From the Core Unit Chip Application (CUCA), Institute of Human Genetics and Anthropology, Friedrich-Schiller-University, 07740 Jena, Germany,
Clinic of ENT Diseases, Friedrich-Schiller-University, 07740 Jena, Germany, ¶ Ciphergen Biosystems GmbH, 37085 Göttingen, Germany, || Institute of Anatomy II, Friedrich-Schiller-University, 07740 Jena, Germany, and ** SIRS-Lab GmbH, 07745 Jena, Germany
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ABSTRACT |
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Head and neck squamous-cell carcinoma (HNSCCs)1 are thought to progress through a series of genetic alterations (4). These single DNA alterations (e.g. loss of heterozygosity and microsatellite instability (5), p16 (6), p53 (7, 8), telomerase reactivation (912), and Stat3 (13)) were investigated in detail in the last 10 years for a better understanding of molecular processes, but with low benefit to a better diagnosis or therapy (14). Therefore, highly parallel genomic and proteomic techniques now have to be applied to give a more detailed insight into the complex genesis and progression of HNSCC as well as to identify new cancer-specific signatures.
Such an arising technique is the surface-enhanced laser desorption/ionization (SELDI) mass spectrometry (MS)-based ProteinChip technology (1517). First described by Hutchens and Yip (18), it utilizes affinity surfaces to retain proteins based on their physico-chemical characteristics, followed by direct analysis by time of flight (TOF)-MS. Proteins being retained on a chromatographic surface can be easily purified from contaminants such as buffer salts or detergents prior to MS analysis, thus eliminating the need for preseparation techniques. Furthermore, the low sample requirements of this technique are ideal for small biopsies or microdissected tissue used to produce homogenous tissue samples in cancer research (1921). Today, it is indisputable that microdissected tissue material, free of contaminating, unwanted tissue components, is extremely important to find reliable biomarkers for cancer diagnosis (22). In the case of epithelial tumors, the epithelial cells have to be separated from all surrounding tissue constituents. Because in normal tissue the lining epithelium consists only of one or few cell rows, and in tumor tissues the boundaries to normal pharyngeal tissue are irregular, this can only be done with an extremely precise technique such as laser-based microdissection. Its compatibility with ProteinChip technology has been shown in different small studies (16, 20, 21, 23). Up to now no studies with a statistically relevant number of cases have been performed, nor were differentially expressed proteins identified after microdissection.
When specific alterations between the protein profile of microdissected tumor and normal pharyngeal epithelium tissue are found by ProteinChip technology, single peaks can be isolated and identified. For the isolation, different techniques are in use. As well as the two-dimensional gel electrophoresis (2-DE) (24) applied in this study, the ProteinChip system can also be used for the on-spot development of purification protocols and the monitoring of the subsequent purification process (25). In either case, the isolated protein is digested by enzymatic cleavage. Subsequently, the mass values of the generated fragments are used for peptide mapping to identify the protein of interest by data base searches. Furthermore, for unambiguous identification selected peptides can be sequenced by collision-induced dissociation (CID) using a ProteinChip interface coupled to a tandem mass spectrometer (26, 27).
In the study presented here, pure microdissected populations of normal pharyngeal epithelium and tumor squamous epithelial cells were analyzed on ProteinChip arrays. One differentially expressed peak showed a calculated mass (m/z value) of 35.90 kDa. Protein extracts of the same specimens were prepared and analyzed by 2-DE. Differentially expressed spots showing an appropriate mass were cut out of the second dimension gels and identified by in-gel digestion, peptide mapping, and tandem mass spectrometry (MS/MS) as human annexin V. The assumption that annexin V is identical to the differentially expressed peak found by ProteinChip analysis was confirmed with an immuno-deplete assay. The localization of annexin V in tissue was subsequently verified on cryostat sections of the HNSCCs by immunohistochemistry using a monoclonal anti-annexin V antibody. Positive tissue areas were microdissected in corresponding unstained sections and re-analyzed on ProteinChip arrays to show that annexin is matching to the differentially expressed peak found in the prior analysis.
Therefore, as shown for the first time on a high number of cases, combinatorial use of laser microdissection of tumorous tissue, ProteinChip technology, and immunohistochemistry show promise to find, isolate, and identify cancer-associated markers.
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EXPERIMENTAL PROCEDURES |
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Laser Microdissection of Tissue Sections
For the microdissection procedure, native air-dried cryostat tissue sections (8 µm thickness) on microscope slides coated with a 1.35-µm membrane (polyethylene naphtalate; Palm, Bernried, Germany) and a laser microdissection and pressure catapulting microscope (LMPC; Palm) were used. Tumor cell areas and normal pharyngeal epithelium were located in comparison with a hematoxylin and eosin (HE)-stained serial section, marked and cut out by a pathologist (Fig. 1). Stained sections revealed no or poor protein profile (data not shown).
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ProteinChip Array Preparation and Analysis
The protein lysates from microdissected HNSCC tissue were analyzed on a strong anionic exchanger array (SAX2; Ciphergen Biosystems, Fremont, CA). First, sample targets on the arrays were equilibrated three times by applying 5 µl binding/washing buffer (100 mM Tris buffer, pH 8.5, containing 0.05% Triton X-100) for 20 min, respectively. After equilibration, the buffer was removed and 5 µl fresh buffer was added to each spot. Into this, 2 µl of sample extract was spiked and the ProteinChip array was incubated in a humidity chamber for 90 min at 20 °C. Afterward, sample droplets were removed and each target was washed three times with 5 µl binding/washing buffer. The targets were then washed two times with 5 µl water to remove the buffer salts and subsequently dried on air. After application of 2x 0.5 µl saturated sinapinic acid (Sigma) dissolved in 50% acetonitrile (Sigma) containing 0.5% trifluoroacetic acid (Sigma), mass analysis was performed in a ProteinChip Reader (PBS-II; Ciphergen Biosystems) according to an automated data collection protocol. This includes an average of 195 laser shots to each spot with a laser intensity of 200 and 270, respectively, dependent on measured region (low = 220 kDa and high = 20200 kDa, respectively). The detector was run at a sensitivity of 9. Normalization of all spectra was performed using total ion current. Cluster analysis of the detected signals and the determination of respective p values were carried out with the Biomarker Wizard Program (Version 3.0; Ciphergen Biosystems). For p value calculation, spectra with at least 10 signals in the range between 2 kDa and 20 kDa exhibiting a signal-to-noise ratio of at least 5 were selected and analyzed with the Mann-Whitney U test for non-parametric data sets.
Two-dimensional Gel Electrophoresis
Samples for 2-DE were prepared directly from surgical material of ProteinChip system-analyzed HNSCC and corresponding normal tissue. A piece of tissue (about 3 mm3) was minced with a lancet and was then homogenized in liquid nitrogen with a mortar. The obtained powder was dissolved in ice-cold lysis buffer (100 mM sodium-phosphate, pH 7.5, 5 mM EDTA, 2 mM MgCl2, 3 mM 2-ß-mercaptoethanol, 0.1% CHAPS, 500 µM leupetin, and 0.1 mM PMSF) and was further mechanically homogenized by means in a douncer (Roth, Karlsruhe, Germany). Tissue homogenate was centrifuged (15 min at 15,000 rpm), and protein concentrations in the supernatant were measured using the Coomassie Plus protein assay reagent (Pierce) according to the manufacturers instructions. Isoelectric focusing (IEF) was carried out using the PROTEAN IEF Cell (Bio-Rad). For analytical 2-DE, 50 µg of total protein, and for semi-preparative 2-DE, 250 µg of total protein were precipitated using standard methods (28). The protein pellet was resuspended in IEF-lysis buffer (8 M urea, 4% (w/v) CHAPS, 0.25% (w/v) Bio-Lytes 3/10 (Bio-Rad), 65 mM dithiothreitol (DTT), and 10 mM Tris base) using a thermomixer (60 min, 20 °C, 800 rpm). After addition of 250 µl of IEF-buffer (8 M urea, 2.4 M thiourea, 4% (w/v) CHAPS, 0.4% (w/v) Bio-Lytes 3/10 (Bio-Rad), and 65 mM DTT) and 0.5 µl of 1% bromphenol blue in 50 mM Tris, the mixture was again incubated on a thermomixer (60 min, 20 °C, 800 rpm). The supernatant recovered by centrifugation (30 min; 20 °C; 16,100 rpm) was used for IEF. IEF was performed on 17-cm immobilized pH gradient strips (pH 310 or pH 58, respectively). Strips were covered with mineral oil during all steps. IEF was carried out at a constant temperature of 20 °C. IPG strips were rehydrated for 16 h at 50 V. After prefocusing (200 V, 2 h; 400 V, 2 h; 600 V, 2 h; 1000 V, 2 h; 2000 V, 2 h), focusing was done at 3,500 to 60000 Vh. Thereafter, strips were shortly rinsed with water and stored at -20 °C. IPG strips were thawed and incubated at room temperature for 2x 10 min in equilibration buffer (6 M urea, 0.375 M Tris-HCl, pH 8.8, 2% SDS, and 20% glycerol) containing 2% (w/v) DTT followed by incubation (2x 10 min) in the same buffer containing 2.5% (w/v) iodoacetamide instead of DTT. Vertical SDS-PAGE was carried out in a cooled PROTEAN II Multi Cell (Bio-Rad). Linear gradient gels with total acrylamide concentrations ranging from 7 to 20% were used. Protein transfer from agarose-embedded IPG strips to the second dimension gels was performed at 50 V for 30 min. Current was then increased to 100 V for 1 h, and protein separation was carried out at 300 V for 5 h. Analytical gels were silver stained using the Vorum protocol (29), and semipreparative gels were stained with Coomassie brilliant blue G-250.
In-gel Digestion
Protein patterns of the two-dimensional gels from normal pharyngeal epithelium and tumor tissue were compared, and consistent differentially expressed proteins with a size of 35 kDa were excised manually by a scalpel and transferred into a 1.5-ml reaction tube. Excised gel pieces were treated twice with 400 µl of 50% methanol containing 10% acetic acid and agitation for 45 min; followed by incubation in 400 µl of a buffer containing 100 mM ammonium bicarbonate (pH 8.0) with agitation for 30 min; followed by incubation in 400 µl of 50% acetonitrile containing 100 mM ammonium bicarbonate with agitation for 1 h; and finally by incubation in 50 µl 100% acetonitrile with agitation for 15 min. Afterward, gel pieces were centrifuged in a SpeedVac (Savant) to complete dryness. For rehydration and digestion, individual gel pieces were covered with 10 µl of a trypsin solution (0.04 µg/µl; Roche) for 10 min followed by the addition of up to 20 µl 25 mM ammonium bicarbonate and incubated at 37 °C for 7 h. Digested samples were centrifuged for 1 min at 13,000 rpm, and 3 µl of the supernatants were applied directly on spots of a ProteinChip array with a hydrophobic surface (H4; Ciphergen Biosystems), which was preactivated with 30% acetonitrile containing 100 mM NaCl. After samples were dried, spots were covered twice with 0.5 µl of 20%
-cyano-4-hydroxy cinnamic acid (Ciphergen Biosystems) in 50% acetonitrile containing 0.5% trifluoroacetic acid. Peptide fragment masses were analyzed with an average of 110 laser shots to each spot with a laser intensity of 180 and a sensitivity of 10 using the PBS II instrument. A standard protein mix (all-in-1 peptide standard mix; Ciphergen Biosystems), including Arg8-vasopressin (1082.2 Da), somatostatin (1637.9 Da), dynorphin (2147.5 Da), ACTH (2933.5 Da), and insulin beta-chain (3495.94 Da) was used for calibration. Proteins were identified using the fragment masses generated through trypsin digestion by searching in a publicly available data base (129.85.19.192/profound_bin/WebProFound.exe). The criteria for positive identification of proteins were as follows: 1) probability index should be 1.0e+000; 2) Z score for the protein should be greater than 1.65 (
95% percentile); 3) molecular mass and isoelectric point of identified proteins should match estimated values obtained from 2-DE.
Tandem Mass Spectrometry
MS/MS data were acquired on a Micromass QTOFTM II (Manchester, UK) tandem quadrupole-TOF mass spectrometer equipped with a Ciphergen PCI 1000 ProteinChip array interface. Ions were created using a pulsed nitrogen laser operated at 30 pulses per second. Nitrogen gas, at 18 mtorr, was used for collisional cooling of formed ions, and argon gas was used for all low-energy CID experiments. Applied collision energy usually followed the rule of 50eV/kDa. The system was externally calibrated in MS/MS mode using the parent ion and selected fragments of ACTH human fragment 1839 (m/z = 2465.1983). MS/MS spectra were exported as Sequest files and used for data base searches with MASCOT (www.matrixscience.com) using NCBI and SwissProt data bases.
Immuno-deplete Assay
Two microliters of anti-human annexin V monoclonal antibody (Vac-; Bender MedSystems, Vienna, Austria) were incubated with 10 µl protein A-agarose (Sigma) for 15 min on ice. A pellet was generated by centrifugation, and the supernatant was discarded. The pellet was washed two times with a buffer containing 20 mM Hepes, pH 7.8, 25 mM KCl, 5 mM MgCl2, 0.1 mM EDTA, and 0.05% Nonidet P-40. Afterward, 5 µl of a lysate from laser-dissected tumor were incubated with this pellet for 45 min on ice. As a negative control, 5 µl of the lysate were incubated with protein A-agarose without antibody for 45 min on ice. After incubation, samples were cleared by centrifugation, and 3 µl of each supernatant were analyzed by ProteinChip arrays.
Immunohistochemistry
Eight micrometers cryostat sections of frozen head and neck cancer tissue containing both normal pharyngeal epithelium as well as and head and neck cancer cells placed on charged slides, dried for 60 min at 20 °C followed by fixation in 2% paraformaldehyde containing 0.1 M cacodylate buffer, pH 7.2 (Fluka) for 25 min at 20 °C. After fixation slides were rinsed twice with aqua dest and then treated with 10% methanol in Tris-buffered saline (TBS) containing 1% H2O2 for 30 min to inhibit endogenous peroxidatic activity. They were subsequently rinsed twice in TBS, and incubated with monoclonal antibody anti-annexin V (Vac-
; Bender MedSystems), diluted 1:500 in 10% fish gelatin in TBS containing 10% Triton X-100 overnight. Slides were rinsed 3x 10 min in TBS and the Vectastain Elite ABC kit (Vector Laboratories, Burlingame, CA) and 3,3'-diaminobenzidine. Jenchrom pxbl-kit (MoBiTec, Göttingen, Germany) was used according manufacturers instructions to visualize antibody localization. Negative controls were incubated only with the labeled secondary antibody provided in the ABC kit. Sections cut in parallel to the immunohistochemistry (IHC)-treated sections were stained by HE for identification of different tissue areas. IHC staining was evaluated by a pathologist and an anatomist.
Laser Scanning Microscopy
The laser scanning microscopy was performed with a LSM 310 (Carl Zeiss, Oberkochen-Jena, Germany), preferably in the transmission mode using an argon ion laser at 488 nm wavelength. In most cases, Zeiss objective Plan-NEO FLUAR 40x/1.30 Oil was employed at a scanning time of 60 s. The non-processed gray values of the typical transmission images were converted to inverted values and then further processed to obtain red-green-blue images out of 3x 28 color values. The chosen false color table was stored as a LUT (Look Up Table) and finally saved as a TIFF file (30).
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RESULTS |
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Profiling of Microdissected Normal Pharyngeal Epithelium and Tumor Tissue
All protein lysates from the microdissected tissues were applied to strong anionic exchanger arrays and analyzed on a PBS-II system. The arrays were run with two different laser intensities to achieve better resolution for low (220 kDa) and high molecular mass (20100 kDa) proteins. In the low range up to 96 peaks and in high range up to 57 protein peaks (signal-to-noise = 3) were detected with normalized intensities. In the high range 47 tumor and 41 normal tissue lysate resulted in profiles that could be evaluated. For p value calculation, 21 tumor and 22 normal samples were selected according to the criteria given above. An in-tumor up-regulated signal at 35.9 kDa was one out of four peaks with extremely low p values of < 0.0001. This one was selected for further characterization and identification (Fig. 2). First, we used the TagIdent tool from ExPASsy (www.expasy.ch/tools/tagident) by entering the mass of this unknown protein. This tool searches for proteins similar in size and in isoelectric point in the SWISS-Prot and TrEMBL data bases, which can give some indication about possible candidates. The highest score yielded annexin V (accession number P08758).
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In the squamous cell carcinoma, clear immune reactivity could be seen in the periphery of the invasive growing regions (Fig. 6A). In the inner parts, only weak labeling could be detected (Fig. 6A). The normal cells of the squamous and ciliated epithelium of the pharynx showed no reactivity, with the exception of sporadic basal cells. Also, in the fibroblasts of the connective tissue as well as in collagen fibers infrequent expression of annexin V could be detected (Fig. 6, A and C). A strong labeling could be found in the epithelia of the mucous glands (data not shown). Inside the cells, annexin V is localized in the cytoplasma (Fig. 6, BD).
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DISCUSSION |
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One of the most promising proteomic tools for the detection of new cancer biomarkers is the ProteinChip technology (e.g. Refs. 32 and 33). Until now, this technique has been preferentially used for body fluid analyses, because they are fast and easy to perform by direct application on the ProteinChip arrays. Nevertheless, it is known that intra-individual changes in serum are high. For instance, sex, hormone level, nutrition state, and inflammation can strongly change the protein profile. Hence, biomarkers responsible for the genesis and progression of cancer must be present at a high level to be observed above normal changes. Despite these concerns, a high number of studies using body fluids as starting material were published (serum (32, 34); urine (35); nipple aspirate fluid (36); pancreatic juice (33)). If markers, however, can be found, they would be ideal for screening in high-risk individuals or even in individuals without elevated risk.
The analysis of tissues is more time consuming because here microdissection is indispensable to separate tumorous from healthy cells, but the chance to find a reliable tumor marker might be higher than in serum. Microdissection, however, has to be done with an extremely precise technique like LMCP, because in the case of normal tissue the lining epithelium consists only of one or a few cell rows and boundaries between tumor tissue and normal tissue are irregular.
To our knowledge, only six small studies combining microdissection and ProteinChip technology are published up to now. This might be due to the fact that laser-based microdissection is tedious and has to be done by an experienced pathologist. Another reason for this low amount of studies may be that up to now the microdissection for ProteinChip system analyses should be carried out on unstained tissue sections for optimal results, where single constituents are hard to recognize and to differentiate. The first study by Wright and coworkers in 1999 (16) used the combination of microdissection and ProteinChip technology to procure defined pure cells from prostate cancer in order to find biomarkers and to develop a clinical assay. In a review article, Paweletz (37) stated that as few as 25 cells are sufficient for the establishment of reproducible protein profiles. In our former investigations published in 2000 and 2001 (20, 21), we worked with a fine glass needle attached to a joystick-controlled electric micromanipulator. Normal epithelia to melanoma and cervical intraepithelial neoplasias to cervix uteri carcinoma were compared. In both studies, at least 5001000 cells were necessary to obtain a reproducible profile. This finding was also affirmed by Wellman (38) and coworkers, who laser-microdissected stroma, epithelium, and tumor cells of the prostate to decipher the epithelial-mesenchymal cross talk. Cazares and coworkers (23) looked for early protein alterations by comparing normal, benign, preneoplastic, and malignant prostate cells. For nine prostatectomy specimens, they could clearly show that proteins were differentially regulated in the different disease states.
For the analysis of proteins from tumor tissue, two problems have to be solved: first, the tissue heterogeneity of samples, and second, the heterogeneity of the tumor itself. Only the first could be solved by LMPC by dividing e.g. epithelial tissue from connective tissue. The tumor heterogeneity concerning the transscriptome and the proteome is morphologically hard to recognize and cannot therefore be completely solved by microdissection.
After a significant protein has been detected by profiling experiments with ProteinChip arrays, two additional questions have to be addressed. First, how the protein can be enriched and identified, and second, whether this identified protein can be found in the starting tissue and where the protein is exactly localized.
In our study, we addressed the first question by detecting differentially expressed proteins in microdissected tissue by ProteinChip technology and subsequently enriched and identified the protein of interest by 2-DE, in-gel digestion, peptide mapping, MS/MS, and immuno-deplete assay. As a first approach, after profiling the obtained masses of the intact protein can be used for data base search. This will give some indication about possible candidates, and in our case the later-identified annexin V was on the candidate list. 2-DE allowed us to enrich and isolate putative candidates and to digest them with trypsin. The generated peptides could then be analyzed again on the PBS II ProteinChip Reader, and a data base search pointed with a high probability to annexin V. To validate that digested protein isolated from two-dimensional gels is identical to the differentially expressed peak found with ProteinChip array, an immuno-depletion assay was performed with the same starting material and an annexin V antibody. In the analyzed supernatant, the peak at 35.90 kDa was missing and must therefore be depleted by the antibody. The identification was further confirmed by sequencing of selected peptides with MS/MS, a powerful but yet not widespread technique. The second question about the localization of annexin V in tissue was then addressed by IHC. Annexin V could be found in different normal and tumor tissue components. Here as well in the re-analysis of annexin V-positive and -negative tissue areas on chip confirmed its identity to the differentially expressed peak at 35.90 kDa. In normal pharyngeal epithelium, annexin V shows the highest abundance in secretory cells of mucous glands that were excluded by microdissection. In carcinoma, it is exclusively expressed in the periphery of the invasively growing tumor areas. Therefore, annexin V might be connected to proliferation and/or cell mobility and could possess metastatic potential. For annexin I and annexin II, it was shown that their expression is associated to metastatic head and neck cell lines by using 2-DE (9).
An already described function of annexin V is the masking of phosphatidylserine on the outer cell membrane, protecting apoptotic cells from phagocytosis. The binding to phosphatidylserine is widely used for the detection of apoptotic cell (39). The localization of the immune reactivity in the periphery of invasive tumor areas does not support this function here. Annexin V belongs to a multigene family with at least 10 unique genes in mammals, but also homologues exist in Drosophila, Candida elegans, Hydra, Dictostelium, and several plant species (40, 41). Annexin V was first described in chick cartilage cells as anchorin CII (42). Annexin V shows the typical annexin structure consisting of the so called annexin core and the unique N-terminal domain. The annexin core is made up by four highly similar structural elements each containing five -helices connected by short loops. This five-helix motif contains the typical calcium and phospholipid binding site of the annexins. The annexin core has also been proposed to form a pore that upon binding of the annexin molecule to the plasma membrane could serve as a calcium channel (43). Besides this and its function as a collagen receptor, several other characteristics have been described (44) that cannot help to explain the immunohistochemical data of this study.
Annexin V cannot be seen as a relevant marker for the whole tumor, but for clonal cell populations of tumor it seems to be characteristic for the invasively growing tumor cells. Furthermore, the results stand for a paradigm of how to discover and identify potential tumor markers. The localization of annexin V shown with IHC is also an interesting hint to a previously unknown biological background of annexin V. Therefore, further tumor entities have to be analyzed for the relevance of this protein.
In conclusion, it can be stated that a better estimation of the biological importance of certain cell populations in regard to the progression from preneoplastic tissue alterations to malignant tumors and the prediction of the metastasis-forming potential of a given cell population by biomarkers will be necessary prerequisites for providing a more detailed insight and understanding of tumor progression. The SELDI-based ProteinChip technology in combination with microdissection and IHC opens up this possibility while reducing the complexity of the proteome by using a defined cell population and therefore allowing a better and earlier cancer diagnosis in future.
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FOOTNOTES |
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Published, MCP Papers in Press, June 23, 2003, DOI 10.1074/mcp.M300033-MCP200
1 The abbreviations used are: HNSCC, head and neck squamous cell carcinoma; 2-DE, two-dimensional protein gel electrophoresis; CID, collision-induced dissociation; HE, hematoxylin and eosin; IHC, immunohistochemistry; LMPC, laser microdissection and pressure catapulting microscope; SELDI, surface enhanced laser desorption ionization; TOF, time-of-flight, MS, mass spectrometry; MS/MS, tandem mass spectrometry; IEF, isoelectric focusing.
* This work was support by a grant of the German Federal Ministry of Education and Research and the Interdisciplinary Center for Clinical Research, Jena, Germany. The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Institut für Humangenetik und Anthropologie, CUCA, 07740 Jena, Germany. Tel.: 0049(0)3641-935526; Fax: 0049(0)3641-935582; E-mail: fegg{at}mti.uni-jena.de
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REFERENCES |
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