binding buffer and passed over the column. The column was washed in five volumes of binding buffer before eluting with 100 mM PBS plus 500 mM NaCl as described by the manufacturer. For SDS-PAGE

analysis, the protein eluted from DEAE columns resolved on tricine gels.33 For western blots, gels were electrotransferred onto PVDF in methanol-glycine buffer,34 blocked in 5% skim milk powder before incubating with mouse anti C3b alpha and detected with Goat anti mouse HRP (Jackson Laboratories, West Grove, PA) using ECL (Amersham-Pharmacia, Uppsala, Sweeden) on Kodak ECL film (Toronto, Canada). For protein sequencing, the gel was stained with CBBR in 40% methanol and 10% acetic acid before the indicated band was cut from the gel, trypsinized30 and identified by MALDI-Qq-TOF using a PE SCIEX, QSTAR pulsar I (MDS-SCIEX, Concord, ON, Canada) and LC-ESIION TRAP (Finnegan, Decca XP-100). Proteolysis of Sera and Plasma Samples. Fresh plasma samples for time course studies were collected in citrated tubes and immediately centrifuged at 14 000 g for 30 s; the supernatant was collected and the plasma rapidly diluted 10 fold in 0.1% TFA. For time course studies, the plasma was left on the bench for the times indicated in the results, before quenching with 10 volumes of 0.1% TFA. PMSF was dissolved in a 0.5 M stock solution in DMSO immediately before use. Alternatively, the PMSF was weighed out and added directly to the serum with similar results. The reaction was permitted to proceed for the times indicated in the results before quenching in 0.1% TFA.

Results By enriching peptides from acidified sera with C18 resin and analyzing the results with a MALDI-TOF it seems possible to discriminate between physiological states. For example, in Figure 1 we show distinctive variations in patterns between normal human sera (NHS) and sera from Myocardial Infarction (MI) subjects. These results were consistent with previous workers who also found distinctive patterns in the sera of cancer patients.1,3 Pre-fractionating sera by reversed-phase chromatography prior to MALDI-TOF analysis produced exceptionally clear differences between normal human sera and MI sera with reasonably good peak shape and symmetry, high signal-to-noise ratios, and baseline to baseline separation of most peaks. In Figure 1, we show the reproducibility of the method with 5 random NHS and MI samples ionized with CHCA matrix. Similar trends were obtained when sinipinic acid served as the matrix (not shown). We used a combination of the fundamental principles in decision tree analysis8 and multivariate analysis35,36 to compare the spectra presented in Figure 1. When a significance level of R ) 0.001 was utilized for the preliminary ANOVA screen, a total of 45 windows were identified within which the difference in mean signal strength between control and MI sera samples was deemed statistically significant. Figure 2 displays the median signal strengths with respect to both control samples and MI samples for each of these windows. The results of the discriminant analysis are displayed in Table 1; all twelve subjects were correctly classified with a minimum posterior probability of 99.9999%. When a significance level of R ) 0.005 was utilized, 200 windows were identified within which the difference in mean signal strength between control sera samples and MI sera samples was deemed significant (Figure 2). By applying the discriminant analysis on the data within these windows, all twelve subjects were correctly classified with a minimum posterior probability of 99.89% (Table 1). It is interesting to note that by employing a lower level of statistical significance, the dimensionality of the retained data set increased 4-fold, with no concomitant increase in the predictive power of the resulting discriminant analysis. The statistical Journal of Proteome Research • Vol. 2, No. 4, 2003 363

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Figure 1. Comparison of mass spectra of control and myocardial infarction serum samples resolved on the Cyphergen Biosystems PBS II MALDI-TOF. The peptides from 10 ul of sera were collected by batch reversed phase chromatography and eluted onto the targets spots of gold chips and matrixed with 1 µL of saturated CHCA matrix immediately before analyzing at a laser intensity of 200 and a sensitivity setting of seven. Five representative spectra of control (left) and MI (right) patients are shown.

techniques employed here appear to provide a powerful methodology with respect to the correct classification of MI and control subjects. 364

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We proceeded to sequence the distinctive peaks in NHS and MI samples using MALDI-Qq-TOF.13,14 We found that the peaks observed in NHS and MI samples were fragments of common

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Mass Spectral Diagnosis of Heart Attack

Table 1. Statistical Probability Associated with Classification of Patients as Either Control or Myocardial Infarction Using Pre-fractionation of the Sera by Reversed-Phase C18 Resin Prior to MALDI-TOF Analysis Using the Cyphergen Biosystems PBSIIa

Figure 2. Distribution of peptides between normal and MI sera that differ in median intensity by a statistically significant amount. The data comprising the spectra shown in Figure 1 plus additional spectra were collected in numerical form with signal strength coordinated with mass. Top: Median signal strengths corresponding with mass levels showing significant differences between controls and MI subjects at a significance level of R ) 0.001. Bottom: Median signal strengths corresponding with mass levels showing significant differences between controls and MI subjects at a significance level of R ) 0.005.

sera proteins. Peptides from human sera albumin were observed in the control spectra (Figure 3). The family of peaks observed in MI samples originated from the C3f portion of the complement C3b alpha chain and the alpha fibrinogen peptide A (Figure 3). MALDI-Qq-TOF analysis recorded the presence of the C3f fragment of complement C3 and the C3f fragment progressively missing amino acids from the N terminus and similar truncations of fibrinogen peptide A. In fact, we even observed, and MS/MS analyzed, each member of a near perfect ladder of C3f in the sera of a heart attack patient by MALDIQq-TOF (Figure 4). The MS/MS analysis of the peptides showed the full C3f fragment SKITHRIHWESASLLR and the loss of residues from the N-terminus resulting in a ladder of fragments. The smallest fragment observed was RIHWESASLL. We obtained MS/MS fragment patterns for each member of the family of peaks observed by MALDI-MS and searched these against the NCBI and Swiss Pro databases to confirm their identify as sub-fragments of C3f. We note that in this case of a progressive loss of single amino acids from the N termini the sequence can be called directly from the MS spectra. Thus, we found that the C3f fragment of complement C3 was released, presum-

subject no.

true subject class

1 2 3 4 5 6 7 8 9 10 11 12

NHS NHS NHS NHS NHS NHS MI MI MI MI MI MI

subject no.

true subject class

1 2 3 4 5 6 7 8 9 10 11 12

NHS NHS NHS NHS NHS NHS MI MI MI MI MI MI

posterior probability of belonging to class: NHS

MI

classification

0.9999999 0.9999999 0.9999999 0.9999999 0.9999999 0.9999999 0.0000001 0.0000001 0.9999999 0.9999998 0.9999998 0.9999999

NHS NHS NHS NHS NHS NHS MI MI MI MI MI MI

posterior probability of belonging to class: NHS

MI

classification

0.9997754 0.9998278 0.9998271 0.9999064 0.9997390 0.9997211 0.0002153 0.0001429 0.0000299 0.0010233 0.0009231 0.0001113

0.0002246 0.0001722 0.0001729 0.0000936 0.0002610 0.0002789 0.9997847 0.9998571 0.9999701 0.9989767 0.9990769 0.9998887

NHS NHS NHS NHS NHS NHS MI MI MI MI MI MI

a Top: Posterior probabilities of classification of control and MI subjects, with respect to the retained data from mass levels showing significant differences between controls and MI subjects at a significance level of R ) 0.001. Bottom: Posterior probabilities of classification of control and MI subjects, with respect to the retained data from mass levels showing significant differences between controls and MI subjects at a significance level of R ) 0.005.

ably by the action of a serine centered endoproteinase.37,38 However, we also observed that the released C3f fragment was apparently degraded from the N-terminus by the action of an N-terminal exopeptidase, i.e., aminopeptidase.39 Although most of the interest in sample profiling to date has been in the use of MALDI-TOF,5 we also point out that other mass spectral devices might be used for comparison or physiological states. For example, when we compared MI versus normal sera samples on LC-ESI-ION TRAP we also observed the presence of peptides of alpha fibrinogen and C3 in the sera of MI patients. We found the presence of the complement C3f fragments and N-terminally truncated C3f in the MI sample [SSKITHRIHWESASLL, THRIHWESALL, and IHWESLL] but we also found other fragments of complement C3 [(T)MSILDISMMTGFAPDTDDLK and (S)HVSELLML] in MI but not in the normal sera samples. In addition, we detected a near perfect ladder of N-terminal deleted peptides of alpha fibrinogen (Table 2). Thus the LC-ESI-ION TRAP showed the presence of a ladder of fibrinogen peptides that, similar to C3f, had apparently also been degraded by a N-terminal exopeptidase, i.e., aminopeptidase. Hence, we identified C3f and fibrinogen peptide A in the serum of MI patients with both MALDI and Journal of Proteome Research • Vol. 2, No. 4, 2003 365

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Marshall et al. Table 2. N-Terminal Deletion Series of Fibrinogen Peptide A Obtained from the Sera of MI Patients Using LC-ESI-ION TRAPa

Figure 3. Identity of peptides in the control and MI sera as determined by a MALDI-Qq-TOF using a Micromass spectrometer related to MALDI-TOF spectra obtained with the Ciphergen Biosystems PBSII. Top: A MALDI-TOF spectrum of control sera showing the identity of the peptides. The H indicates the peptide is derived from Human Serum Albumin. Bottom: A MALDI-TOF spectrum of MI sera showing the identity of the peptides. The letters C and A indicate that the peptide or fragment was derived from Complement C3f and FPA, respectively.

a The peptides from the sera of MI patients were collected by batch reversed phase chromatography over C18 resin before analysis by LC-ESIION TRAP. The ladder of N-terminally deleted alpha fibrinogen fragment was found with strong signal intensity in the sera of MI patients. The 8 peptides shown had X-correlation values ranging from 4.3 to 2.78 as calculated by Sequest.

Figure 5. Western blot against the complement C3 alpha chain from control and MI serum pre-fractionated with DEAE sepharose. Five typical MI and 3 typical control serum samples are shown. The precursor complement C3 molecule, the full-length alpha chain (control) and a processed form of the C3 alpha chain (predominately in MI) are apparent. The arrow shows the location of the ∼68 kD processed form in control samples that is absent in MI. The approximate position of the molecular weight markers are shown.

MI patients compared to controls and both methods agreed on the presence of N-terminally deleted peptide fragments.12

Figure 4. Example of an N-terminal deletion series of the C3f fragment of complement C3 as determined by MALDI-Qq-TOF. Note that the parent C3f fragment is produced by a tryptic-like cleavage on the N-terminal side of arginine but occasionally with cleavage on the C-terminal side of arginine. The C3f fragment shows the progressive loss of amino acids from the N-terminal end.

ESI based spectrometry; both methods agreed that C3 peptides and alpha fibrinogen were found predominantly in the sera of 366

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Because C3f is derived from the proteolytic cleavage of the complement C3 alpha chain, the generation of the C3f fragment in MI samples indicated that the proteolytic processing of C3b alpha had occurred. To confirm this prediction, we performed western blot analysis with a monoclonal antibody against the C3b alpha chain. We determined empirically that DEAE prefractionation of sera yielded the clearest picture of C3 alpha chain proteins when gels were visualized by western staining. We confirmed that alternative proteolytic processing of C3b occurred in MI patients by using a Western blot against the DEAE fraction with an anti C3b antibody. In normal human sera, we found that the complement C3 chain was typically fragmented into three main polypeptides with relative molecular masses of approximately 120, 68, and 42 kD (Figure 5). By contrast, in MI sera, the polypeptide with mass of 68 kD was essentially missing, while the protein product with a mass of about 42 kD was more intense.

Mass Spectral Diagnosis of Heart Attack

Figure 6. CBBR stained gel of sera from control and MI sera prefractionated with DEAE sepharose. The sera were resolved by SDS-PAGE prior to staining with CBBR 250. The location of the band sequenced by MALDI-Qq-TOF and LC-ESI-ION TRAP is shown by an arrow. The standard masses on the right-hand edge of the figure in descending order were: 250, 150, 100, 75, 50, 37, and 25 kD. From the band indicated the sequences VHQYFNVELIQPGAVK and SGSDEVQVGQQR showed significant mathches by MALDI-Qq-TOF and the sequences SGSDEVQVGQQR, NTLIIYLDK, and VTIKPAPETEK showed significant matches, whereas QLANGVDR was not significant, by ION TRAP.

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Figure 8. Effect of time on the MALDI-TOF spectra of normal human plasma. Venous blood was collected into citrated tubes and centrifuged at 14 000 g for 30 s before the plasma was collected and either immediately diluted (Time 0), or left on the bench at 25 °C for the time indicated prior to dilution 10-fold in 0.1% TFA in water followed by batch collection of the peptides by reversed phase C18 chromatography. The sample was analyzed at a laser intensity of 210 and a sensitivity of 7 on a Ciphergen Biosystems PBSII. The result of one experiment representative of three is shown.

of the C3 alpha chain that would be released after proteolytic cleavage of C3f. Hence, we apparently found that this band is comprised of the bulk of C3 alpha from the C3f site to the C-terminus of the molecule.

Figure 7. Summary of mass spectral data collected concerning complement C3 processing. The complement C3f fragment (aa1303 to aa1320) was detected by both MALDI-Qq-TOF and LCESI-ION TRAP. The portion of the C3 alpha chain C-terminal to the C3f fragment was resolved by SDS-PAGE and six peptides were identified by MALDI-Qq-TOF and ESI-ION TRAP (see Figure 6). The letters reflect the nomenclature regarding the structural features of complement C3. The thioester site that may covalently attach to cellular surfaces is located in segment DG.

In Figure 6, we depict the presence of a fragment of the carboxy-terminal region of the C3 alpha chain displaying a relative molecular mass of about 40 kD as detected by SDSPAGE. The CBBR stained gel reveals an apparently greater amount of the 40 kD band. We confirmed the identity of this band as the carboxy terminal region of C3 alpha using MS/MS fragmentation by both MALDI-Qq-TOF and LC-ESI-ION TRAP. The result of the peptide coverage obtained with respect to the complement C3b sequence by both LC-ESI-ION TRAP and MALDI-Qq-TOF is presented in Figure 7. The peptide coverage of this C3 alpha fragment is intense on the C terminal side of the C3f fragment site, but no sequences were detected on the N-terminal side of the C3f fragment. Moreover, the mass of the protein product is also consistent with the C-terminus

As noted above, upon MS/MS analysis of the main polypeptide peaks of less than 3000 D in normal human sera with a MALDI-Qq-TOF, we also found that the main peptides were proteolytic fragments of commonly abundant sera proteins such as HSA. As the distinctive pattern in MI patients was derived from complement and fibrinogen fragments, and that in the control subjects was derived from other abundant proteins such as serum albumin, we examined the hypothesis that the astonishing utility of the disease specific SELDI profiles resulted from the differential modification of common blood proteins that uniquely reflect each physiological state. Furthermore, we attempted to reveal the mode by which these diagnostic patterns were formed. One of the initial questions we posed was to determine whether these fragmentation patterns exist in vivo or if they are generated ex vivo. Because sera, by nature, is an ex vivo artifact produced by the activation of the proteolytic coagulation cascade, for the initial experiments, we used both freshly drawn plasma and plasma that had been left on the bench for various lengths of time. We observed that absolutely fresh plasma does not show the characteristic family of peptides that were found in plasma left sitting at room temperature for 4 h (Figure 8). The pattern of fragments in plasma changes within as little as 2 h at room temperature, with some of the larger polypeptides apparently lost from the spectra and some lower mass peptides apparently increasing in intensity. Thus, we Journal of Proteome Research • Vol. 2, No. 4, 2003 367

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Figure 9. Effect of the iron-sulfur protease inhibitor EDTA and the serine-centered protease inhibitor PMSF on the MALDI-TOF spectra of normal human sera as detected by MALDI-TOF. Crystals of PMSF or the sodium salt of EDTA were added directly to 1 mL of sera and incubated for 4h before sampling. At the time of sampling a 25 µL aliquot of sera was diluted 10 fold in 0.1% TFA before collection of peptides by batch C18 reversed phase chromatography and spotting on gold MALDI-TOF targets. The sample was analyzed at a laser intensity of 190 and an amplifier sensitivity of 7 on a Ciphergen Biosystems PBSII. The result of one experiment representative of three is shown. The arrows show an example of variation in peak intensity with treatment.

observed that the patterns in plasma were apparently generated ex vivo and were generally stable for a couple of hours once formed. These changes in the plasma profile soon after removal of the blood from the body indicate that some process occurs in the blood ex vivo that influences the peptide spectra. The most obvious possibility to pursue was the role of proteases. To establish a role for proteases in the formation of the diagnostic peptide pattern in sera, we employed the serinecentered protease inhibitor PMSF and the iron sulfur protease inhibitor EDTA. We observed that incubation of sera samples with EDTA had no effect on the distribution of peptides in the mass spectra by MALDI-TOF (Figure 9). However, we observed a concentration-dependent effect of PMSF on the pattern of polypeptides in the MALDI-TOF spectrum. Concentrations of PMSF in the micromolar range had little effect on the peptide pattern, but concentrations of 1 mM PMSF or greater produced a dramatic reduction in signal strength of higher mass polypeptides and an increase in the apparent complexity of lower mass peptides. Thus we observed that the peptide distribution across the serum mass spectrum could be perturbed by the inhibition of serine centered proteases. The perturbation of the peptide profile by PMSF indicates that the profile results in part from the action of proteases. We also examined the effect of time on the peptide profile and the interaction of time and serine protease inhibition. We 368

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Figure 10. Interaction of time and PMSF on the MALDI-TOF spectra of Normal human sera. Aliquots of human sera were thawed and were either instantaneously treated with PMSF or left untreated. Twenty-five µL aliquots were then immediately diluted (Time 0), or left on the bench at 25 °C for the time indicated before being diluted 10 fold in 0.1% TFA. The peptides were collected by batch reversed phase chromatography, eluted onto gold MALDI targets matrixed with CHCA and analyzed at a laser energy 210 and a sensitivity of 7 on a Ciphergen Biosystems PBSII. The result of one experiment representative of three is shown. The arrows show an example of variation in peak intensity with time and treatment.

found that the profile of the sera changed with the time of incubation at room temperature (Figure 10). After about 8 h of incubation, clear alterations in the peptide profile were observed in the sera. These differences became even more pronounced after 24 h of incubation at room temperature. These results indicated that the sera was unstable and that the increasingly complex profile is a direct reflection of the degradation with time of proteolytic activity. This observation was reinforced by the interaction of time with serine proteinase inhibitor treatment. No difference was observed in normal sera immediately after the addition of the PMSF. However, within as little as 2 h, and typically between 4 and 8 h of incubation, PMSF showed distinct effects on the pattern of peptide mass distribution, resulting in the appearance of some higher molecular mass peptides. A strong interaction between time and PMSF treatment was observed within 24 h, when the failure of PMSF treated sera to generate peptide fragments via endopeptidase activity apparently resulted in a generalized loss of peptides from the MALDI-TOF spectrum.

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Mass Spectral Diagnosis of Heart Attack

Discussion

Figure 11. Effect of serine endo proteinase inhibition on the MALDI-TOF spectral pattern of normal human and MI sera. Sera were either sampled immediately or left on the bench after treatment with PMSF for the time indicated, before it was diluted in acid. The peptides were collected by batch reversed phase chromatography, eluted onto gold MALDI targets, matrixed with CHCA and analyzed at a laser intensity of 190 and a sensitivity of 7 with a Ciphergen Biosystems PBSII. The result of one experiment representative of three is shown.

The requirement for time to reveal the effects of PMSF indicated that the change in the spectra was not a direct result of the presence of PMSF but was the result of the inhibitor’s influence on enzymatic activity during the course of incubation. In addition to the control of adding PMSF to sera immediately before processing, we also used acidified sera incubated with PMSF for several hours or added PMSF directly to boiled sera before incubation to ensure that the loss of peptides from the mass spectra was not due to any inhibitory effect of PMSF on the MALDI ionization process (not shown). Thus, we observed that the effect of PMSF in reducing peptide complexity and signal strength did not result from a contaminating effect of PMSF on the MALDI process but seemed to result from the inhibition of cleavage by serine proteases. Hence, we can state with confidence that we found the low molecular mass polypeptide patterns in human sera to be dependent in part on the activity of proteases. The distinctive patterns of peptides in both normal human sera and MI sera were found to be sensitive to PMSF over time. Before the addition of PMSF, the normal human sera and MI sera showed different distributions of polypeptides (Figure 11). However, upon addition of PMSF, the profiles appeared remarkably similar within several hours. Hence, we found that the activity of serine-centered protease was responsible for the different peptide profiles between normal and MI sera. With extended incubation time, adding PMSF to normal human sera resulted in a loss of most low molecular weight peptides from the MALDI-TOF spectra (Figure 11). Similarly, the addition of PMSF destroyed the pattern of the peptides found in both NHS and MI. Thus, the addition of PMSF ablated the differences in spectra between the control and disease state and essentially erased most of the spectral elements. From these data we found that serine centered proteases were responsible for the distinctive MALDI-TOF spectra of normal and MI sera.

As previously described,1,3 we found that a high-sensitivity, low mass accuracy form of MALDI-TOF4,40 could be used to rapidly generate serum peptide fingerprints that distinguish between disease states. In particular, we found that preparing sera by rapid preseparation over C18 reversed-phase resin prior to MALDI-TOF resulted in strong signals, excellent signal-tonoise ratio, reproducible spectra and sharp statistical resolving power. Our results, together with the previously published work, indicate that many diseases and specific variants may well be distinguishable by rapidly performed mass spectral assays that do not require disease-specific-reagents. The statistical analysis of the mass spectral patterns by a method that is quantitative, rigorous, and statistically powerful will be a key component of this type of analysis.35,36 Multivariate analysis is a powerful method for contrasting populations but lacks a quantitative element and thus might differentiate between groups of peaks that only show modest real differences. Hence, in this paper, we inserted a quantitative cutoff in signal intensity, not dissimilar in concept to decision tree analysis,8 and thus only analyzed raw data in which the media intensities in each 5D window were significant and differed by at least a factor of 2. Of course, by adjusting the stringency factor prior to multivariate analysis even greater levels of confidence might be obtained. In the data sets shown herein, where sets of peak intensities were used to contrast samples, very convincing probabilities were associated with each sample. Thus, we feel that a quantitative decision step that ensures the set of scalar values subjected to analysis are markedly different between treatments prior to multivariate analysis will ensure that these approaches are robust, reliable, and powerful. The observation that the patterns in sera or plasma depend on how the sample has been collected, stored and assayed leads to a practical consideration in the coming worldwide effort to characterize the proteome of human blood.41 We suggest that one of the most important standards set by the Human Proteome Organization (HUPO) should be the standardization of sample collection procedures. In terms of sera profiling for disease, we recommend that standards should be set for time and temperature at which blood is clotted, the conditions of centrifugation, the time sera remains unfrozen, and how it is aliquoted, frozen, thawed, and used. Without such standards, it is apparent that it will be impossible to meaningfully compare the results obtained in one laboratory with those of another. We recommend that sera be coagulated at room temperature for less than 2 h before clinical centrifugation for 20 min and that the sera be frozen at the clinical site. After shipping on dry ice, the sample may be thawed once for aliquoting at the laboratory site, re-frozen, and the aliquots subsequently used once and discarded. Of course, it matters little which reasonable sample standard is adopted, as long as one reasonable standard is adopted. With respect to the MALDI assay conditions, we suspect that given the sensitivity of the results to the instrument and surface employed, and given the large effect of laser power and amplifier sensitivity settings (cf. Figures 10 and 11), standard controls collected by the same protocol will have to be run alongside each disease sera for every assay (see Figure 1). We found that low molecular weight families of polypeptides can be used to distinguish between control and MI patients. If we envisage that each disease is associated with damage or death of specific cells or organs, then it is not unreasonable to assume that the disease will result in the differential release, Journal of Proteome Research • Vol. 2, No. 4, 2003 369

research articles secretion, or activation of different enzymes from the affected cells or perhaps in response to the damaged cells. If different modification activities or specificities are manifest with each disease and have different affinities for the major proteins in the blood, then it is not difficult to imagine that that each different disease might be associated with different processing or modifications of major blood proteins. The concentration of proteins released into the blood directly from the damaged cells, or the changes in potent regulatory factors associated with disease, are likely to be far too small to be directly detected by MALDI-TOF. Therefore, it is not reasonable to assume that the altered peptide spectra are a direct measure of disease proteins. Rather, the changes in the spectra seem to reflect the action of disease-associated enzymatic activity or specificity on major blood proteins. Hence, the data here indicate that differential reactions of major blood proteins by disease-associated enzyme activities is the most tenable explanation for the phenomena of disease specific MALDI-TOF spectra at least in the case of normal sera versus MI sera. The MS/MS spectra of the low molecular mass analytes found in blood of MI sera showed a significant correlation with the C3f fragment and the fibrinogen alpha peptide. The C3f fragment is produced by a proteolytic cleavage of C3, a major protein component of blood. The fibrinogen alpha peptide (FPA) results from the activation of fibrinogen by thrombin. The appearance of these patterns in the sera indicate the presence of functional proteases in blood that generated peptide fragments from the major serum proteins complement C3 and alpha fibrinogen. Hence, the main components of the control spectrum (fragment of HSA) and the MI spectrum (fragments of C3f and fibrinogen peptide A) appeared to be generated from common blood proteins by endoproteinases. Moreover, the cleavage sites of C3f and FPA were flanked by the presence of lysine or arginine residues indicating a trypsinlike mechanism of action. Previous reports have indicated that both complement C3 and fibrinogen were specifically released by highly regulated trypsin-like processing enzymes during complement activation26,27 and clot formation,42 respectively. Furthermore, both thrombotic clot formation and complement activation have been previously associated with myocardial infarction. Thus, on the basis of the data present here and elsewhere, we conclude that both C3 and fibrinogen were proteolytically activated during heart attack, releasing C3f and fibrinogen peptide A, respectively. We observed that both the C3f and alpha fibrinogen peptide showed the progressive loss of amino acids from the N terminus. The loss of amino acids from the N-terminal end of both peptides resulted in the production of families of truncated fragments. These two families of peptide fragments comprised the bulk of the low molecular mass peptide patterns observed in MI patients. The progressive loss of amino acids was consistent with the activity of an N-terminal exo-peptidase(s), i.e., aminopeptidase. We conclude that specific proteases generated the C3f and FPA parent peptides and that subsequently an aminopeptidase(s) apparently degraded them. The ladder of peptides showing the progressive loss of Nterminal amino acids alone is sufficient to conclude that the patterns in MI must result from the balance of protease activity generating the parent fragment and aminopeptidase activities degrading the full-length peptide in the sera. Hence, it appears that at least in the case of normal versus MI sera, MALDI-TOF peptide pattern diagnosis works by comparing the mass distribution of peptides and their associated N-terminal exo370

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Marshall et al.

proteolytic products. The measurement of these peptides forms the basis of the rapid and unambiguous mass spectral diagnosis for MI that requires no specialized reagents. Hence, the success of diagnosis by MALDI patterns may extend to those diseases that cause a significant change in balance of concentration or activity of enzymes that modify common proteins, or their fragments, in the blood. We examined the inference that both protease and amino peptidase activities form the diagnostic pattern in control versus MI sera in more detail using time course and inhibitor studies. Because the distinctive pattern of normal plasma was not present in plasma immediately after collection but was generated with time, we could infer the activity of proteases that generated the fragment patterns in sera in vitro after collection of the blood. Experiments in sera, demonstrating that the effect of PMSF was dependent on both concentration and time, support the view that serine-centered proteases were responsible for the diagnostic peptide patterns. The concentration required to prevent the pattern, g 2 mM, closely matches the concentration of PMSF commonly used to prevent proteolysis. If the effect of PMSF was derived from some chemical interference with the MALDI process, then we might expect that it should have shown an inhibitory effect in the submillimolar range and also should have shown its effect immediately upon addition rather than requiring several hours to ablate the profile. Hence, from the appearance of peptides after collection of the plasma, and from the effect of PMSF on sera with time, we conclude that part of the distinctive patterns generated in normal human sera and MI sera result from the activity of serine centered proteases ex vivo. From the observation that the peptide pattern in serum is relatively stable for 1 or 2 h on the bench, we infer that peptides were being constitutively generated in sera samples at roughly a steady state with respect to their degradation. Because adding PMSF initially inhibited the formation of the high mass peptides coupled to the accumulation of low mass peptides, and eventually resulted in the erasure of the pattern of peptides, we might conclude that this is evidence that aminopeptidase(s) were constantly degrading peptides in the blood. The eventual loss of the distinctive family of peptides upon addition of PMSF indicates that aminopeptidases remain functional in sera and plasma and are constantly degrading the peptides that form the diagnostic pattern. Thus, the distinctive patterns of