MALDI TOF imaging mass spectrometry in clinical pathology: A valuable tool for cancer diagnostics (Review)

  • Authors:
    • Jörg Kriegsmann
    • Mark Kriegsmann
    • Rita Casadonte
  • View Affiliations

  • Published online on: December 4, 2014     https://doi.org/10.3892/ijo.2014.2788
  • Pages: 893-906
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Abstract

Matrix-assisted laser desorption/ionization (MALDI) time-of-flight (TOF) imaging mass spectrometry (IMS) is an evolving technique in cancer diagnostics and combines the advantages of mass spectrometry (proteomics), detection of numerous molecules, and spatial resolution in histological tissue sections and cytological preparations. This method allows the detection of proteins, peptides, lipids, carbohydrates or glycoconjugates and small molecules.Formalin-fixed paraffin-embedded tissue can also be investigated by IMS, thus, this method seems to be an ideal tool for cancer diagnostics and biomarker discovery. It may add information to the identification of tumor margins and tumor heterogeneity. The technique allows tumor typing, especially identification of the tumor of origin in metastatic tissue, as well as grading and may provide prognostic information. IMS is a valuable method for the identification of biomarkers and can complement histology, immunohistology and molecular pathology in various fields of histopathological diagnostics, especially with regard to identification and grading of tumors.

1. Introduction

Matrix-assisted laser desorption/ionization (MALDI) time-of-flight (TOF) techniques are versatile analytical tools used in various areas of medical diagnostics and basic research. Mass spectrometry (MS) has been successfully applied to study microbiological colonies (13), plants (4), insects (5), vertebrates including whole animals (68), human cells (9,10) and tissues (11,12).

This method allows the analysis of proteins (13,14), peptides (15,16), lipids or phospholipids (6,1719), carbohydrates or glycoconjugates (20) and exogenous or endogenous small molecules, especially molecules involved in drug metabolism (2127).

MALDI imaging mass spectrometry (IMS), first described by Caprioli et al (28), links molecular evaluation of numerous analytes and the high sensitivity and selectivity of mass spectrometry with morphological information about spatial distribution of molecules in cells or tissues (29) and thereby provides unbiased visualization of the arrangement of biomolecules in tissue (30).

Since cancer tissue contains all information on proteomic and genetic changes, it represents the best possible sample material for any molecular research (29). Thus, pathology is not only a large field of medical research but also a basis for the diagnosis of various diseases with direct impact on clinical treatment decisions. The information contained in tissues cannot be replaced by investigation of serum or blood (29).

MALDI IMS has been applied to various organ systems and diseases such as cardiovascular- (31), neurologic- (32), or joint disorders (11,33), amyloidosis (34) inflammatory bowel diseases (35), renal diseases (3638), the field of reproductive medicine (39) and various tumor entities (13,15,4045). The following review will focus on MALDI IMS in human tumor tissues as well as applications that have a potential in pathology (22).

2. Technical considerations

Despite some technical limitations, mainly in the area of detection limits and instrument sensitivity at high spatial resolution, this method has the potential to improve cancer diagnostics (42). There are several reviews addressing the complete process of MALDI IMS, in particular regarding experimental considerations: sample collection, sample preparation, matrix deposition, ionization process, instrumentation and data processing (22,30,31,4654).

IMS experiments can generally be performed in two related modes, imaging (57) and profiling (58). Whereas imaging allows correlation with histology, profiling is generally used when tissues are completely homogeneous and, therefore, different compartments do not have to be considered.

Concerning sample collection and sample preparation, workflow solutions have to be exactly defined beginning from the handling of various tissues in the operation theatre, followed by dehydration and paraffin-embedding process as well as deposition of sections onto conductive slides.

Sample handling and preparation are critical to achieve good spectral quality and reproducibility. In the past few years, several groups have worked on strategies to improve the detection of peptides and proteins (55,56); however, optimization and standardization in clinical application to minimize variability of results are still needed.

IMS requires minimal sample preparation for analysis (59). In the past years, there has been a significant improvement in image spatial resolution that is in the range of 20–50 μm and can be improved to up to 5 μm with special techniques (60,61).

Data processing and statistical analysis are of tremendous importance for accurate and reliable results. In the processing step MALDI datasets are typically subjected to smoothing, baseline correction and calibration. Normalization is generally the next step intended to minimize the experimental variation arising from day-to-day instrument fluctuations, or artifacts related to sample preparation (62). Statistical analysis is then performed in order to elucidate spectral features that are consistently associated within a cohort for biomarker discovery or for disease classification. Most statistical methods can be performed using a supervised method requiring at least two groups of spectral data that need to be discriminated or an unsupervised analysis applied without any prior knowledge of the samples to generate a classification model. Principal component analysis (PCA) is a well known method used to describe the variability in the dataset in a reduced number of dimensions (63). The software for data analysis, such as ClinProTools and SCiLS Lab (Bruker Daltonik), MassLynx (Waters) and BioWorks (Thermo Fisher Scientific) is usually commercially available and provided by the manufacturer of the MALDI instruments. In addition, BioMap software (Novartis, Basel, Switzerland) is freely available for calculating basic statistics of the full dataset. Despite the different data analysis approaches that have been developed, there is a need for more advanced biostatistical software in order to be able to handle huge data files (5,000–50,000 spectra).

A new and emerging application is the three-dimensional illustration of organ structures. It has been shown that MALDI IMS can be combined with other imaging modalities such as positron emission tomography (PET) and magnetic resonance imaging (MRI), improving the interpretation of the proteomic data and providing 3D visualization of proteins that may not be apparent with other imaging methods (64,65).

Another promising development represents MS for single cell analysis to determine protein and peptide contents in cells (47).

Combination of MALDI IMS with cytological preparations of oral brush biopsies has been shown by Remmerbach et al (9). These authors could discern non-malignant from malignant cells by MS. Furthermore, IMS could be applied as a specific diagnostic tool for routine cervical cytology specimen (10). Thus, IMS as a relatively new technique is still at an early stage, and technical advances concerning sample preparation and instrumentation will certainly improve specificity and sensitivity and enlarge the potential for further applications.

3. MALDI IMS as an adjunct to immunohistochemistry

Contrary to antibody-based methods, target structures do not need to be known when MALDI IMS is applied (52) which makes it a valuable discovery tool, since broad range of proteins may be surveyed simultaneously (67).

Furthermore, MS techniques may have a higher reproducibility between laboratories than immunohistochemistry because human bias is abolished (68).

However, MALDI IMS cannot only be an adjunct tool to immunohistochemistry but also to histochemistry. For examle, it has been shown that the Berlin-blue reaction for the detection of hemosiderin can be replaced by MALDI IMS of ferritin chains (33). Likewise, mucous substances detected by histochemical reactions could be identified applying MS (69) as well as soft tissue constituents (7072).

4. Frozen vs. formalin-fixed paraffin-embedded tissue samples and analysis of tissue microarrays

The investigation of frozen tissues by MALDI IMS requires immediate freezing, storage at −80°C and rapid cutting (48) enabling the study of proteins, drugs or their metabolites and lipids. Formalin-fixed paraffin-embedded (FFPE) tissues have to be digested and, therefore, allow analysis of peptides only (Fig. 1). Although frozen samples are easier to be analyzed and imaged as they do not require multiple steps for sample preparation (deparaffination and antigen retrieval), handling and storage of frozen specimens has disadvantages, since proteins are degraded during repeated freeze-thaw cycles and there is a need for expensive freezers.

Despite the difficulties in sample handling, numerous reports have described the application of MALDI IMS on whole sections (12,13,43,44,57,7378) and even on small biopsy samples of fresh frozen tissue (79).

Millions of FFPE tissues of various diseases including numerous cancer tissues are available in the archives of institutes of pathology. These samples are well documented and include information on patient treatments, treatment response, disease progression and other relevant clinical data (51).

One of the advantages of using fixed specimens is that FFPE tissues are well suited for tissue microarray (TMA) construction, where multiple FFPE core biopsies can be assembled in a single paraffin block. The direct analysis of FFPE TMA using MALDI IMS allows the analysis of multiple tissue samples in a single experiment (67,80). This high-throughput method was used to investigate gastric (16), pancreatic (81), non-small cell lung (67), prostate (82), renal cancer (15) and to discriminate pancreatic from breast cancer tissues (83). The correlation of MALDI IMS data with histology can be performed by two methods: either by staining a serial section with hematoxylin and eosin (H&E) (67) or by staining the tissue after the MALDI experiment, since the tissue is not destroyed during the laser ionization process (47).

5. Identification of peptides and proteins

There are many techniques used in the study of proteins, such as western blot analysis, liquid chromatography and reverse phase protein arrays (8487).

The most common approach to identify proteins using MS technique is the bottom-up approach achieved through protein separation/isolation, proteolytic digestion, sequencing of peptides by LC-MS/MS, and matching the peptides to genome-based protein databases (8890). Another approach is top-down, where proteins of interest are isolated from a complex protein mixture and directly fragmented in the mass spectrometer without previous digestion of proteins. This approach provides direct measurement of the molecular masses of the intact proteins (91,92). An alternative method for protein identification is on-tissue digestion, where tissue samples are in situ digested so that proteins of interest can be isolated and directly fragmented from the tissue section using MALDI MS/MS. This method offers the advantage to identify proteins from a tissue section without separation or homogenization, while preserving the spatial integrity of the tissue sample (30,67). However, protein identification directly from tissue is not always straightforward due to sample complexity and limited sample per unit area, unless peptides are present at high abundance in the sample. Recently, an imageID approach has been developed where consecutive tissue sections are processed in parallel to provide both, protein identification by LC-MS/MS and spatial information by MALDI IMS simultaneously (83) (Fig. 2). New public databases for the identification of proteins such as MSiMass list (93) and MaTisse (94) have been created enabling users to search either for proteins or for m/z values and assign identities to the peaks observed in their experiments. Such databases will improve implementation of MSI in the histopathological and clinical setting.

6. Tumor heterogeneity

The biology of a tumor depends not only on tumor cells but also on the interaction with stroma, blood vessels and the immune system (e.g. tumor-associated macrophages and lymphocytes). Homogenization of the tissue sample would lead to loss of information (29). Moreover, when considering personalized medicine, demonstration of tumor heterogeneity (Fig. 3) will be one of the most challenging issues in the future and MALDI IMS seems to be the ideal tool to solve this problem (29,40,95). As an alternative to MALDI IMS in complete tissue sections, captured cells can be mounted directly onto a MALDI target following microdissection thereby maintaining the spatial conformation for IMS (72). DNA- and RNA-based molecular methods have limitations to show tumor heterogeneity since spatial integrity is destroyed during the preparation process of the nucleic acids.

The potential application of MALDI IMS in a clinical workflow has been suggested by Caprioli (96) who stated in 2005 that this method may aid in diagnosis, prognosis and therapy of cancer bringing a new dimension of molecular information into pathological assessment of tissue specimen.

Today, nearly 10 years later, MALDI IMS is considered a powerful technique to evaluate tumor margins, and to acquire information on tumor typing, grading, prognosis and prediction.

7. Tumor margins

MALDI IMS is an objective method to demonstrate molecular tumor margins (resection borders). This was first proposed by Chaurand et al (97). Evidence has shown that adjacent tissue that appears histologically normal may already be molecularly compromised. For example, it has been shown in tumors of the ovary that MALDI analysis could detect two interface-specific proteins, plastin 2 and peroxiredoxin 1 as differentially expressed in the interface zones between tumors and normal tissues, suggesting these proteins as predictive markers for the presence of residual disease (98). Another study on tumor margins was conducted on kidney samples by Oppenheimer et al (44). These authors demonstrated that cells without phenotypic characteristics of tumor cells, have malignant molecular features. Specifically, mass spectral profiles were compared among four different regions of tissue consisting of tumor, margin-tumor, margin-normal and normal. Two statistical methods, the significance analysis of microarrays (SAM) and permutation t-test, were used in this work demonstrating the presence of patterns resembling tumor in the margin-normal microenvironment outside of the histological tumor border. For example, proteins involved in the mitochondrial electron transport system were consistently underexpressed in the tumor as well as in the histologically normal tissue adjacent to the tumor. Another application of MALDI MS dealing with surgical tumor margins has been shown on liver tissue (99). These investigators detected molecular signatures as classifiers of non-tumor and tumor regions that could be applied to the interface between normal liver tissue and hepatocellular carcinoma.

Thus, a potential advantage of IMS for the evaluation of tumor margins is the ability to identify molecular changes that are not detectable by histopathological evaluation alone (47).

8. Tumor typing

Numerous antibodies are often required for the correct diagnosis of a tumor. In the future, pathologists will be confronted more frequently with small biopsies since minimally invasive methods have been emerged in the past. Hence, effective and tissue sparing molecular techniques are important for correct classification of tumors. Despite the introduction of multi-antibody stains in immunohistochemistry, numerous tissue sections are often required for tumor typing. Since only one tissue section is needed when MALDI IMS is applied, this technique is perfect for the evaluation of very small tissue samples, and the remaining tissue is available for further molecular classification such as mutation screening (e.g. in lung tumors).

The combination of MALDI IMS for tumor classification with typing, grading and subsequent application of MALDI TOF techniques for mutation screening would be a very fast, sensitive and cost efficient workflow able to reduce human bias.

Published results indicate that MALDI IMS has the potential to develop into a valuable diagnostic technique that can complement established histological and histochemical as well as immunohistochemical methods. Biomarkers or signal classifiers can be robustly reproduced in different biomedical centers (73).

MALDI IMS for tumor typing has been demonstrated on frozen (13) as well as on FFPE tissue (16,67). It has been shown that classification of 6 common tumor entities was possible using frozen tissue sections (13). Furthermore, squamous carcinoma and adenocarcinoma of the lung (67), papillary and clear cell renal cancer (15) and gastric carcinoma (16) have been subclassified.

9. Grading and prognosis

MALDI IMS has been successfully used to identify subsets of markers that correlate with cancer progression in several cancers including non-small cell lung cancer (76) and pre-invasive bronchial lesions (43), brain tumors (21,101), breast (58), ovarian (102), renal cancer (15), Barrett’s adenocarcinoma (103), intestinal-type gastric cancer (78), prostate carcinoma (104) lymph node metastasis of melanoma (105), prostate cancer (82), colonic cancer (13), papillary thyroid carcinoma (14) and urothelial neoplasia (106).

The accuracy to discriminate normal, pre-invasive and invasive lung tissues obtained by MALDI IMS was >90% (43).

MS studies have also been used to determine tumor grading. In myxoid sarcomas high-grade tumors could be separated from low-grade tumors. Likewise, MS/MS technique revealed signals specific for poorly differentiated gastric cancer (16).

Additionally, proteomic tissue profiling improved the grading of non-invasive papillary urothelial neoplasia (106). Variation in the protein expression pattern of low-grade and high-grade gliomas could also be demonstrated (107,108).

Besides grading, IMS has been employed to identify early stage disease (79) as well as predictive proteomic signatures for lymph node metastasis in gastric cancer (109). Since hypoxia is related to poor survival and increased frequency of metastasis, one study investigated hypoxia associated protein-patterns and identified around 100 proteins that may serve as prognostic markers (81). Notably, one group could also show MALDI IMS as a tool to identify peptide signals to predict tumor response to molecular targeted therapy in a breast cancer mouse model (110). All of these applications have a great potential to find their way into routine diagnostics, as methods are needed that reduce human bias.

10. Identification of drugs and metabolites

IMS has been used to study drug localization in human tissues as well as in animal models (54,111119). The visualization and quantitative analysis of the native drug distribution by IMS techniques with enhanced resolution and sensitivity is desirable for evaluating drug effects and optimizing drug design as it has been shown for paclitaxel in tumor-bearing mice (118). Fresh frozen tumor sections from mice bearing BxPC3 pancreatic cancer xenografts, were analyzed by MALDI IMS and LC-MS after paclitaxel (PTX)-incorporating micelle (NK105) administration (50 or 100 mg/kg) at various time-points (15 min, 1, 24, 48 and 72 h). These sections were compared with tumor sections from mice treated with PTX alone at the same time-points as well as untreated mice. MALDI IMS demonstrated that NK105 successfully delivered a large amount of the PTX within the tumor tissue after NK105 injection compared with PTX injection alone. Quantification of PTX and NK105 were evaluated by LC-MS analysis of the extracted drugs from serial tissue sections for MALDI IMS. The content of the PTX released from NK105 was significantly higher and retained for a longer period of time than the free PTX and control (untreated), suggesting that the antitumor activity of NK105 is superior to that of PTX alone. The high sensitivity and selectivity of IMS combined with visualization of molecular spatial distribution in tissue provides a valuable platform in targeted drug and untargeted metabolomic analysis in biological and clinical research (115). IMS is useful in the comparison of different ways of drug delivery to organs and tissues (120).

Another application is the identification of drugs and their metabolites in the primary or metastatic tumor tissue (112). Furthermore, IMS allowed the characterization of the distribution of small molecules in the microenvironment of tissue compartments of tumors isolated from lung cancer patients and rat xenograft tissues (111). Three experimental models were described in the present study for measuring drug localization. In the ‘concentration gradient model’, an entire solid xenograft tumor (lung adenocarcinoma A549) tissue was immersed in a solution of the drug mixture containing tiotropium and erlotinib for 2.5 h. A passive transfer of the drug mixture into solid tissue samples displayed a decreasing concentration gradient toward the center of the tissue. In this model investigators wanted to show the efficiency of transport of drugs through various cell types. For example, the signal intensity of drugs from tumor cells was substantially lower than that from stroma. In the ‘dispersion model’, 10-μm tissue section of resected lung adenocarcinoma specimens were immersed into the drug solution, where either adsorption or adsorption/absorption occurred. In this model, the distribution of erlotinib localized well to the area of tumor cells identified by the pathologist. Finally, in the ‘directed dosage model’ a drug solution was evenly deposited in small spots (~150 μm in diameter) on the tissue surface of adenocarcinoma tumors using a microdispenser-based spotter apparatus. As in the previous model, the localization of erlotinib was found in tumor areas.

As tumor tissue can be resected during the course of therapy, IMS is suitable for the evaluation of treatment efficacy and the therapy may be optimized (113).

11. MALDI IMS in various organs or tissues

To enable readers of the present review a fast overview on application of MALDI IMS to tumor tissue, Table I provides a brief summary of the different studies and findings.

Table I

Outline of MALDI MS-based studies and findings in the field of cancer research.

Table I

Outline of MALDI MS-based studies and findings in the field of cancer research.

Tissue type/organ/entityContent of the study/findingsAuthors (ref.)
BrainPeptide and protein patterns of primary glial brain tumors and non-tumor tissue; discrimination of increasing tumor gradeSchwartz et al (108)
Identification of protein pattern of gliomas, which could predict short-term and long-term survival (prognosis)Schwartz et al (101)
Grading of meningioma based on different protein patternAgar et al (122)
Classification of brain tumors based on lipid information; discrimination of meningioma from gliomasEberlin et al (100)
Demonstration of drug transit of small molecules through the blood-brain barrierLiu et al (114)
Visualization of brain and tumor distribution of PI3K-inhibitors in models of glioblastomaSalphati et al (119)
BreastMALDI IMS of normal breast tissue, ductal carcinoma in situ, invasive breast cancer and peritumoral stromaCornett et al (58)
Optimized tissue preparation for obtaining peptide mass spectrum profiles from FFPE tissue of breast cancerRonci et al (123)
Visualization of proteins specific for ductal carcinoma in situ and invasive ductal carcinoma (different stage of the disease)Seeley and Caprioli (34)
Determination of lymph node status of breast carcinoma and prediction of response to chemotherapySeeley and Caprioli (125)
Localization of choline metabolites and cations in viable and necrotic tumor regions in a breast cancer xenograft modelAmstalden van Hove et al (127)
Novel approach that combines MALDI-IMS and principal component analysis for generating tumor classificationDjidja et al (63)
Protein identification to predict Her2-status of breast carcinomas-identified cysteine-rich intestinal protein 1Rauser et al (74)
IMS of acylcarnitines, phosphatidylcholines, and sphingomyelin in breast tumor modelsChughtai et al (128)
Discrimination of breast and pancreatic carcinoma based on the peptide profileCasadonte et al (83)
Comparison of protein signals of intratumoral and extratumoral stroma in breast cancer; interlaboratory comparison of spectraDekker et al (73)
Gastrointestinal tract
 OralIMS of biopsy specimen of oral squamous cell carcinoma with reproducible imagesPatel et al (129)
 EsophagusDetection of COX7A2, TAGLN2 and S100-A10 as prognostic markers in Barrett’s adenocarcinomaElsner et al (103)
 StomachDistinguished gastric cancer from normal mucosa; signals overexpressed in tumor were defensins and calgranulins; stage of disease could be predictedKim et al (79)
TMA with classification of signals which could discern between normal gastric tissue and adenocarcinoma; signal specific to poor differentiation corresponds to histone H4Morita et al (16)
Identification of prognostic seven protein signature in intestinal-type gastric cancerBalluff et al (78)
Identification of S100A8 and S100A9 as negative regulators for lymph node metastasis of gastric cancerChoi et al (109)
 ColonClassification algorithm of six common tumors; liver metastasis of colonic cancer was identifiedMeding et al (13)
Lipid signatures in biopsies of liver metastases of colonic cancerThomas et al (130)
IMS of platinum-based metallodrugs in colorectal and ovarian cancerBianga et al (113)
 PancreasDiscrimination of m/z species of normal pancreas, intraepithelial neoplasia, and intraductal papillary mucinous neoplasmsGrüner et al (77)
TMA peptide profiles to discriminate pancreatic from breast cancerCasadonte et al (83)
Imaging of glucose-regulated protein in pancreatic adenocarcinomaDjidja et al (81)
 LiverDemonstration of protein profiles of hepatocellular carcinoma and liver cirrhosisLe Faouder et al (75)
 LungClassification of protein peaks according to lung cancer histology; distinguished primary tumor from metastases, discrimination of patients with good and poor prognosis (frozen tissue)Yanagisawa et al (76)
Predictive accuracy of over 90% of normal tissue, preinvasive lesions and invasive lung cancer based on proteomic profiles of proteins in frozen sectionsRahman et al (131)
TMA of lung tissues with distinction of adenocarinoma and squamous cell carcinoma of the lung by peptide pattern; identification of peptidesGroseclose et al (67)
Non-small cell cancers, classified according to the MALDI lipid profileLee et al (132)
Erlotinib and gefitinib and tiotropium were localized in their microenvironmentVegvari et al (111)
 LymphomaDiscrimination of Hodgkin’s lymphoma and lymphadenitis with a sensitivity and specificity of 83.92% and 89.37% by IMSSchwamborn et al (134)
 SkinDetection of protein signatures for survival and recurrence in malignant melanomaHardesty et al (105)
Differentiation of Spitz nevi from Spitzoid malignant melanoma by IMSLazova et al (135)
Identification of vemurafenib in malignant melanoma and provided evidence of colocalization of drug and targetSugihara et al (112)
 ThyroidIdentification of S100A10, thioredoxin, and S100-A6 as biomarkers of papillary thyroid carcinomas with lymph node metastasisNipp et al (14)
Detection of ribosomal protein P2 specific for papillary thyroid cancerMin et al (136)
Good reproducibility of IMS data on cytological samples to distinguish different thyroid lesions; characterization of the proteomic profile of medullary thyroid carcinomaPagni et al (66)
Urogenital tract
 KidneyAnalysis of tumor margins in renal cell carcinomaOppenheimer et al (44)
Detection of race specific profiles in Wilms’ tumorsAxt et al (139)
Discrimination of papillary and clear cell renal cancer using TMA samples, prediction of tumor survivalSteurer et al (140)
 BladderProteomic tissue profiling improved grading of non-invasive papillary urothelial neoplasiaOezdemir et al (106)
Evaluation of signals associated with tumor aggressiveness, histologic phenotype (growth pattern), and cell proliferation in bladder cancerSteurer et al (140)
 OvaryInvestigation of the interface between serous ovarian carcinoma and normal tissueKang et al (98)
Identification of a fragment of the 11S proteasome activator complex and Reg α fragment as biomarkers for ovarian carcinomaLemaire et al (102)
Platinum anticancer imaging in ovarian carcinomasBianga et al (113)
Integrated transcriptomic and lipidomic analysis of sulfatides in ovarian cancerLiu et al (141)
Presentation of a tryptic peptide reference dataset for IMS on FFPE ovarian cancer tissuesMeding et al (142)
 ProstateDiscrimination of cancerous from non-cancerous prostatic tissue based on protein profile obtained by IMSSchwamborn et al (41)
Identification of cancer and non-cancer tissue on the basis of specific fragment of mitogen-activated protein kinase/extracellular signal regulated kinaseCazares et al (143)
Detection of signals associated with favorable tumor phenotype, prolonged time to PSA relapse; multiple signals associated with the ERG-fusion status and with ERG expressionSteurer et al (82)
 SarcomasIdentification of proteins and lipids in myxoid sarcomas specific to tumor type and grade; could show intra-tumor heterogeneityWillems et al (40)
Brain

There are only a few studies applying IMS in neurobiological science. The reasons for this include limited access to the technology, relatively low sample throughput and difficult sample preparation. However, MS techniques have been applied to a variety of brain tumors including oligodendrogliomas, astrocytomas, meningiomas and gliomas (100,108,121,122). The technique was used in the differential diagnosis, defining the tumor margins, the assessment of the tumor grade and to distinguish different survival groups. Schwartz et al (101) developed a peptide-based profile that could sub-classify gliomas according to different histologic grades on human brain biopsies. Moreover, a short-long and long-term survival-group could be distinguished by the investigators, using the weighted flexible compound covariate method (WFCCM). A proteomic signature of 24 different MS signals discriminated between patients from a short-term survival group (52 patients with a mean survival of <15 months) and a long-term survival group (56 patients with a mean survival of >90 months). These results were also verified as an independent predictor of patient survival using a multivariate Cox proportional hazards model.

IMS has great potential in exploring biomolecular mechanisms underlying disorders. An IMS study developed a preliminary proteomic algorithm that could discriminate meningioma, glioma and non-tumor tissue, although the number of patients was very small (122). In the present review, investigators used support vector machine models able to classify meningioma spectra using a training set built from: i) a single brain tumor class that compared both glioma and meningioma with non-tumor tissue (including blood); ii) a meningioma brain tumor class and non-tumor brain class; and iii) a meningioma class, a glioma class, and a non-tumor brain class. Training sets were built based on the gold standard of WHO histopathology classification of tumors of the central nervous system. Another group was able to discern glioblastoma and oligodendroglioma tumor biopsies by MS but not by IMS (121).

In conjunction with proteomic approaches to assess brain tumors, lipidomic signatures could also provide beneficial information regarding diagnosis, grading and the resection margins (100). Furthermore, pharmacokinetics and pharmacodynamics studies have been performed. Salphati et al (119) visualized and compared the distribution of PI3K inhibitors in glioblastoma multiforme in mouse brain by IMS. Drug transit through the blood-brain barrier (BBB) is essential for therapeutic response in malignant glioma and was studied by IMS (114). In this review, three examples of drug transit through the BBB were reported in mouse brain. Drugs and/or drugs metabolites (BKM120, RAF265 and erlotinib) were imaged in mouse brain tissue sections together with heme, used as a molecular marker delineating the lumen of blood vessels in the brain. In all cases, drugs were found to penetrate the BBB. Specifically, RAF265 and erlotininb were localized within tumor regions, whereas BKM120 distributed in the brain parenchyma. Notably, drugs distributed independently of the heme signal, indicating the escape of the drug molecules from the tumor vasculature.

Breast

MALDI IMS has been applied in breast cancer tissue (58,74,83,123). Additionally, other proteomic mass spectrometric techniques contributed to new insights into breast cancer pathogenesis and prognosis (reviewed in ref. 124). Dijda et al (63) used human breast tumor tissue for the optimization of the protocol for detection of peptides in FFPE sections.

Cornett et al (58) described an automated workflow integrating histopathology and breast tissue profiling of various components in breast cancer tissue. A further IMS analysis of human breast cancer sections revealed three proteins to be specifically localized in different regions of the cancer tissue (34). IMS of metastatic breast cancer in a lymph node found protein signals specifically localized in histologically defined regions (34). An IMS study comparing breast primary tumors from patients with or without lymph node involvement highlighted six differently expressed proteins that could predict lymph node status (125). Besides efforts to elucidate prognostic biomarkers, also predictive profiles have been identified. In a study of breast cancer patients IMS has been shown as a new tool for HER2/neu receptor analysis (74). This is of special interest since at present HER2 amplification status is determined by immunohistochemistry or in situ hybridization or both. These methods suffer from subjective interpretation as well as from high costs and are time-consuming (126).

Dekker et al (73) were able to demonstrate mass signals for stromal activation in breast carcinoma. Furthermore, IMS has been utilized to assess the distribution of lipids in breast cancer showing that heterogeneity is not only restricted to the proteome (127,128).

Since most metastases are adenocarcinomas it might be challenging for the pathologist to determine the origin of the primary tumor. Casadonte et al (83) developed an algorithm to discriminate metastases of breast and pancreatic cancer by MALDI IMS (Fig. 4).

Gastrointestinal tumors

Various studies have addressed MALDI IMS of gastrointestinal tumors including typing, grading and prognosis (13,16,35,75,77,79).

Oral

MALDI IMS was applied to human oral biopsies and revealed a proteomic signature for squamous cell carcinomas (129).

Esophagus

Several prognostic markers could be identified in Barrett’s adenocarcinoma (103).

Stomach

IMS was able to discern between the gastric cancer and the normal gastric mucosa (79). Furthermore, protein profiles from early stage gastric cancer were significantly different from advanced stage gastric tumors (79). Also, specific signals for poorly differentiated gastric cancer were found (16). Choi et al (109) identified proteins as negative regulators for lymph node metastasis in gastric adenocarcinoma. A seven-protein signature was associated with unfavorable overall survival independent of major clinical covariates as demonstrated by MALDI IMS on frozen tissues (78).

Colon

Thomas et al (130) applied IMS technique to detect lipids in human colorectal liver metastasis biopsies. With the help of a tissue based proteomic approach, a large panel of proteins that are associated with regional lymph node metastasis was identified (13). The penetration and distribution of platinum-based metallodrugs was demonstrated in metastatic tissue of colon cancer by IMS (113).

Pancreas

Djidja et al (81) identified a glucose-regulated protein as a biomarker within pancreatic tumor tissue sections. Grüner et al (77) detected several discriminative m/z species that could distinguish between intraepithelial neoplasia, intraductal papillary mucinous neoplasm and normal pancreatic tissue in genetically engineered mouse models. Moreover, metastatic tissue from breast cancer could be discerned from pancreatic cancer with an overall accuracy of 83.38%, a sensitivity of 85.95% and a specificity of 76.96% resulting in a more accurate result than immunohistochemistry even when several antibodies are applied (83).

Investigation of large tissue sections of duodenal mucosa, normal pancreatic tissue and pancreatic carcinoma by MALDI IMS could clearly discern the various tissue compartments (Fig. 5). This method allows ‘painting’ of the different tissues by tissue specific peptide signals in tumor cells (m/z 945), duodenal epithelium (m/z 2264), normal pancreatic tissue (m/z 1506) and smooth muscle (m/z 1185).

Liver

Le Faouder et al (75) were able to distinguish hepatocellular carcinoma from cirrhosis by IMS.

Lung

Rahman et al (131) and Yanagisawa et al (76) reported proteomic patterns specific for normal alveolar and bronchial tissues, pre-invasive lesions and invasive lung cancer. Analysis of microarrays of biopsies from adenocarcinoma and squamous cell carcinoma was performed by Groseclose et al (67) and could clearly discern both tumor types without immunohistochemistry. Besides the proteomic profile, lung cancer could be subclassified also by lipid analysis (132). Proteomic strategies in lung cancer diagnostics in tissue, blood and serum are described elsewhere in detail (133). Notably, EGF-receptor antagonists as target drugs in lung cancer were characterized in lung cancer tissue (111).

Lymphoma

IMS was applied to Hodgkin’s lymphoma and could result in pinpointing differentially expressed molecules, which might represent potential biomarkers. Schwamborn et al (134) could distinguish between classical Hodgkin lymphoma and lymphadenitis.

Skin

Skin malignancies, especially melanoma, are another field where MALDI IMS has been applied successfully. Hardesty et al (105) found peptides that discriminate prognostic subgroups in melanoma patients. Additionally, this group identified signatures associated with favorable and poor survival. IMS has also been utilized to differentiate Spitz naevus and melanoma, which is important due to the completely different therapeutic consequences of both entities (135). Sugihara et al (112) introduced IMS to provide new information on one of the drugs (vemurafenib) currently used in the treatment of malignant melanoma.

Thyroid

MALDI IMS studies have rarely been performed on thyroid cancer tissue. IMS techniques have been used to discriminate thyroid cancer specific peptides from normal thyroid tissue (136). The authors found a thyroid cancer specific protein, however, only five patients were included in the study. Other investigators (14) identified not only a specific proteomic pattern to discriminate non-metastatic from metastatic thyroid cancers but showed also a functional relationship between these proteins and a specific pathway. Pagni et al (66) were able to distinguish between different thyroid lesions applying IMS to fine needle aspiration smears. In the present review, unsupervised statistical analysis and principal component analysis were used to cluster proteomic spectra between papillary thyroid carcinoma, Hürthle cell adenoma, medullary thyroid carcinoma and hyperplastic nodules. Different proteomic signatures were obtained between the histological types with a receiver operating characteristic (ROC) analysis showing an area under the curve >0.8, and a Student’s t-test P-value <0.05. For example, three different proteins detected at 4965, 6278 and 6651 m/z were downregulated in the Hürthle cell adenoma, medullary thyroid carcinoma and papillary thyroid carcinoma patients, when compared to patients with hyperplastic nodules. Nevertheless, by comparing the proteomic profiles obtained from the Hürthle cell adenoma patients with the medullary thyroid carcinoma patients, proteins at 7263, 8294 and 8310 m/z were differentially expressed between the two entities. With these results, investigators highlighted a potential role of MALDI IMS as a supporting tool to discriminate malignant from benign thyroid lesions as well as between different types of thyroid lesions.

Urogenital tract
Kidney

Oppenheimer et al (44) studied tumor margins of renal cell carcinoma by IMS. Junker et al (137) analyzed stage-related protein alterations in kidney cancer using MALDI TOF MS/MS but not IMS. Chinello et al (138) were able to discriminate patients with renal cell carcinoma from normal controls by MALDI TOF technique applied to serum. IMS has been used to identify and map specific peptides that accurately distinguished malignant from normal renal tissue (72). Axt et al (139) identified spectra from both Wilms’ tumor blastema and stroma that independently classified specimens according to race with an accuracy of >80%.

Bladder

Oezdemir et al (106) reported improvement of grading of non-invasive papillary urothelial neoplasia applying IMS. A recent report utilized IMS for the analysis of a bladder cancer tissue microarray to evaluate prognostically relevant molecules (140). From the analysis of 697 patients, numerous m/z signals were found statistically associated with one or several phenotypes including decrease (12 signals) or increase (6 signals) of cell proliferation, papillary (3 signals) or solid (5 signals) growth pattern, and tumor aggressiveness based on stage, grade and nodal status (30 signals).

Ovary

Lemaire et al (102) not only discriminated between benign and malignant ovarian tumors, but identified a new candidate protein biomarker only present in ovarian carcinoma.

Specific proteins in tumor interface zones associated with ovarian serous cancer tissues, were described by Kang et al (98). Liu et al (141) demonstrated that sulfatides are more abundant in ovarian cancer than control tissues.

By analysis of tryptic digests of the FFPE tissue microarray cores by LC-MS/MS, various m/z species observed in MALDI IMS experiments on ovarian cancer could be correctly identified (142). Drug distribution of platinum-based drugs was shown in peritoneal carcinomatosis of ovarian cancer (113).

Prostate

Studies of prostate cancer have utilized IMS to aid diagnosis and for the discovery of proteins relevant to the underlying biology (41,82,143). The first clinical study of human prostate cancer by IMS was performed by Schwambor et al (41).

A specific fragment of mitogen activated protein kinase could discriminate cancer from normal prostatic tissue (143). Furthermore, a marker for early recurrence of prostate cancer has been identified by Steurer et al (82).

Sarcomas

One report utilized IMS for the classification of myxoid sarcomas. Willems et al (40) could discriminate myxofibrosarcoma and myxoid liposarcoma that may share a similar histology. Furthermore, intratumoral heterogeneity was demonstrated in myxofibrosarcomas.

12. Summary

MALDI IMS is a versatile technique which had been applied to various organisms including plants, animals and human tissue. In human tissue and cells, tumor-associated alterations were studied in various entities. MALDI IMS may improve exact determination of tumor margins, tumor typing, grading and prognosis and could have therapeutic implications.

Diagnostic procedures in pathology are based on histology, histochemistry, immunohistochemistry and molecular pathology and will include proteomic techniques like MALDI IMS to improve diagnostic accuracy.

13. Perspectives

MALDI IMS will extend or replace histochemical techniques such as periodic acid-Schiff- and Prussian blue-reaction as well as methods that highlight connective tissue compounds as Masson’s trichrome reaction. Additionally, we foresee that immunohistochemical methods will be at least partly replaced by IMS. This is of great importance, especially if molecular testing is required for diagnostics and only small tissue biopsies are available for such tests. In this regard, MALDI IMS requires only one tissue section for the analysis, thus adequate remaining tissue is available for additional molecular testing. In this scenario, elaborate molecular testing of DNA and RNA alterations will be performed either by next generation sequencing or by mass spectrometric techniques. Applications of IMS in the clinic are growing as this technology has proved its feasibility and versatility. The implementation of biocomputational tools combined with IMS will allow biostatistical evaluation for determination of molecular signals able to type or grade tumors and will provide information about prognosis. Furthermore, drug distribution in different tissue types and cellular components may be monitored by IMS. To ensure similar sample preparation and processing, robust standard operating procedures need to be developed for the application of IMS in routine histopathology. Quality control will be achieved by interlaboratory validation as well as by sharing large databases of MALDI signatures of tumors or other diseases.

References

1 

Patel R: MALDI-TOF mass spectrometry: transformative proteomics for clinical microbiology. Clin Chem. 59:340–342. 2013. View Article : Google Scholar

2 

Clark AE, Kaleta EJ, Arora A and Wolk DM: Matrix-assisted laser desorption ionization-time of flight mass spectrometry: a fundamental shift in the routine practice of clinical microbiology. Clin Microbiol Rev. 26:547–603. 2013. View Article : Google Scholar : PubMed/NCBI

3 

Moore JL, Caprioli RM and Skaar EP: Advanced mass spectrometry technologies for the study of microbial pathogenesis. Curr Opin Microbiol. 19C:45–51. 2014. View Article : Google Scholar

4 

Kueger S, Steinhauser D, Willmitzer L and Giavalisco P: High-resolution plant metabolomics: from mass spectral features to metabolites and from whole-cell analysis to subcellular metabolite distributions. Plant J. 70:39–50. 2012. View Article : Google Scholar : PubMed/NCBI

5 

Schoenian I, Spiteller M, Ghaste M, Wirth R, Herz H and Spiteller D: Chemical basis of the synergism and antagonism in microbial communities in the nests of leaf-cutting ants. Proc Natl Acad Sci USA. 108:1955–1960. 2011. View Article : Google Scholar : PubMed/NCBI

6 

Chaurand P, Cornett DS, Angel PM and Caprioli RM: From whole-body sections down to cellular level, multiscale imaging of phospholipids by MALDI mass spectrometry. Mol Cell Proteomics. 10:O110.004259. 2011. View Article : Google Scholar :

7 

Trim PJ, Henson CM, Avery JL, et al: Matrix-assisted laser desorption/ionization-ion mobility separation-mass spectrometry imaging of vinblastine in whole body tissue sections. Anal Chem. 80:8628–8634. 2008. View Article : Google Scholar : PubMed/NCBI

8 

Reyzer ML, Chaurand P, Angel PM and Caprioli RM: Direct molecular analysis of whole-body animal tissue sections by MALDI imaging mass spectrometry. Methods Mol Biol. 656:285–301. 2010. View Article : Google Scholar : PubMed/NCBI

9 

Remmerbach TW, Maurer K, Janke S, et al: Oral brush biopsy analysis by matrix assisted laser desorption/ionisation-time of flight mass spectrometry profiling: a pilot study. Oral Oncol. 47:278–281. 2011. View Article : Google Scholar : PubMed/NCBI

10 

Schwamborn K, Krieg RC, Uhlig S, Ikenberg H and Wellmann A: MALDI imaging as a specific diagnostic tool for routine cervical cytology specimens. Int J Mol Med. 27:417–421. 2011.

11 

Kriegsmann M, Seeley EH, Schwarting A, et al: MALDI MS imaging as a powerful tool for investigating synovial tissue. Scand J Rheumatol. 41:305–309. 2012. View Article : Google Scholar : PubMed/NCBI

12 

Seeley EH and Caprioli RM: MALDI imaging mass spectrometry of human tissue: method challenges and clinical perspectives. Trends Biotechnol. 29:136–143. 2011. View Article : Google Scholar : PubMed/NCBI

13 

Meding S, Nitsche U, Balluff B, et al: Tumor classification of six common cancer types based on proteomic profiling by MALDI imaging. J Proteome Res. 11:1996–2003. 2012. View Article : Google Scholar : PubMed/NCBI

14 

Nipp M, Elsner M, Balluff B, et al: S100-A10, thioredoxin, and S100-A6 as biomarkers of papillary thyroid carcinoma with lymph node metastasis identified by MALDI imaging. J Mol Med. 90:163–174. 2012. View Article : Google Scholar

15 

Steurer S, Seddiqi AS, Singer JM, et al: MALDI imaging on tissue microarrays identifies molecular features associated with renal cell cancer phenotype. Anticancer Res. 34:2255–2261. 2014.PubMed/NCBI

16 

Morita Y, Ikegami K, Goto-Inoue N, et al: Imaging mass spectrometry of gastric carcinoma in formalin-fixed paraffin-embedded tissue microarray. Cancer Sci. 101:267–273. 2010. View Article : Google Scholar

17 

Gode D and Volmer DA: Lipid imaging by mass spectrometry - a review. Analyst. 138:1289–1315. 2013. View Article : Google Scholar : PubMed/NCBI

18 

Horn PJ and Chapman KD: Lipidomics in situ: insights into plant lipid metabolism from high resolution spatial maps of metabolites. Prog Lipid Res. 54:32–52. 2014. View Article : Google Scholar : PubMed/NCBI

19 

Sparvero LJ, Amoscato AA, Dixon CE, et al: Mapping of phospholipids by MALDI imaging (MALDI-MSI): realities and expectations. Chem Phys Lipids. 165:545–562. 2012. View Article : Google Scholar : PubMed/NCBI

20 

Harvey DJ: Analysis of carbohydrates and glycoconjugates by matrix-assisted laser desorption/ionization mass spectrometry: An update for 2009–2010. Mass Spectrom Rev. May 26–2014. View Article : Google Scholar : (Epub ahead of print).

21 

Reyzer ML, Hsieh Y, Ng K, Korfmacher WA and Caprioli RM: Direct analysis of drug candidates in tissue by matrix-assisted laser desorption/ionization mass spectrometry. J Mass Spectrom. 38:1081–1092. 2003. View Article : Google Scholar : PubMed/NCBI

22 

Norris JL and Caprioli RM: Analysis of tissue specimens by matrix-assisted laser desorption/ionization imaging mass spectrometry in biological and clinical research. Chem Rev. 113:2309–2342. 2013. View Article : Google Scholar : PubMed/NCBI

23 

Groseclose MR and Castellino S: A mimetic tissue model for the quantification of drug distributions by MALDI imaging mass spectrometry. Anal Chem. 85:10099–10106. 2013. View Article : Google Scholar : PubMed/NCBI

24 

Honisch C, Chen Y, Mortimer C, et al: Automated comparative sequence analysis by base-specific cleavage and mass spectrometry for nucleic acid-based microbial typing. Proc Natl Acad Sci USA. 104:10649–10654. 2007. View Article : Google Scholar : PubMed/NCBI

25 

Okamoto I, Sakai K, Morita S, et al: Multiplex genomic profiling of non-small cell lung cancers from the LETS phase III trial of first-line S-1/carboplatin versus paclitaxel/carboplatin: results of a West Japan Oncology Group study. Oncotarget. 5:2293–2304. 2014.PubMed/NCBI

26 

Castellino S, Groseclose MR and Wagner D: MALDI imaging mass spectrometry: bridging biology and chemistry in drug development. Bioanalysis. 3:2427–2441. 2011. View Article : Google Scholar : PubMed/NCBI

27 

Rompp A, Guenther S, Takats Z and Spengler B: Mass spectrometry imaging with high resolution in mass and space (HR(2) MSI) for reliable investigation of drug compound distributions on the cellular level. Anal Bioanal Chem. 401:65–73. 2011. View Article : Google Scholar : PubMed/NCBI

28 

Caprioli RM, Farmer TB and Gile J: Molecular imaging of biological samples: localization of peptides and proteins using MALDI-TOF MS. Anal Chem. 69:4751–4760. 1997. View Article : Google Scholar : PubMed/NCBI

29 

Schone C, Hofler H and Walch A: MALDI imaging mass spectrometry in cancer research: combining proteomic profiling and histological evaluation. Clin Biochem. 46:539–545. 2013. View Article : Google Scholar : PubMed/NCBI

30 

Gessel MM, Norris JL and Caprioli RM: MALDI imaging mass spectrometry: spatial molecular analysis to enable a new age of discovery. J Proteomics. 107:71–82. 2014. View Article : Google Scholar : PubMed/NCBI

31 

Thomas A, Lenglet S, Chaurand P, et al: Mass spectrometry for the evaluation of cardiovascular diseases based on proteomics and lipidomics. Thromb Haemost. 106:20–33. 2011. View Article : Google Scholar : PubMed/NCBI

32 

McClure RA, Chumbley CW, Reyzer ML, et al: Identification of promethazine as an amyloid-binding molecule using a fluorescence high-throughput assay and MALDI imaging mass spectrometry. Neuroimage Clin. 2:620–629. 2013. View Article : Google Scholar : PubMed/NCBI

33 

Kriegsmann M, Casadonte R, Randau T, et al: MALDI imaging of predictive ferritin, fibrinogen and proteases in haemophilic arthropathy. Haemophilia. 20:446–453. 2014. View Article : Google Scholar : PubMed/NCBI

34 

Seeley EH and Caprioli RM: Molecular imaging of proteins in tissues by mass spectrometry. Proc Natl Acad Sci USA. 105:18126–18131. 2008. View Article : Google Scholar : PubMed/NCBI

35 

Seeley EH, Washington MK, Caprioli RM and M’Koma AE: Proteomic patterns of colonic mucosal tissues delineate Crohn’s colitis and ulcerative colitis. Proteomics Clin Appl. 7:541–549. 2013. View Article : Google Scholar : PubMed/NCBI

36 

Lalowski M, Magni F, Mainini V, et al: Imaging mass spectrometry: a new tool for kidney disease investigations. Nephrol Dial Transplant. 28:1648–1656. 2013. View Article : Google Scholar : PubMed/NCBI

37 

Mainini V, Pagni F, Ferrario F, et al: MALDI imaging mass spectrometry in glomerulonephritis: feasibility study. Histopathology. 64:901–906. 2014. View Article : Google Scholar

38 

Xu BJ, Shyr Y, Liang X, et al: Proteomic patterns and prediction of glomerulosclerosis and its mechanisms. J Am Soc Nephrol. 16:2967–2975. 2005. View Article : Google Scholar : PubMed/NCBI

39 

Lagarrigue M, Becker M, Lavigne R, et al: Revisiting rat spermatogenesis with MALDI imaging at 20-microm resolution. Mol Cell Proteomic. 10:M110.005991. 2011. View Article : Google Scholar

40 

Willems SM, van Remoortere A, van Zeijl R, Deelder AM, McDonnell LA and Hogendoorn PC: Imaging mass spectrometry of myxoid sarcomas identifies proteins and lipids specific to tumour type and grade, and reveals biochemical intratumour heterogeneity. J Pathol. 222:400–409. 2010. View Article : Google Scholar : PubMed/NCBI

41 

Schwamborn K, Krieg RC, Reska M, Jakse G, Knuechel R and Wellmann A: Identifying prostate carcinoma by MALDI-Imaging. Int J Mol Med. 20:155–159. 2007.PubMed/NCBI

42 

Rodrigo MA, Zitka O, Krizkova S, Moulick A, Adam V and Kizek R: MALDI-TOF MS as evolving cancer diagnostic tool: a review. J Pharm Biomed Anal. 95:245–255. 2014. View Article : Google Scholar : PubMed/NCBI

43 

Rahman SM, Gonzalez AL, Li M, et al: Lung cancer diagnosis from proteomic analysis of preinvasive lesions. Cancer Res. 71:3009–3017. 2011. View Article : Google Scholar : PubMed/NCBI

44 

Oppenheimer SR, Mi D, Sanders ME and Caprioli RM: Molecular analysis of tumor margins by MALDI mass spectrometry in renal carcinoma. J Proteome Res. 9:2182–2190. 2010. View Article : Google Scholar : PubMed/NCBI

45 

Jones EE, Powers TW, Neely BA, et al: MALDI imaging mass spectrometry profiling of proteins and lipids in clear cell renal cell carcinoma. Proteomics. 14:924–935. 2014. View Article : Google Scholar : PubMed/NCBI

46 

Angel PM and Caprioli RM: Matrix-assisted laser desorption ionization imaging mass spectrometry: in situ molecular mapping. Biochemistry. 52:3818–3828. 2013. View Article : Google Scholar

47 

Boggio KJ, Obasuyi E, Sugino K, Nelson SB, Agar NY and Agar JN: Recent advances in single-cell MALDI mass spectrometry imaging and potential clinical impact. Expert Rev Proteomics. 8:591–604. 2011. View Article : Google Scholar : PubMed/NCBI

48 

Eriksson C, Masaki N, Yao I, Hayasaka T and Setou M: MALDI imaging mass spectrometry-A mini review of methods and recent developments. Mass Spectrom. 2:S00222013. View Article : Google Scholar

49 

Dreisewerd K: Recent methodological advances in MALDI mass spectrometry. Anal Bioanal Chem. 406:2261–2278. 2014. View Article : Google Scholar : PubMed/NCBI

50 

Fujimura Y and Miura D: MALDI mass spectrometry imaging for visualizing in situ metabolism of endogenous metabolites and dietary phytochemicals. Metabolites. 4:319–346. 2014. View Article : Google Scholar : PubMed/NCBI

51 

Gorzolka K and Walch A: MALDI mass spectrometry imaging of formalin-fixed paraffin-embedded tissues in clinical research. Histol Histopathol. 29:1365–1376. 2014.PubMed/NCBI

52 

Schwamborn K and Caprioli RM: Molecular imaging by mass spectrometry: looking beyond classical histology. Nat Rev Cancer. 10:639–646. 2010. View Article : Google Scholar : PubMed/NCBI

53 

Chaurand P: Imaging mass spectrometry of thin tissue sections: a decade of collective efforts. J Proteomics. 75:4883–4892. 2012. View Article : Google Scholar : PubMed/NCBI

54 

Rompp A and Spengler B: Mass spectrometry imaging with high resolution in mass and space. Histochem Cell Biol. 139:759–783. 2013. View Article : Google Scholar : PubMed/NCBI

55 

Goodwin RJ: Sample preparation for mass spectrometry imaging: small mistakes can lead to big consequences. J Proteomics. 75:4893–4911. 2012. View Article : Google Scholar : PubMed/NCBI

56 

Kaletas BK, van der Wiel IM, Stauber J, et al: Sample preparation issues for tissue imaging by imaging MS. Proteomics. 9:2622–2633. 2009. View Article : Google Scholar : PubMed/NCBI

57 

Stoeckli M, Chaurand P, Hallahan DE and Caprioli RM: Imaging mass spectrometry: a new technology for the analysis of protein expression in mammalian tissues. Nat Med. 7:493–496. 2001. View Article : Google Scholar : PubMed/NCBI

58 

Cornett DS, Mobley JA, Dias EC, et al: A novel histology-directed strategy for MALDI-MS tissue profiling that improves throughput and cellular specificity in human breast cancer. Mol Cell Proteomics. 5:1975–1983. 2006. View Article : Google Scholar : PubMed/NCBI

59 

Seeley EH, Schwamborn K and Caprioli RM: Imaging of intact tissue sections: moving beyond the microscope. J Biol Chem. 286:25459–25466. 2011. View Article : Google Scholar : PubMed/NCBI

60 

Zavalin A, Yang J and Caprioli R: Laser beam filtration for high spatial resolution MALDI imaging mass spectrometry. J Am Soc Mass Spectrom. 24:1153–1156. 2013. View Article : Google Scholar : PubMed/NCBI

61 

Caprioli RM: Imaging mass spectrometry: molecular microscopy for enabling a new age of discovery. Proteomics. 14:807–809. 2014. View Article : Google Scholar : PubMed/NCBI

62 

Norris JL, Cornett DS, Mobley JA, et al: Processing MALDI Mass Spectra to improve mass spectral direct tissue analysis. Int J Mass Spectrom. 260:212–221. 2007. View Article : Google Scholar : PubMed/NCBI

63 

Djidja MC, Claude E, Snel MF, et al: Novel molecular tumour classification using MALDI-mass spectrometry imaging of tissue microarray. Anal Bioanal Chem. 397:587–601. 2010. View Article : Google Scholar : PubMed/NCBI

64 

Andersson M, Groseclose MR, Deutch AY and Caprioli RM: Imaging mass spectrometry of proteins and peptides: 3D volume reconstruction. Nat Methods. 5:101–108. 2008. View Article : Google Scholar : PubMed/NCBI

65 

Crecelius AC, Cornett DS, Caprioli RM, Williams B, Dawant BM and Bodenheimer B: Three-dimensional visualization of protein expression in mouse brain structures using imaging mass spectrometry. J Am Soc Mass Spectrom. 16:1093–1099. 2005. View Article : Google Scholar : PubMed/NCBI

66 

Pagni F, Mainini V, Garancini M, et al: Proteomics for the diagnosis of thyroid lesions: preliminary report. Cytopathology. Jul 20–2014. View Article : Google Scholar : (Epub ahead of print).

67 

Groseclose MR, Massion PP, Chaurand P and Caprioli RM: High-throughput proteomic analysis of formalin-fixed paraffin-embedded tissue microarrays using MALDI imaging mass spectrometry. Proteomics. 8:3715–3724. 2008. View Article : Google Scholar : PubMed/NCBI

68 

Gancberg D, Jarvinen T, di Leo A, et al: Evaluation of HER-2/NEU protein expression in breast cancer by immunohistochemistry: an interlaboratory study assessing the reproducibility of HER-2/NEU testing. Breast Cancer Res Treat. 74:113–120. 2002. View Article : Google Scholar : PubMed/NCBI

69 

Thaysen-Andersen M, Wilkinson BL, Payne RJ and Packer NH: Site-specific characterisation of densely O-glycosylated mucin-type peptides using electron transfer dissociation ESI-MS/MS. Electrophoresis. 32:3536–3545. 2011. View Article : Google Scholar : PubMed/NCBI

70 

Ronci M, Sharma S, Chataway T, et al: MALDI-MS-imaging of whole human lens capsule. J Proteome Res. 10:3522–3529. 2011. View Article : Google Scholar : PubMed/NCBI

71 

Bona A, Papai Z, Maasz G, et al: Mass spectrometric identification of ancient proteins as potential molecular biomarkers for a 2000-year-old osteogenic sarcoma. PLoS One. 9:e872152014. View Article : Google Scholar : PubMed/NCBI

72 

Morgan TM, Seeley EH, Fadare O, Caprioli RM and Clark PE: Imaging the clear cell renal cell carcinoma proteome. J Urol. 189:1097–1103. 2013. View Article : Google Scholar :

73 

Dekker TJ, Balluff BD, Jones EA, et al: Multicenter Matrix-assisted laser desorption/ionization mass spectrometry imaging (MALDI MSI) identifies proteomic differences in breast-cancer-associated stroma. J Proteome Res. May 2–2014.(Epub ahead of print). View Article : Google Scholar

74 

Rauser S, Marquardt C, Balluff B, et al: Classification of HER2 receptor status in breast cancer tissues by MALDI imaging mass spectrometry. J Proteome Res. 9:1854–1863. 2010. View Article : Google Scholar : PubMed/NCBI

75 

Le Faouder J, Laouirem S, Chapelle M, et al: Imaging mass spectrometry provides fingerprints for distinguishing hepatocellular carcinoma from cirrhosis. J Proteome Res. 10:3755–3765. 2011. View Article : Google Scholar : PubMed/NCBI

76 

Yanagisawa K, Shyr Y, Xu BJ, et al: Proteomic patterns of tumour subsets in non-small-cell lung cancer. Lancet. 362:433–439. 2003. View Article : Google Scholar : PubMed/NCBI

77 

Gruner BM, Hahne H, Mazur PK, et al: MALDI imaging mass spectrometry for in situ proteomic analysis of preneoplastic lesions in pancreatic cancer. PLoS One. 7:e394242012. View Article : Google Scholar : PubMed/NCBI

78 

Balluff B, Rauser S, Meding S, et al: MALDI imaging identifies prognostic seven-protein signature of novel tissue markers in intestinal-type gastric cancer. Am J Pathol. 179:2720–2729. 2011. View Article : Google Scholar : PubMed/NCBI

79 

Kim HK, Reyzer ML, Choi IJ, et al: Gastric cancer-specific protein profile identified using endoscopic biopsy samples via MALDI mass spectrometry. J Proteome Res. 9:4123–4130. 2010. View Article : Google Scholar : PubMed/NCBI

80 

Casadonte R and Caprioli RM: Proteomic analysis of formalin-fixed paraffin-embedded tissue by MALDI imaging mass spectrometry. Nat Protoc. 6:1695–1709. 2011. View Article : Google Scholar : PubMed/NCBI

81 

Djidja MC, Chang J, Hadjiprocopis A, et al: Identification of hypoxia-regulated proteins using MALDI-mass spectrometry imaging combined with quantitative proteomics. J Proteome Res. 13:2297–2313. 2014. View Article : Google Scholar : PubMed/NCBI

82 

Steurer S, Borkowski C, Odinga S, et al: MALDI mass spectrometric imaging based identification of clinically relevant signals in prostate cancer using large-scale tissue microarrays. Int J Cancer. 133:920–928. 2013. View Article : Google Scholar : PubMed/NCBI

83 

Casadonte R, Kriegsmann M, Zweynert F, et al: Imaging mass spectrometry to discriminate breast from pancreatic cancer metastasis in formalin-fixed paraffin-embedded tissues. Proteomics. 14:956–964. 2014. View Article : Google Scholar : PubMed/NCBI

84 

Ikeda K, Monden T, Kanoh T, et al: Extraction and analysis of diagnostically useful proteins from formalin-fixed, paraffin-embedded tissue sections. J Histochem Cytochem. 46:397–403. 1998. View Article : Google Scholar : PubMed/NCBI

85 

Becker KF, Schott C, Hipp S, et al: Quantitative protein analysis from formalin-fixed tissues: implications for translational clinical research and nanoscale molecular diagnosis. J Pathol. 211:370–378. 2007. View Article : Google Scholar

86 

Chung JY, Lee SJ, Kris Y, Braunschweig T, Traicoff JL and Hewitt SM: A well-based reverse-phase protein array applicable to extracts from formalin-fixed paraffin-embedded tissue. Proteomics Clin Appl. 2:1539–1547. 2008. View Article : Google Scholar : PubMed/NCBI

87 

Nirmalan NJ, Harnden P, Selby PJ and Banks RE: Development and validation of a novel protein extraction methodology for quantitation of protein expression in formalin-fixed paraffin-embedded tissues using western blotting. J Pathol. 217:497–506. 2009. View Article : Google Scholar : PubMed/NCBI

88 

Crockett DK, Lin Z, Vaughn CP, Lim MS and Elenitoba-Johnson KS: Identification of proteins from formalin-fixed paraffin-embedded cells by LC-MS/MS. Lab Invest. 85:1405–1415. 2005. View Article : Google Scholar : PubMed/NCBI

89 

Hood BL, Darfler MM, Guiel TG, et al: Proteomic analysis of formalin-fixed prostate cancer tissue. Mol Cell Proteomics. 4:1741–1753. 2005. View Article : Google Scholar : PubMed/NCBI

90 

Palmer-Toy DE, Krastins B, Sarracino DA, Nadol JB Jr and Merchant SN: Efficient method for the proteomic analysis of fixed and embedded tissues. J Proteome Res. 4:2404–2411. 2005. View Article : Google Scholar : PubMed/NCBI

91 

Becker KF, Berg D, Malinowsky K, et al: Update on protein analysis of fixed tissues. Pathologe. 31(Suppl 2): 263–267. 2010. View Article : Google Scholar

92 

Shi SR, Liu C, Balgley BM, Lee C and Taylor CR: Protein extraction from formalin-fixed, paraffin-embedded tissue sections: quality evaluation by mass spectrometry. J Histochem Cytochem. 54:739–743. 2006. View Article : Google Scholar : PubMed/NCBI

93 

McDonnell LA, Walch A, Stoeckli M and Corthals GL: MSiMass list: a public database of identifications for protein MALDI MS imaging. J Proteome Res. 13:1138–1142. 2014. View Article : Google Scholar

94 

Maier SK, Hahne H, Gholami AM, et al: Comprehensive identification of proteins from MALDI imaging. Mol Cell Proteomics. 12:2901–2910. 2013. View Article : Google Scholar : PubMed/NCBI

95 

Deininger SO, Ebert MP, Futterer A, Gerhard M and Rocken C: MALDI imaging combined with hierarchical clustering as a new tool for the interpretation of complex human cancers. J Proteome Res. 7:5230–5236. 2008. View Article : Google Scholar

96 

Caprioli RM: Deciphering protein molecular signatures in cancer tissues to aid in diagnosis, prognosis, and therapy. Cancer Res. 65:10642–10645. 2005. View Article : Google Scholar : PubMed/NCBI

97 

Chaurand P, Sanders ME, Jensen RA and Caprioli RM: Proteomics in diagnostic pathology: profiling and imaging proteins directly in tissue sections. Am J Pathol. 165:1057–1068. 2004. View Article : Google Scholar : PubMed/NCBI

98 

Kang S, Shim HS, Lee JS, et al: Molecular proteomics imaging of tumor interfaces by mass spectrometry. J Proteome Res. 9:1157–1164. 2010. View Article : Google Scholar

99 

Han EC, Lee YS, Liao WS, Liu YC, Liao HY and Jeng LB: Direct tissue analysis by MALDI-TOF mass spectrometry in human hepatocellular carcinoma. Clin Chim Acta. 412:230–239. 2011. View Article : Google Scholar

100 

Eberlin LS, Norton I, Orringer D, et al: Ambient mass spectrometry for the intraoperative molecular diagnosis of human brain tumors. Proc Natl Acad Sci USA. 110:1611–1616. 2013. View Article : Google Scholar : PubMed/NCBI

101 

Schwartz SA, Weil RJ, Thompson RC, et al: Proteomic-based prognosis of brain tumor patients using direct-tissue matrix-assisted laser desorption ionization mass spectrometry. Cancer Res. 65:7674–7681. 2005.PubMed/NCBI

102 

Lemaire R, Menguellet SA, Stauber J, et al: Specific MALDI imaging and profiling for biomarker hunting and validation: fragment of the 11S proteasome activator complex, Reg alpha fragment, is a new potential ovary cancer biomarker. J Proteome Res. 6:4127–4134. 2007. View Article : Google Scholar : PubMed/NCBI

103 

Elsner M, Rauser S, Maier S, et al: MALDI imaging mass spectrometry reveals COX7A2, TAGLN2 and S100-A10 as novel prognostic markers in Barrett’s adenocarcinoma. J Proteomics. 75:4693–4704. 2012. View Article : Google Scholar : PubMed/NCBI

104 

Flatley B, Malone P and Cramer R: MALDI mass spectrometry in prostate cancer biomarker discovery. Biochim Biophys Acta. 1844:940–949. 2014. View Article : Google Scholar

105 

Hardesty WM, Kelley MC, Mi D, Low RL and Caprioli RM: Protein signatures for survival and recurrence in metastatic melanoma. J Proteomics. 74:1002–1014. 2011. View Article : Google Scholar : PubMed/NCBI

106 

Oezdemir RF, Gaisa NT, Lindemann-Docter K, et al: Proteomic tissue profiling for the improvement of grading of noninvasive papillary urothelial neoplasia. Clin Biochem. 45:7–11. 2012. View Article : Google Scholar

107 

Chaurand P, Schwartz SA, Billheimer D, Xu BJ, Crecelius A and Caprioli RM: Integrating histology and imaging mass spectrometry. Anal Chem. 76:1145–1155. 2004. View Article : Google Scholar : PubMed/NCBI

108 

Schwartz SA, Weil RJ, Johnson MD, Toms SA and Caprioli RM: Protein profiling in brain tumors using mass spectrometry: feasibility of a new technique for the analysis of protein expression. Clin Cancer Res. 10:981–987. 2004. View Article : Google Scholar : PubMed/NCBI

109 

Choi JH, Shin NR, Moon HJ, et al: Identification of S100A8 and S100A9 as negative regulators for lymph node metastasis of gastric adenocarcinoma. Histol Histopathol. 27:1439–1448. 2012.PubMed/NCBI

110 

Reyzer ML, Caldwell RL, Dugger TC, et al: Early changes in protein expression detected by mass spectrometry predict tumor response to molecular therapeutics. Cancer Res. 64:9093–9100. 2004. View Article : Google Scholar : PubMed/NCBI

111 

Vegvari A, Fehniger TE, Rezeli M, et al: Experimental models to study drug distributions in tissue using MALDI mass spectrometry imaging. J Proteome Res. 12:5626–5633. 2013. View Article : Google Scholar : PubMed/NCBI

112 

Sugihara Y, Vegvari A, Welinder C, et al: A new look at drugs targeting malignant melanoma - an application for mass spectrometry imaging. Proteomics. 14:1963–1970. 2014. View Article : Google Scholar : PubMed/NCBI

113 

Bianga J, Bouslimani A, Bec N, et al: Complementarity of MALDI and LA ICP mass spectrometry for platinum anticancer imaging in human tumor. Metallomics. 6:1382–1386. 2014. View Article : Google Scholar : PubMed/NCBI

114 

Liu X, Ide JL, Norton I, et al: Molecular imaging of drug transit through the blood-brain barrier with MALDI mass spectrometry imaging. Sci Rep. 3:28592013.PubMed/NCBI

115 

Buck A and Walch A: In situ drug and metabolite analyzes in biological and clinical research by MALDI MS imaging. Bioanalysis. 6:1241–1253. 2014. View Article : Google Scholar : PubMed/NCBI

116 

Jirasko R, Holcapek M, Kunes M and Svatos A: Distribution study of atorvastatin and its metabolites in rat tissues using combined information from UHPLC/MS and MALDI-Orbitrap-MS imaging. Anal Bioanal Chem. 406:4601–4610. 2014. View Article : Google Scholar : PubMed/NCBI

117 

Huber K, Aichler M, Sun N, et al: A rapid ex vivo tissue model for optimising drug detection and ionisation in MALDI imaging studies. Histochem Cell Biol. 142:361–371. 2014. View Article : Google Scholar : PubMed/NCBI

118 

Yasunaga M, Furuta M, Ogata K, et al: The significance of microscopic mass spectrometry with high resolution in the visualisation of drug distribution. Sci Rep. 3:30502013. View Article : Google Scholar : PubMed/NCBI

119 

Salphati L, Shahidi-Latham S, Quiason C, et al: Distribution of the phosphatidylinositol 3-kinase inhibitors Pictilisib (GDC-0941) and GNE-317 in U87 and GS2 intracranial glioblastoma models-assessment by matrix-assisted laser desorption ionization imaging. Drug Metab Dispos. 42:1110–1116. 2014. View Article : Google Scholar : PubMed/NCBI

120 

Zecchi R, Trevisani M, Pittelli M, et al: Impact of drug administration route on drug delivery and distribution into the lung: an imaging mass spectrometry approach. Eur J Mass Spectrom. 19:475–482. 2013. View Article : Google Scholar

121 

Bouamrani A, Ternier J, Ratel D, et al: Direct-tissue SELDI-TOF mass spectrometry analysis: a new application for clinical proteomics. Clin Chem. 52:2103–2106. 2006. View Article : Google Scholar : PubMed/NCBI

122 

Agar NY, Malcolm JG, Mohan V, et al: Imaging of meningioma progression by matrix-assisted laser desorption ionization time-of-flight mass spectrometry. Anal Chem. 82:2621–2625. 2010. View Article : Google Scholar : PubMed/NCBI

123 

Ronci M, Bonanno E, Colantoni A, et al: Protein unlocking procedures of formalin-fixed paraffin-embedded tissues: application to MALDI-TOF imaging MS investigations. Proteomics. 8:3702–3714. 2008. View Article : Google Scholar : PubMed/NCBI

124 

Qin XJ and Ling BX: Proteomic studies in breast cancer (Review). Oncol Lett. 3:735–743. 2012.PubMed/NCBI

125 

Seeley EH and Caprioli RM: Imaging mass spectrometry: towards clinical diagnostics. Proteomics Clin Appl. 2:1435–1443. 2008. View Article : Google Scholar : PubMed/NCBI

126 

Walch A, Rauser S, Deininger SO and Hofler H: MALDI imaging mass spectrometry for direct tissue analysis: a new frontier for molecular histology. Histochem Cell Biol. 130:421–434. 2008. View Article : Google Scholar : PubMed/NCBI

127 

Amstalden van Hove ER, Blackwell TR, Klinkert I, Eijkel GB, Heeren RM and Glunde K: Multimodal mass spectrometric imaging of small molecules reveals distinct spatio-molecular signatures in differentially metastatic breast tumor models. Cancer Res. 70:9012–9021. 2010. View Article : Google Scholar : PubMed/NCBI

128 

Chughtai K, Jiang L, Greenwood TR, Glunde K and Heeren RM: Mass spectrometry images acylcarnitines, phosphatidylcholines, and sphingomyelin in MDA-MB-231 breast tumor models. J Lipid Res. 54:333–344. 2013. View Article : Google Scholar :

129 

Patel SA, Barnes A, Loftus N, et al: Imaging mass spectrometry using chemical inkjet printing reveals differential protein expression in human oral squamous cell carcinoma. Analyst. 134:301–307. 2009. View Article : Google Scholar : PubMed/NCBI

130 

Thomas A, Patterson NH, Marcinkiewicz MM, Lazaris A, Metrakos P and Chaurand P: Histology-driven data mining of lipid signatures from multiple imaging mass spectrometry analyses: application to human colorectal cancer liver metastasis biopsies. Anal Chem. 85:2860–2866. 2013. View Article : Google Scholar : PubMed/NCBI

131 

Rahman SM, Shyr Y, Yildiz PB, et al: Proteomic patterns of preinvasive bronchial lesions. Am J Respir Crit Care Med. 172:1556–1562. 2005. View Article : Google Scholar : PubMed/NCBI

132 

Lee GK, Lee HS, Park YS, et al: Lipid MALDI profile classifies non-small cell lung cancers according to the histologic type. Lung Cancer. 76:197–203. 2012. View Article : Google Scholar

133 

Hassanein M, Rahman JS, Chaurand P and Massion PP: Advances in proteomic strategies toward the early detection of lung cancer. Proc Am Thorac Soc. 8:183–188. 2011. View Article : Google Scholar : PubMed/NCBI

134 

Schwamborn K, Krieg RC, Jirak P, et al: Application of MALDI imaging for the diagnosis of classical Hodgkin lymphoma. J Cancer Res Clin Oncol. 136:1651–1655. 2010. View Article : Google Scholar : PubMed/NCBI

135 

Lazova R, Seeley EH, Keenan M, Gueorguieva R and Caprioli RM: Imaging mass spectrometry - a new and promising method to differentiate Spitz nevi from Spitzoid malignant melanomas. Am J Dermatopathol. 34:82–90. 2012. View Article : Google Scholar :

136 

Min KW, Bang JY, Kim KP, et al: Imaging mass spectrometry in papillary thyroid carcinoma for the identification and validation of biomarker proteins. J Korean Med Sci. 29:934–940. 2014. View Article : Google Scholar : PubMed/NCBI

137 

Junker H, Venz S, Zimmermann U, Thiele A, Scharf C and Walther R: Stage-related alterations in renal cell carcinoma-comprehensive quantitative analysis by 2D-DIGE and protein network analysis. PLoS One. 6:e218672011. View Article : Google Scholar

138 

Chinello C, Gianazza E, Zoppis I, et al: Serum biomarkers of renal cell carcinoma assessed using a protein profiling approach based on ClinProt technique. Urology. 75:842–847. 2010. View Article : Google Scholar

139 

Axt J, Murphy AJ, Seeley EH, et al: Race disparities in Wilms tumor incidence and biology. J Surg Res. 170:112–119. 2011. View Article : Google Scholar : PubMed/NCBI

140 

Steurer S, Singer JM, Rink M, et al: MALDI imaging-based identification of prognostically relevant signals in bladder cancer using large-scale tissue microarrays. Urol Oncol. Aug 14–2014. View Article : Google Scholar : (Epub ahead of print).

141 

Liu Y, Chen Y, Momin A, et al: Elevation of sulfatides in ovarian cancer: an integrated transcriptomic and lipidomic analysis including tissue-imaging mass spectrometry. Mol Cancer. 9:1862010. View Article : Google Scholar : PubMed/NCBI

142 

Meding S, Martin K, Gustafsson OJ, et al: Tryptic peptide reference data sets for MALDI imaging mass spectrometry on formalin-fixed ovarian cancer tissues. J Proteome Res. 12:308–315. 2013. View Article : Google Scholar

143 

Cazares LH, Troyer D, Mendrinos S, et al: Imaging mass spectrometry of a specific fragment of mitogen-activated protein kinase/extracellular signal-regulated kinase kinase kinase 2 discriminates cancer from uninvolved prostate tissue. Clin Cancer Res. 15:5541–5551. 2009. View Article : Google Scholar : PubMed/NCBI

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March-2015
Volume 46 Issue 3

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Spandidos Publications style
Kriegsmann J, Kriegsmann M and Casadonte R: MALDI TOF imaging mass spectrometry in clinical pathology: A valuable tool for cancer diagnostics (Review). Int J Oncol 46: 893-906, 2015
APA
Kriegsmann, J., Kriegsmann, M., & Casadonte, R. (2015). MALDI TOF imaging mass spectrometry in clinical pathology: A valuable tool for cancer diagnostics (Review). International Journal of Oncology, 46, 893-906. https://doi.org/10.3892/ijo.2014.2788
MLA
Kriegsmann, J., Kriegsmann, M., Casadonte, R."MALDI TOF imaging mass spectrometry in clinical pathology: A valuable tool for cancer diagnostics (Review)". International Journal of Oncology 46.3 (2015): 893-906.
Chicago
Kriegsmann, J., Kriegsmann, M., Casadonte, R."MALDI TOF imaging mass spectrometry in clinical pathology: A valuable tool for cancer diagnostics (Review)". International Journal of Oncology 46, no. 3 (2015): 893-906. https://doi.org/10.3892/ijo.2014.2788