Abstract
The aim of this study was to identify biomarkers for gastric cancer (GC) by iTRAQ. Using proteins extracted from a panel of 4 pairs of gastric adenocarcinoma samples (stage III-IV, Her-2 negative), we identified 10 up regulated and 9 down regulated proteins in all four pairs of GC samples compared to adjacent normal gastric tissue. The up regulated proteins are mainly involved in cell motility, while the down regulated proteins are mitochondrial enzymes involved in energy metabolism. The expression of three up regulated proteins (ANXA1, NNMT, fibulin-5) and one of the down regulated proteins (UQCRC1) was validated by Western Blot in 97 GC samples. ANXA1 was up regulated in 61.36% of stage I/II GC samples compared to matched adjacent normal gastric tissue, and its expression increased further in stage III/IV samples. Knockdown of ANXA1 by siRNA significantly inhibited GC cell migration and invasion, whereas over expression of ANXA1 promoted migration and invasion. We found decreased expression of UQCRC1 in all stages of GC samples. Our data suggest that increased cell motility and decreased mitochondrial energy metabolism are important hallmarks during the development of GC.
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Introduction
Gastric cancer is a serious threat to public health worldwide. It was estimated that about 10,000 Americans will die from gastric cancer in 20161. Although stage I GC may be curable by surgery alone, many patients with advanced GCs die due to recurrence of the disease after initial tumor resection and failure to response to subsequent chemotherapy2,3. Chemotherapy failure results from genetic mutations, epigenetic alterations of DNA and post-translational modification of proteins. These changes result in aberrant expression of certain proteins, which leads to altered cellular metabolism, proliferation and metastatic potential. In order to improve outcomes, it is crucial to identify proteins that can be used as markers for early diagnosis and treatment. Several biomarkers, including Her-24, EGFR5, VEGF6, and HGF/MET7, have been identified in the past. Among these markers, only Her-2 inhibition has led to clinical benefit4. However, only 8–18% of GC tumors are Her-2 positive8,9. Therefore, a new comprehensive molecular classification from proteomic study on Her-2 negative GCs may bring new therapeutic strategies into clinical practice in the near future.
iTRAQ (isobaric tags for relative and absolute quantitation) is one of the new techniques used in modern proteomics that couples stable isotopes labeling and tandem mass spectrometry to compare the relative amount of proteins from normal and diseased samples in a single experiment. iTRAQ-based quantitative proteomics have revealed myoferlin as a novel prognostic predictor in pancreatic adenocarcinoma10. This present study utilized the iTRAQ approach to profile the differentially expressed proteins in Her-2 negative stage III–IV human gastric adenocarcinoma. We performed Gene Ontology (GO) and pathway analyses in order to explore the role of dysregulated proteins in tumor progression. Selected differentially expressed proteins were validated by Western Blot and immunofluorecence staining. We also performed migration and invasion experiments using a human gastric cancer line in order to exam the role of these proteins in tumor metastasis.
Results
Detection and quantification of proteins in gastric cancer
Four pairs of gastric adenocarcinoma samples (stage III-IV, Her-2 negative) were used for this study to identify differentially expressed proteins involved in the development and progression of gastric cancer (Table 1). Both tumor (A) and adjacent normal gastric tissue (B) were taken from each patient during surgical resection. Proteins from samples 31A, 31B, 10A, 10B, 5A, 5B, 101A, 101B were labeled with ITRAQ reagents 113,114,115,116,117,118,119,121, respectively. Thus, the ratio of labels 113 and 114 would indicate the relative abundance of proteins from sample 31A/31B, etc. Data was analyzed by Protein Pilot Software v. 5.0 (AB SCIEX, USA) using the Paragon algorithm based on Homo sapiens data base11. An automatic decoy database search strategy was used to determine the false discovery rate (FDR) using the Proteomics System Performance Evaluation Pipeline Software (PSPEP). The FDR was calculated as the false positive matches divided by the total matches. A total of 3245 proteins with the value of global FDR from fit less than 1% were detected. In order to reduce false positives, we included an additional 1.3-fold and a 0.77-fold cutoff for up or down regulated proteins, respectively. Based on this selection, 120 proteins were found differentially expressed in the gastric tumors compared to their adjacent normal gastric tissues. Nineteen proteins were selected for further analysis because these proteins are either up or down regulated in all 4 pairs of samples (Tables 2 and 3).
Classification of differentially expressed proteins
The functional classification of the 19 proteins was cataloged according to biological processes (BPs), molecular functions (MFs), and cellular components (CCs) according to the GO database. The proteins under the category of BPs are involved in tricarboxylic acid cycle (15%), isocitrate metabolic process (10%), response to activity (10%), small molecule metabolic process (42%), and oxidation reduction process (10%). The proteins under the category of MFs are involved in calcium ion binding (31%), NAD binding (10%), integrin binding (10%), and protein complex binding (10%). The proteins under the category of CCs were classified as mitochondrial respiratory chain (10%), mitochondrial inner membrane (26%), mitochondrial matrix (20%), extracellular matrix (15%), extracellular vesicular exosome (10%), proteinaceous extracellular matrix (15%), and neuromuscular junction (10%).
The differentially expressed proteins were mapped to KEGG pathways based on their gene ID. The up regulated proteins are involved in the following pathways: malaria, nicotinate and nicotinamide metabolism, salmonella infection, ECM-receptor interaction, tight junction, phagosome, Alzheimer’s disease, focal adhesion, regulation of actin cytoskeleton, PI3K-Akt signaling pathway and metabolic pathways (Fig. 1). The down regulated proteins are involved in the following pathways: 2-oxocarboxylate acid metabolism, glyoxylate and dicarboxylate metabolism, butanoate metabolism, citrate cycle, carbon metabolism, tryptophan metabolism, valine leucine and isoleucine degradation, fatty acid degradation, fatty acid metabolism, lysine degradation, synthesis and degradation of ketone bodies, biosynthesis of amino acids, terpenoid backbone biosynthesis, fatty acid elongation, nicotinate and nicotinamide metabolism, propanoate metabolism, metabolic pathways, Parkinson’s disease, oxidative phosphorylation, African trypanosomiasis, non-alcoholic fatty liver disease, pyruvate metabolism, Alzheimer’s disease, malaria, glutathione metabolism, Huntington’s disease, cardiac muscle contraction and peroxisome (Fig. 2).
Figure 3 shows a network of interactions among the 19 proteins using the String data base (http://string-db.org), which is helpful in dissecting out groups of proteins involved in a particular pathway. For example, it is obvious from the network that myosin-9 (MYH9), plastin-3 (PLS3) and transgelin-2 (TAGLN2) are linked together because all of the three proteins are involved in actin binding and cell motility. Previous studies showed that MYH9 promotes cancer cell migration and invasion and were up regulated in non-small cell lung cancer (NSCLC)12 and esophageal squamous cell carcinoma (ESCC)13. PLS3 has been identified as a novel marker for circulating tumor cells in colorectal cancer (CRC)14. Over expression of PLS3 induced epithelial mesenchymal transition in CRC, which showed enhanced migration and invasion ability14. MYH9 and PLS3 have never been implicated in gastric cancer. TAGLN2 promote tumor cell migration and invasion15 and is highly expressed in human pancreatic cancer16 and gastric cancer17.
Among the down regulated proteins, 7 of 9 (77.7%) proteins are located within mitochondria (Table 3), which are interconnected as shown in Fig. 3. All of these proteins are enzymes involved in energy metabolism.
Mitochondrial dysfunction and deregulated cellular energy metabolism is one of the hallmarks during cancer development. Deregulated energy metabolism can be caused by either mitochondrial DNA mutations or mitochondrial enzyme defects, which could result in altered signal transduction pathways that eventually modify gene expression. Indeed, our results show that isocitrate dehydrogenase (IDH2), an enzyme in the citric acid cycle, is down regulated in advanced gastric cancer. The main function of IDH2 is to catalyze the oxidative decarboxylation of isocitrate into alpha-ketoglutarate. Defect in IDH2 can cause accumulation of 2-hydroxyglutarate, which renders cells more accommodating for epigenetic modification and potential transformation due to DNA hypermethylation18,19,20,21. IDH2 has been considered a tumor suppressor because its loss was associated with progression of GC via NF-κB-dependent increases in MMP7 activity22.
ACO2 is another enzyme of the citric acid cycle that is down regulated in stage III/IV gastric cancer (Table 3). Our results are consistent with a previous report that expression of ACO2 was significantly down-regulated in gastric cancer tissues compared with matched adjacent cancer tissues, and reduced expression of ACO2 was associated with clinical stage and pathological differentiation states23.
Our data revealed the down regulation of three proteins involved in electron transfer and respiration (NNT, NDUFS1, UQCRC1), and two proteins involved in fatty acid metabolism and ketone body formation (ACAT1, HADH) in stage III/IV GC. NNT is a mitochondrial enzyme that produces NADPH, and this enzyme has not been implicated in cancer so far in the literature. NDUFS1 belongs to the complex I, located at the mitochondrial inner membrane. This protein transfers electrons from NADH to the respiratory chain. NDUFS1 has been identified as candidate gene in ovarian cancer24. UQCRC1 is a component of the cytochrome b-c1 complex (complex III), which is part of the mitochondrial respiratory chain. The expression of UQCRC1 is increased in osteosarcoma cells25. ACAT1 catalyzes the reversible formation of acetoacetyl-CoA from two molecules of acetyl-CoA. It has been shown that ACAT1 expression was significantly greater in prostate cancer compared to normal prostate tissue26. HADH is involved in fatty acid oxidation and has not been implicated in cancer development.
Validation of iTRAQ results on selected proteins
To confirm the iTRAQ results, three up regulated proteins, namely, Nicotinamide -N-methyltransferase (NNMT), Fibulin-5 (FBLN5), Annexin A1 (ANXA1) and one of the down regulated proteins, cytochrome b-c1 complex subunit 1 (UQCRC1) were chosen for further analysis by Western Blot and immunofluorescence assay. The GC samples used for validation comprised 70 males and 27 female (Table 4). Western Blot analysis revealed that NNMT, FBLN5 and ANXA1 are clearly up regulated in stages III-IV GC (Fig. 4Fig. 5 and Fig. 6) compared to stage I-II samples. NNMT, FBLN5 and ANXA1 were up regulated in 45.45%, 47.73%, and 61.36% of stage I/II GC samples, respectively. Our data suggest that ANXA1 is a better marker for early diagnosis of GC.
Because of the contradicting reports in the literature regarding the role of ANXA1 in gastric cancer27,28, we investigated ANXA1 further by examining the expression of ANXA1 on frozen tissue sections by immunofluorescence technique, which confirmed that ANXA1 expression was increased in GC compared to adjacent normal gastric tissue (Fig. 7). In order to investigate the functional role of ANXA1 in GC progression and metastasis, we assessed the impact of ANXA1 knockdown and over expression on gastric cancer cell migration and invasion. Cancer cell migration was assessed using a wound healing assay, which revealed a decreased migration capacity in siRNA-Annexin A1 transfected AGS cells compared to controls (Fig. 8), but increased migration in cells transfected with a plasmid overexpressing Annexin A1 (Fig. 9).
Real-time PCR results confirmed that Annexin A1 mRNA expression was significantly reduced in AGS cells transfected with siRNA (Fig. 10a). whereas its expression was up regulated in cells that were transfected with an expression plasmid carrying Annexin A1 cDNA (Fig. 10b).
We then performed migration and invasion assays using transwell plates. Consistent with the findings from wound healing assay, migration and invasion were inhibited in AGS cells transfected with siRNA specific for ANXA1 (Figs 11 and 12), but increased in cells transfected with an expression plasmid carrying ANXA1 (Figs 13 and 14).
We next validated the expression of UQCRC1 in the above mentioned 97 GC samples. Western Blot analysis revealed that UQCRC1 expression was decreased in all stages of GC samples, compared to adjacent normal gastric tissue (Fig. 15). UQCRC1 expression was decreased in 76.47%, 74.07%, 86.05%, and 70.00% in stages I, II, III, and IV GC samples, respectively. Western Blot data were confirmed by immunofluorecence staining (Fig. 16). Our results suggest that reduced expression of UQCRC1 is associated with tumor progression. The iTRAQ procedures are summarized in Fig. 17.
The images of Western Blot and immunofluorecence staining of all 97 pairs of samples are shown in Supplementary Figures S1 And 2. The specificity of the antibodies was confirmed by blocking the antibodies with their corresponding recombinant proteins. The immunofluorecence staining for ANXA1, NNMT, FBLN5 and UQCRC1 disappeared after the antibodies have been pre-incubated with their corresponding recombinant proteins (Supplementary Fig. S3). Full length blots of Figures 4, 5, 6 and 15 are presented in Supplementary Figure S4.
Discussion
Management of advanced gastric cancer remains a major challenge in oncology. Response to treatment is often difficult to predict due to the heterogeneity of the disease. A better understanding of tumor biology will lead to the identification of new markers for both early diagnosis and treatment. In the present study, we analyzed protein expression profile in 4 pairs of stage III/IV gastric cancer samples by iTRAQ. We found 19 proteins that are differentially expressed in all 4 pairs of samples. We then selected ANXA1, NNMT, FBLN5 and UQCRC1 for further study. These proteins were chosen because reports on their roles in gastric cancer progression remain controversial.
ANXA1 is a member of a family of calcium and membrane-binding proteins, located on the cytosolic face of plasma membrane29. Previous reports suggest that ANXA1 is involved in membrane aggregation, cell matrix interaction, vesicle transport, phagocytosis, proliferation, apoptosis, inflammation and cell transformation29. ANXA1 expression is up-regulated in breast cancer30, hepatocellular carcinoma31, melanoma32, and rectal cancer, but down regulated in nasopharyngeal carcinoma33 and cervical cancer34. In breast cancer, ANXA1 expression is associated with BRCA1/2 mutations35. Similarly, high ANXA1 expression correlated with advanced TNM stage and poor survival of human hepatocellular carcinoma (HCC) patients31. It has been shown that ANXA1 expressing cancer cells are resistant to chemo- and radiation therapy because these cells acquired cancer stem cell like features36,37. However, the role of ANXA1 in gastric cancer has not been established27,28. Gao et al. showed profound ANXA1 expression in normal gastric mucosa and glands, but reduced expression in poorly differentiated gastric tumors27. Another study from the same group of investigators also showed that ANXA1 expression decreased significantly as gastric cancer progressed and metastasized38. Results from these two studies suggest that ANXA1 is a tumor suppressor. By contrast, Sato et al. did not detect ANXA1 in normal gastric mucosa, but found ANXA1 expression in 56.3% cases of gastric cancer28. Our data demonstrated that ANXA1 is indeed over–expressed in gastric cancer, but expressed at low levels in normal gastric tissue. We further showed that ANXA1 knockdown inhibited AGS cell migration and invasion. These data suggest that ANXA1 overexpression in gastric cancer is involved in tumor progression.
NNMT catalyzes the N-methylation of nicotinamide and other pyridines to form pyridinium ions. This enzyme plays an important role in biotransformation of many drugs and xenobiotic compounds in liver. Using two dimensional gel electrophoresis techniques, it was shown that NNMT was over expressed in gastric tumor compared to normal gastric tissues39. Another study showed that NNMT expression is associated with poor prognosis40. These are the only two reports that we could find in the literature regarding the involvement of NNMT in gastric cancer. Our findings that NNMT is over expressed in GC are consistent with these previous reports. However, the mechanisms whereby NNMT promotes tumor progression remain poorly understood. Potential mechanisms include activation of Akt signaling41, anti-apoptosis42 and activation of matrix metalloproteinase-243. NNMT over expression could also impair the methylation potential of cancer cells, resulting hypomethylated histones and increased expression of oncogenes44.
FBLN5 is a secreted extracellular matrix protein that plays a critical role in the assembly of elastic fibers. Using immunohistochemistry technique, Hwang et al. found high expression of FBLN5 in 48 of 84 nasopharyngeal carcinoma (NPC) samples and FBLN5 expression correlated with advanced tumor stage. They further showed that overexpxression of FBLN5 in NPC cells promote cell migration and invasion through activation of phospho-Akt45. There is only one report showing over expression of FBLN5 in gastric cancer46. In that study, FBLN5 protein expression correlated with poor differentiation and advanced TNM tumor stage. These data are consistent with our findings that FBLN5 expression is higher in stage III/IV gastric cancer samples, suggesting an important role of FBLN5 expression in cancer progression. However, the mRNA and protein expression of FBLN5 were down-regulated in ovarian carcinomas compared with control tissues47. Over expression of FBLN5 in ovarian cancer line SKOV3 inhibited migration and invasion in wound-healing and invasion assays. Over expression of FBLN5 in SKOV3 cells also induced G2/M arrest and increased cyclin B1, CDC2 and CDC25C47. Therefore, FBLN5 acts as a tumor suppressor in ovarian cancer. Similarly, FBLN5 over expression inhibited invasion and proliferation capacity of several breast cancer lines including MCF-7, T47D and MDA-MB-23148. Interestingly, FBLN5 also prevent these cells from forming mammospheres, a key feature of cancer stem cells48. Thus, depending on tumor type, FBLN5 may either promote or inhibit tumor growth through mechanisms that are not totally understood.
UQCRC1 is a component of complex III of mitochondrial respiratory chain. Liu et al. compared osteosarcoma cells and human primary cultured osteoblastic cells by two-dimensional gel electrophoresis and identified UQCRC1 as one of the proteins that were up regulated in osteosarcoma cells25. Kulawiec et al. analyzed the expression of UQCRC1 gene in breast and ovarian tumors and found that 74% of breast carcinomas cases were positive for UQCRC1, with positive correlation to tumor grade49. By contrast, only 34% ovarian adeno-carcinomas cases showed UQCRC1 expression, with a negative correlation to tumor grades49. Feng et al. investigated protein profile of human hepatocarcinoma cell line SMMC-7721 by two-dimensional electrophoresis and identified UQCRC1 as one of the novel proteins for hepatocarcinoma cell50. But no control cells were used, therefore, it is not possible to draw any conclusions on whether UQCRC1 was up or down regulated in hepatocarcinoma cells50. Using mass spectrometry, UQCRC1 was identified as one of the three up regulated proteins in the serum from patients with esophageal squamous cell carcinoma and the results suggested that UQCRC1 might be a useful serological marker for this type of cancer51. UQCRC1 is normally located within mitochondria; it is not known how UQCRC1 is released into circulation. Using two-dimensional gel electrophoresis technique, Cai et al. reported down regulation of UQCRC1 in gastric cardia cancer samples and the results were verified by RT-PCR. In our opinion, they should have performed Western Blot to confirm their findings at protein level rather than at mRNA level. Nonetheless, Cai’s findings on UQCRC1 down regulation in gastric cardia cancer samples are consistent with our results in gastric adenocarcinoma. How does UQCRC1 influence tumor progression? Previous studies have shown that deficiency in respiratory complex I activity is associated with overproduction of ROS and high metastatic potential52. Whether UQCRC1 deficiency could lead to ROS overproduction, which in turn promotes GC invasion, remain to be investigated.
In conclusion, our study revealed the role of ANXA1, NNMT, Fibulin-5 and UQCRC1 in gastric cancer progression. Knockdown of ANXA1 by siRNA significantly inhibited GC cell migration and invasion, whereas overexpression of ANXA1 promoted migration and invasion. We also revealed the role of decreased expression of UQCRC1, a mitochondrial enzyme involved in energy metabolism, in GC development. Future studies will clarify how these proteins participate in gastric cancer development and progression.
Materials and Methods
Patient sample collection
All experiments involving human subjects were performed in accordance with the Code of Ethics of the World Medical Association (Declaration of Helsinki), and the relevant guidelines and regulations of Soochow University. All experimental protocols were approved by the Research Ethics Committee of the First Affiliated Hospital of Soochow University. With informed consent from all subjects, paired specimens of gastric adenocarcinoma and adjacent normal tissues were obtained from patients who underwent surgical resection of gastric adenocarcinoma at the Department of General Surgery, First Affiliated Hospital of Soochow University. None of the patients received any anti-cancer treatment before surgery.
iTRAQ
The detailed procedure has been described previously53. Briefly, the protein samples were acetone-TCA precipitated, digested by trypsin to generate proteolytic peptides which were labeled with iTRAQ reagents. The combined peptide mixtures were analyzed by LC-MS/MS for both identification and quantification (Fig. 9). Functional enrichment analysis was performed using Gene Ontology (GO) (http://www.geneontology.org/). Pathway analysis was performed by KEGG mapping (http://www.genome.jp/kegg/).
Western Blot
Proteins extracted from patient’s samples were separated by SDS-PAGE and then transferred to PVDF membrane. After incubating with primary antibodies at 4 °C overnight, the membranes were then washed three times with Tris-buffered saline containing Tween-20 (TBST) and incubated with horseradish peroxidase-conjugated secondary antibodies (anti-rabbit or anti-mouse IgG: 1:4000, Sigma, USA) for 2 h at room temperature. The membranes were then washed again in TBST and visualized using an Enhanced ChemiLuminescence Kit (PerkinElmer). Rabbit anti-Annexin A1 (1/1000) and anti-GAPDH (1/5000) were from Cell Signaling, mouse anti-NNMT was from Santa Cruz Biotechnology (1/500), mouse anti-fibulin-5 (1/500) and rabbit anti- UQCRC1 (1/1000) were from ThermoFisher Scientific. The band density was quantified by ImageJ and normalized to GAPDH.
Immunofluorescence staining
Frozen sections (10 μm) were incubated with Annexin A1 (Cell Signaling Technology), UQCRC1 (ThermoFisher Scientific) antibodies produced in rabbit, NNMT (Santa Cruz Biotechnology), Fibulin-5 (ThermoFisher Scientific) antibodies produced in mouse. After washing, the sections were incubated with goat anti-rabbit IgG - Alexa Fluor® 568 conjugate (Thermo Fisher Scientific), or goat anti-mouse IgG- Alexa Fluor® 488 conjugate, followed by incubation with DAPI to stain nuclei. Images were acquired using a Multiphoton Laser Scanning Microscope (FV1000, Olympus).
Blocking experiments
The antibodies against ANXA1, NNMT, FBLN5 and UQCRC1 were pre-incubated with their corresponding recombinant proteins (antibody/recombinant protein: 1/5, by weight) diluted in blocking buffer (5% non-fat dry milk, 0.1% Tween-20 in TBS) and incubated at room temperature for 4 hours before adding to tissue sections. Recombinant human ANXA1, NNMT, and UQCRC1 proteins were from Abcam, recombinant human FBLN5 protein was from R & D Systems.
Cell line
The human gastric carcinoma cell line AGS was purchased from Cell Bank of the Chinese Academy of Sciences (Shanghai, China), and cultured in Ham’s F-12K (Gibco) containing 10% FBS. The AGS cell line was validated by STR (short tandem repeat) analysis performed by Cell Bank of the Chinese Academy of Sciences (Shanghai, China) and the cells was resuscitated immediately after purchase and was used within 6 passages.
siRNA transfection
For knockdown of Annexin A1, AGS cells were transfected with small interfering RNA (siRNA) targeting Annexin A1. siRNA and negative control (NC) were purchased from GenePharma (Shanghai, China). NC: 5′-UUCUCCGAACGUGUCACGUTT-3′, 5′-ACGUGACACGUUCGGAGAATT-3′AnnexinA1–452: 5′-GCAGCAUAUCUCCAGGAAATT-3′, 5′-UUUCCUGGAGAUAUGCUGCTT-3′, AnnexinA1-743: 5′-GCUUUGCUUUCUCUUGCUATT-3′, 5′-UAGCAAGAGAAAGCAAAGCTT-3′AnnexinA1-1061: 5′-GCCAUGAAAGGUGUUGGAATT-′, 5′-UUCCAACACCUUUCAUGGCTT-3′.
The cells were transfected according to the manufacturer’s instructions. AGS cells were seeded to 6-well plates (1 × 106 cells/well) the night before transfection. The transfection was designed for one RNA amount (A) combined with one amount of Lipofectamine RNAiMAX (B). A. 1.5 μl siRNAs (30 pmol) was added to 150 μl Opti-MEM; B. Lipofectamine RNAiMAX (9 μl, Invitrogen), was added to 150 μl Opti-MEM. A and B was combined and incubated at room temperature for 20 mins. Finally, 250 μl of the mixture was added to each well of the 6-well plates.
Annexin A1 overexpression
Expression plasmids carrying Annexin A1 was purchased from Sino biological Inc (Beijing, China). The plasmid (3 μg) was diluted in 150 μl Opti-MEM which were then mixed with equal volumes of Opti-MEM containing 6 μl Lipofectamine 2000. The mixture was incubated for 20 minutes at room temperature before adding to cells.
Wound-healing assay
Cell migration was evaluated by wound healing assay. Briefly, 1 × 106 AGS cells/well were plated in a 6-well plate and cultured overnight to yield a sub-confluent monolayer. The cells were transfected with Annexin A1 siRNA or plasmid overexpressing Annexin A1, then wounded with a 200 μl pipette tip. The remaining cells were washed with PBS. Photographs were taken at 0 and 24 hours. The distance of the remaining open wound area was calculated as percentage of the area at time 0.
Migration and Invasion assays
Cell invasion was determined using a transwell matrigel invasion assay in 24-well Transwell units (Costar). Matrigel diluted with the precooled serum-free Ham’s F-12K (50 μl) was added to the upper chamber of the Transwell and incubated at 37 °C for 30 minutes. The siRNAs or NC was prepared as described above. Following incubation for 20 minutes, 100 μl of the siRNA mixture was mixed to 100 μl serum-free Ham’s F-12K containing 1 × 105 cells and then transferred to Matrigel coated top chambers. The lower chambers were filled with 500 μl Ham’s F-12K supplemented with 10% FBS. After incubation at 37 °C for 24 hours, the non-invading cells were removed with a cotton swab. The inserts were removed from the top chambers, washed with PBS, fixed and stained with Giemsa. The invaded cells were counted in five random fields under a light microscope. The procedure for cell migration is similar to that of invasion, except that matrigel was not added.
Real-time PCR
RNA was extracted using the Trizol reagent (Ambion), and cDNA was synthesized using the RevertAid First Strand cDNA Synthesis Kit (ThermoFisher Scientific). Real-time PCR was performed using the ABI 7500 Real Time PCR System (ABI) with the following primers: AnnexinA1-F:AAGCAGGAGAAAGGAGAAAGG AnnexinA1-R:AACTCCAGGTCCAGAACTTTG, GAPDH-F:ACCCAGAAGACTGTGGATGG GAPDH-R:CAGTGAGCTTCCCGTTCAG. Relative expression was calculated from cycle threshold (Ct; relative expression = 2−(SΔCt−CΔCt)) values using GAPDH as internal control for each samples.
Statistical analysis
Data were presented as means ± SD. The t-test was used to determine the significance of the differences between two groups for the invasion assay. Mann-whitney test was used to determine the significance for Western Blot experiments for validation of iTRAQ results in 97 stage I-IV gastric cancer samples. P < 0.05 was considered statistically significant.
Additional Information
How to cite this article: Wang, X. et al. Identification of specific biomarkers for gastric adenocarcinoma by ITRAQ proteomic approach. Sci. Rep. 6, 38871; doi: 10.1038/srep38871 (2016).
Publisher's note: Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
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Acknowledgements
This work was supported by the project for the Priority Academic Program Development of Jiangsu Higher Education Institutions.
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X.X.W., Q.M.Z., S.B.L., Z.X.T., Y.H.S. and J.Z. designed the experiments. X.X.W., Q.M.Z., S.B.L., S.L.X., Y.X.L., C.F.W., W.C.C., C.C.S., J.S. and M.Y.B. performed the experiments. X.X.W., Q.M.Z., S.B.L., Z.X.T., Y.X.L.,Y.H.S. and J.Z. analyzed data. X.X.W., Y.H.S. and J.Z. wrote the manuscript. All authors reviewed the manuscript.
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Wang, X., Zhi, Q., Liu, S. et al. Identification of specific biomarkers for gastric adenocarcinoma by ITRAQ proteomic approach. Sci Rep 6, 38871 (2016). https://doi.org/10.1038/srep38871
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DOI: https://doi.org/10.1038/srep38871
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