Abstract
Simultaneous assessment of a panel of protein markers is becoming essential in order to enhance biomarker research and improve diagnostics. Specifically, postmortem diagnostics of early myocardial ischemia in sudden cardiac death cases could benefit from a multiplex marker assessment in the same tissue section. Current analytical antibody-based techniques (immunohistochemistry and immunofluorescence) limit multiplex analysis usually to not more than three antibodies. In this study, mass spectrometry-immunohistochemistry (MS-IHC) was performed by combining laser ablation inductively coupled plasma mass spectrometry (LA-ICP-MS) with rare-metal-isotope-tagged antibodies as a technique for multiplex analysis of human postmortem myocardial tissue samples. Tissue sections with myocardial infarction were simultaneously analyzed for seven primary, rare-metal-isotope-tagged antibodies (troponin T, myoglobin, fibronectin, C5b-9, unphosphorylated connexin 43, VEGF-B, and JunB). Comparison between the MS-IHC approach and chromogenic IHC showed similar patterns in ionic and optical images. In addition, absolute quantification was performed by MS-IHC, providing a proportional relationship between the signal intensity and the local marker concentration in tissue sections. These data demonstrated that LA-ICP-MS combined with rare-metal-isotope-tagged antibodies is an efficient strategy for simultaneous testing of multiple markers and allows not only visualization of molecules within the tissue but also quantification of the signal. Such imaging approach has a great potential in both diagnostics and pathology-related research.
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Diagnostics of several pathological conditions would benefit from concurrent assessment of a panel of markers but this requires development of analytical techniques capable of detecting several biomarkers simultaneously (multiplexing), at good spatial resolution, and with high sensitivity. In particular, a panel of markers (instead of just one single marker) has been recently proposed for pathological diagnostics of early myocardial ischemia (EMI) [1, 2]. This acute condition represents the most frequent cause of sudden cardiac death. EMI occurs during the initial 4 to 6 h after occlusion of coronary flow to myocardium and, in cases where it is not suddenly fatal, EMI can lead to the development of myocardial infarction (MI) [1, 2]. Because EMI lacks gross anatomical changes and specific tissue morphology at histological analysis, much effort was made over the past several decades to improve recognition of EMI pathology by identifying pathological pathways and developing new diagnostic tools (molecular targets, strategies, methodologies, and instrumentation) [1, 3]. Currently, efforts are being made to develop multiplex approaches in order to both accelerate the discovery process and integrate multiplexing into routine work for improving diagnostics.
Despite progress in this field, the prevalent methods for tissue pathology diagnosis still lack high-throughput capabilities and allow only semi-quantitative analysis (e.g., immunoassays, immunohistochemistry (IHC), immunofluorescent microscopy (IFM), Western blotting, and antibody-based in situ hybridization). The most frequent and feasible color combination with IHC or IFM is three markers on a single-tissue section [4]. Aspects that impede concurrent screening of more molecules on a single-tissue section include spectral and spatial overlap of reporters, cross-reactivity between the detection reagents (in cases where indirect detection methods are used), and tissue autofluorescence (in cases of fluorescently labeled antibodies) [4]. In addition, quantification of the signal remains inaccurate due to non-linear characteristics of signal amplification. Furthermore, quantification of chromogenic IHC is performed by analyzing pixel intensities of digital scans of slides instead of measuring the reporter on the antibody [5].
Mass spectrometry IHC (MS-IHC) is an emerging approach with the potential for multiplex analysis of markers directly on tissue section [6]. This technique utilizes an innovative antibody tagging method that was originally developed for extensive multiplex analysis of single cells in mass cytometry [7,8,9,10]. Briefly, the primary antibody is tagged with a combination of rare-earth-metal isotopes and specific metal-chelating polymers instead of enzymatic or fluorescent probes. After incubation with primary antibodies, the entire surface of tissue section is rastered either by laser or ion beam in a coordinated way, using a grid array at a fixed lateral resolution. At each coordinate, the generated ions are analyzed by MS to generate a data set, which is used for reconstruction of ion images (similar to other imaging mass spectrometry technologies, e.g., matrix assisted laser desorption/ionization) [6, 11, 12]. Recently, this method was successfully applied to simultaneously assess 10 and 32 makers in breast cancer tissues by secondary ion mass spectrometry (SIMS) and laser ablation inductively coupled plasma mass spectrometry (LA-ICP-MS), respectively [13, 14].
In this study, MS-IHC was evaluated as a multiplex method to quantitatively analyze human postmortem formalin-fixed, paraffin embedded (FFPE) samples by LA-ICP-MS for seven markers: troponin T, myoglobin, fibronectin, C5b-9, unphosphorylated connexin 43 (Cx43), JunB, and vascular endothelial growth factor-B (VEGF-B).
Materials and methods
Autopsy specimens
Cardiac samples were collected from six autopsy cases, performed at the University Center of Legal Medicine in Geneva, Switzerland, between December 2010 and November 2014. In all cases (n = 6; 5 males, 1 female; mean age 61.7 years), the cause of death was acute MI, defined by the presence of polymorphonuclear leucocyte infiltration (associated or not with hemorrhagic infiltrates and eventually contraction band necrosis) and cardiomyocyte coagulation necrosis, in sections stained with hematoxylin and eosin (H&E). In order to ensure the presence of ischemic myocardium, samples with evident MI were intentionally selected for this study. In accordance with our standard sampling protocol, eight cardiac regions were evaluated in every case (anterior, lateral, and posterior wall of both ventricles, anterior and posterior septum) but only one region representative of each case was used for further investigation in this study: the region with the most severely infarcted area, as observed by histological examination. In total, one tissue block from each case was examined in this study (the total number of sections per case is illustrated in Supplementary Fig. 1). Tissue samples were fixed in 4% buffered formaldehyde for 24 h, embedded in paraffin, and cut in 5-μm thick sections. The postmortem interval (time from death to autopsy) ranged from 5 to 36 h.
Immunohistochemistry
Chromogenic IHC on serial sections for troponin T, myoglobin, fibronectin, and C5b-9 were used for comparison to MS-IHC by LA-ICP-MS, as “positive controls.” Although chromogenic IHC and MS-IHC are different techniques, the overall pattern for markers’ distribution (accumulation or depletion) was expected to be approximately similar because the same primary antibodies were used in both techniques and evaluated on consecutive sections. In addition, three experimental markers were added to the multiplex panel, namely, Cx43, VEGF-B, and JunB. FFPE tissue sections were deparaffinized and treated for epitope retrieval by either incubation with proteinase K (Sigma-Aldrich®, 0.1 mg/ml in 50 mM Tris-Buffered Saline) for C5b-9 and fibronectin or microwaving for 15 min at 95 °C in Dako Target Retrieval Solution for the other antibodies. Following epitope retrieval, the sections were treated with 1% H2O2 in 10% methanol, blocked with bovine serum albumin, and subsequently probed with primary and secondary antibodies in a humidified chamber. Primary antibodies were against troponin T (mouse monoclonal, Abcam®, 1:250; n = 5), myoglobin (Bond™ mouse monoclonal, Leica, 1:50; n = 6), fibronectin (rabbit polyclonal, Dako, 1:2000; n = 6), C5b-9 (mouse monoclonal, Quidel®, 1:2000; n = 6), Cx43 (mouse monoclonal, Invitrogen™, 1:500; n = 4), JunB (rabbit polyclonal, Abcam®, 1:200; n = 3), VEGF-B (mouse monoclonal, R&D System®, 1:500; n = 2). Secondary antibodies were biotinylated anti-mouse (Vector Laboratories) or anti-rabbit (Vector Laboratories) IgG, followed by incubation with either VECTASTAIN® ABC Complex HRP kit (Vector Laboratories) for JunB or streptavidin/horseradish peroxidase-conjugate (Dako) for the rest. Colorimetric detection was performed using either Vector® DAB (Vector Laboratories) or Vector® AEC (Vector Laboratories) kits, according to the manufacturer’s instructions, with hematoxylin as counter-staining. For chromogenic IHC, negative controls without primary antibody were tested for all antibodies; moreover, negative controls were run in every IHC series and the slides were evaluated only if the negative controls showed negative results.
Tissue and antibody preparation for MS-IHC
The overall workflow for the entire procedure consisted of three major stages: sample preparation, data acquisition, and data analysis (Fig. 1). The protocol for sample preparation and tissue labeling was similar to the process used in chromogenic IHC and IFM but instead of conjugating the antibody with enzyme or fluorophore, the primary antibody was coupled to a polymer tagged with rare-metal isotope. Sections (5 μm) from human autopsy FFPE samples with infarcted myocardium were deparaffinized, treated for epitope retrieval using microwave (10 min at 95 °C in Dako target retrieval solution), pre-treated with 1% H2O2 in 10% methanol, and blocked with bovine serum albumin. The sections were then incubated for 90 min with a 200-μl mixture (per slide) of seven antibodies that were pre-labeled with a complex containing MAXPAR® X8 Polymer and a rare-metal isotope (MAXPAR® Antibody Labeling Kit, Fluidigm®): C5b-9 tagged with 139La (0.5 μg/ml; n = 6), fibronectin tagged with 141Pr (2.5 μg/ml; n = 6), myoglobin tagged with 144Nd (15.0 μg/ml; n = 6), troponin T tagged with 151Eu (4.0 μg/ml; n = 5), JunB tagged with 159Tb (20.0 μg/ml; n = 5), Cx43 tagged with 175Lu (1.0 μg/ml; n = 5), and VEGF-B tagged with 162Dy (1.0 μg/ml; n = 5). After incubation with the mixture of antibodies, the sections were rinsed in Dako Wash Buffer (Dako) and dried at room temperature prior to MS analysis.
MS-IHC data acquisition
Tissue pre-incubated with rare-metal-isotope-tagged antibodies was placed into the laser ablation chamber and was ablated by a Nd:YAG/213-nm laser focused on 8 or 40 μm diameter spot using laser ablation system (NWR-213, New Wave, Fremont, USA) coupled to quadrupole mass analyzer (Agilent 7700 ICP series, Darmstadt, Germany). The generated ablated particles were transported to the ICP ion source by a helium carrier gas of 800 mL/min and exposed to plasma torch. Only the metal tags were able to withstand this step and were subsequently passed to mass spectrometer for detection and quantification. The LA-ICP-MS parameters were optimized to provide the best signal-to-noise ratio while keeping the maximum reproducibility between analyses. In this way, the energy output was set at 23% corresponding to a laser fluency of 0.35 J/cm2. The lateral resolution was fixed at 10 or 50 μm in the raster mode with a scan speed of 10 or 50 μm/s, respectively. The laser repetition frequency was set at 20 Hz. Rare-earth metals (139La, 141Pr, 144Nd, 151Eu, 159Tb, 175Lu, and 162Dy) were monitored for a duty cycle of 1 s.
Data analysis and image visualization
The acquired raw data were extracted using the MassHunter software (Agilent, Darmstadt, Germany). Data files (.d) of IMS experiment were successively converted to mzML and imzML formats using msconvert and imzMLConverter tools, respectively. Ion images were reconstructed and visualized using either the MSIReader v0.06 software or MALDIQuant and Cardinal packages in R environment (http://cran.r-project.org) [15, 16].
Calibration procedure
The concentration ranges for each rare-metal-isotope reporter were calculated using corresponding calibration curves, which were generated using laboratory standards. Briefly, synthetic laboratory standards were prepared from human heart homogenates of analogous control autopsy cases doped with rare-metal isotope at four different concentrations (50, 500, 1000, and 5000 ng/g; Supplementary Table S1 lists these concentrations in nmol/g) as described elsewhere [17, 18]. For each rare-metal isotope, the 80 μm × 100 μm rectangles from the spiked areas were analyzed, i.e., 80 pixels at each concentration, and average intensities of those 80 pixels were calculated for each concentration. Then the average pixel intensity (u.a.) was plotted against the concentration of a metal isotope to generate a calibration curve. The calibration curves were then used to convert the intensity scales recorded by LA-ICP-MS to the concentrations of rare-earth metals, which is directly proportional to the amounts of markers.
Results
Multiplex tissue imaging of MI in human postmortem samples with MS-IHC
Chromogenic IHC results showed cytoplasmic depletion of troponin T and myoglobin from large groups of cardiomyocytes in the infarcted areas and accumulation of fibronectin, C5b-9, Cx43, and JunB (Fig. 2). Fibronectin and C5b-9 accumulation was observed in cytoplasm of cardiomyocytes located in the infarcted area. Increased Cx43 signal localized at gap junctions and in some cardiomyocytes also in cytoplasm. JunB positive reactions were found in nuclei of cardiomyocytes and infiltrating leucocytes. Evaluation of IHC with microscope at high magnification showed some VEGF-B positive reactions only in endothelial cells of few vessels (Supplementary Fig. 2). After analysis of the samples by MS-IHC and data acquisition, image reconstruction was performed for each rare-metal-isotope (Fig. 2, Supplementary Fig. 2). Reconstructed ion images obtained with MS-IHC showed similar distribution patterns as the consecutive sections stained with chromogenic IHC (Fig. 2). Concerning VEGF-B–162Dy, some variations in signal were also observed in reconstructed ion images but due to the expression of this marker in endothelial cells of blood vessels, the accurate interpretation of the LA-ICP-MS data would require analysis at a higher resolution than was selected in this study.
This approach for multiplex tissue imaging allows reconstruction of composite images. Figure 3 shows two composite reconstructions: (1) troponin T–151Eu and fibronectin–141Pr, and (2) troponin T–151Eu and C5b-9–139La. Increased fibronectin–141Pr and C5b-9–139La levels were evident in the areas with decreased troponin T–151Eu.
Due to its sensitivity, the multiplex MS-IHC allowed in some cases more precise determination of areas with marker’s accumulation or depletion. For example, evaluation of one of the cases for fibronectin by chromogenic IHC showed accumulation of fibronectin (positive staining) in the entire region. However, reconstruction of ion image for fibronectin–141Pr showed obvious distinction between areas with and without signal (Fig. 4). This difference between the two methods and strong signal from chromogenic IHC could possibly be explained by signal amplification in chromogenic IHC during both the incubation with secondary antibody and the exposure to substrate for development of colored precipitate.
Sensitive method that permits accurate marker quantification
Quantification was performed for selected cases (representative case is shown in Fig. 4). Since the metal isotopes are measured by mass spectrometer and the isotopes are conjugated to the primary antibody, quantification is fairly straightforward. The signal intensity is proportional to the local marker concentration in the tissue section (in contrast to IHC or IFM, where the quantified signal is often amplified by incubations with additional antibodies needed for the detection and visualization). Using calibration curves for each rare-metal isotope, the intensity color scale was converted to concentration scale (Fig. 4, Supplementary Fig. 3). Utilizing the concentration scale already provides a more objective way for comparison. For instance, visual examination of ionic reconstruction for C5b-9–139La and fibronectin–141Pr (Fig. 4) suggests similar distribution of these markers in the selected tissue area. Despite similar distribution, the concentration of C5b-9–139La was much higher (nearly doubled) in comparison to fibronectin–141Pr.
Discussion
Majority of postmortem studies are in agreement that no single marker would be both sensitive and specific enough to precisely detect EMI, and, therefore a panel of markers should be used for accurate diagnostics. But chromogenic IHC (the most widely used tool to evaluate markers in postmortem samples) limits the number of antibodies that can be simultaneously tested on the same tissue sections. Availability of techniques capable of multiplex tissue imaging would be an advantage for evaluating a panel of markers. The main novelty of this study is the evaluation of MS-IHC with LA-ICP-MS as a technique to simultaneously visualize and quantify seven ischemic markers in the same tissue section from human postmortem cardiac tissue with evident MI. Cases with evident MI were intentionally selected in order to ensure the presence of ischemic myocardium. The only two previous MS-IHC studies assessed markers in breast cancer and did not investigate the absolute quantification capability of the approach [13, 14]. Primary antibodies tagged directly with the innovative reporters (rare-earth-metal isotopes combined with metal-chelating polymer) have the potential to greatly surpass multiplex options available with IHC and IFM and to improve multiplex tissue imaging in the same tissue cross section to a new high-throughput level.
The selected panel of seven markers consisted of four established postmortem markers (C5b-9, fibronectin, troponin T, and myoglobin, where troponin T and myoglobin are also currently used as serum markers for the clinical diagnosis of MI), and three experimental markers (Cx43, JunB, and VEGF-B). Our results for the established four markers (C5b-9, fibronectin, troponin T, and myoglobin) were consistent with previously published studies: C5b-9 and fibronectin accumulated in MI tissue and troponin T and myoglobin were depleted [1, 19,20,21,22,23,24,25,26]. Cx43, JunB, and VEGF-B are markers that were recently shown in experimental research to be influenced by ischemia, already during its onset [2, 27,28,29,30,31]. Connexin43 is gap junctional protein. Cardiac gap junction channels are located at the intercalated disks and are responsible for intercellular exchange of ions and small regulatory molecules. EMI was shown to induce Cx43 and to lead to its accumulation at the intercalated disks as early as 15 min after ischemia onset [2]. Our results concerning the changes of Cx43 in MI are consistent with the only one other study that also evaluated protein level of Cx43 in human postmortem MI samples [26]. The function of JunB during EMI is not yet well understood but it was shown to be induced by EMI [2, 32]. VEGF-B is one of the five secreted glycoproteins in the VEGF family. This released growth factor appears to play a role in the growth of coronary arteries, enlargement of capillaries, and cardiac hypertrophy [29]. Overall, previous studies performed on human postmortem MI samples investigated various combinations of these markers. But only a maximum of four markers were investigated in two separate studies and not in the same section but using consecutive sections [1, 21]. All other postmortem MI investigations evaluated two or three markers at a time in a given study.
Identifying various potential ischemic markers is currently needed in order to improve knowledge about this acute pathology and select a panel of targets that could be used for diagnosis and chronological dating of EMI [33]. Although we investigated only six cases, our results demonstrate that MS-IHC is suitable for performing multiplex tissue imaging in a larger study. Future application of MS-IHC offers a great potential to accelerate research utilizing human postmortem EMI samples. The ultimate goal is to implement this methodology for development of a diagnostic panel of markers and potentially use it as a tool to detect EMI. While seven markers were evaluated in this study, the method allows for a more high-throughput analysis: not only a panel of 32 tags was already successfully evaluated using similar approach in the context of tumor biology but also nearly 100 rare-earth-metal isotopes might be available in the future [14]. Several aspects of this multiplex approach are currently being developed, including the number of available isotopes and metal-chelating chemistries [14]. Innovations in these areas are likely to further improve the multiplexing ability and accuracy of this method. But the persisting challenge for any techniques using rare-earth-metal-tagged antibodies will remain to be the availability of specific primary antibody for a given target.
In imaging MS, the selected criteria are often a compromise between resolution and the analysis time: higher resolution can be achieved but with longer duration for data acquisition [12]. In this study, resolution at cellular level was chosen (either 10 or 50 μm) to evaluate broader area within reasonable amount of time. Assessment of a larger tissue area is more relevant in EMI and in several other forensic investigations. But higher resolution can be obtained with this method. Using similar approach, resolution at 1 μm was recently reported but assessment of 0.5 mm × 0.5 mm area took about 3.5 h [14]. In the near future, innovations in designs of laser ablation chamber and laser properties will improve the efficiency and allow more rapid scanning [34].
In addition to high-throughput multiplexing, other advantages of this technique include single incubation step for labeling with multiple antibodies, elimination of labeling with secondary antibody without losing sensitivity, and improved quantification of the signal. Importantly, this method is highly sensitive and has a wide dynamic range, which allows absolute and precise quantification of the markers [35]. In comparison to MS-IHC, other available multiplex methods employ lengthy and laborious staining techniques with less precise quantification. Quantitative analysis of tissue samples by LA-ICP-MS has been successfully demonstrated showing powerful quantification capabilities [36, 37]. Improved marker quantification within the exact same section is particularly powerful in research context because it allows more precise statistical analysis between study cases and controls, more accurate evaluation of affected area, and establishing cutoff values for marker’s concentration. Since the initiation of this study, several additional markers have been proposed for EMI (e.g., GAL1, GAL3, HIF-1α, MIF, MCP-1) [33, 38,39,40,41]. The challenge for selecting the most useful panel of diagnostic markers is comparison of specificity and sensitivity among all of them. In this case, accurate quantification will be useful for performing appropriate statistical tests to determine the optimal combination of markers and to validate their usefulness. Furthermore, quantification based on external calibration makes it possible to establish a threshold value, similarly to other standard laboratory tests that utilize calibration. In forensic and clinical pathology, implementation of threshold values for ischemic markers in routine work would allow a more accurate comparison of data from different samples and a precise diagnosis of this acute pathology, which otherwise remains undiagnosed, misdiagnosed, or, in the best scenario, only hypothesized. Moreover, quantification of the markers could give information about the severity of the ischemic insult (infarction size), duration of ischemia prior to death, and the time of death. These data are undoubtedly crucial for researchers, clinicians, and pathologists. Besides EMI, accurate marker quantification can be applied to a variety of pathological conditions in order to improve their diagnosis and to obtain information about their time of appearance, evolution, vitality, and contribution to death. Wound vitality and wound age estimation are an example of the possible applications. Lastly, quantitative multiplex tissue imaging allows more efficient and accurate way to study changes in markers’ level over time. Temporal study can be performed in a relatively short amount of time: several targets can be analyzed within one-day procedure (a process that would take several days to test with chromogenic IHC). At the same time, accurate quantification is dependent on reliable calibrations curves. Prior to incorporating this approach for routine work in forensic medicine, the method needs to be validated according to the international guidelines.
In summary, the method presented in this investigation offers the advantage of simultaneously multiplexing and quantifying markers in the same tissue section, in human postmortem cases of MI. Current technologies for biomarker discovery that utilize untargeted strategies are rapidly generating candidate markers that can potentially improve diagnostics. MS-IHC has a great potential for accelerating translational research by simultaneously validating multiple markers of interest and also for improving clinical and forensic diagnostic of pathologies that require a multiplex evaluation of markers.
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Acknowledgements
We would like to thank Max Villa and Catia Pomponio for the support and assistance with LA-ICP-MS and immunohistochemistry, respectively.
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For this type of study, formal consent is not required. All cases included in this study were obtained from the autopsy database in our center. In agreement with the local ethics committee and the local general prosecutor, these cases can be included in this type of studies, provided that they are anonymized. In this investigation, no information allowing the identification of a person is given. People, who had previously refused, in a written form, their consent to bequeath their body parts for research use, were excluded from the study.
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Aljakna, A., Lauer, E., Lenglet, S. et al. Multiplex quantitative imaging of human myocardial infarction by mass spectrometry-immunohistochemistry. Int J Legal Med 132, 1675–1684 (2018). https://doi.org/10.1007/s00414-018-1813-9
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DOI: https://doi.org/10.1007/s00414-018-1813-9