Screening differentially expressed genes of pancreatic cancer between Mongolian and Han people using bioinformatics technology

Microarray Analysis ◽

Cancer Tissue ◽

Tissue Samples ◽

Abstract Objective: To screen and analyze differentially expressed genes in pancreatic carcinoma tissues taken from Mongolian and Han patients by Affymetrix Genechip. Methods: Pancreatic ductal cell carcinoma tissues were collected from the Mongolian and Han patients undergoing resection in the Second Affiliated Hospital of Nanchang University from March 2015 to May 2018 and the total RNA was extracted. Differentially expressed genes were selected from the total RNA qualified by Nanodrop 2000 and Agilent 2100 using Affymetrix and a cartogram was drawn; The gene ontology (GO) analysis and Pathway analysis were used for the collection and analysis of biological information of these differentially expressed genes. Finally, some differentially expressed genes were verified by real-time PCR. Results: Through the microarray analysis of gene expression, 970 differentially expressed genes were detected by comparing pancreatic cancer tissue samples between Mongolian and Han patients. A total of 257 genes were significantly up-regulated in pancreatic cancer tissue samples in Mongolian patients; while a total of 713 genes were down-regulated. In the Gene Ontology database, 815 differentially expressed genes were identified with clear GO classification, and CPB1 gene showed the highest increase in expression level (multiple difference: 31.76). The pathway analysis detected 28 signaling pathways that included these differentially expressed genes, involving a total of 178 genes. Among these pathways, the enrichment of differentially expressed genes in the FAK signaling pathway was the strongest and COL11A1 gene showed the highest multiple difference (multiple difference: 5.02). The expression of differentially expressed genes CPB1, COL11A1、ITGA4、BIRC3、PAK4、CPA1、CLPS、PIK3CG and HLA-DPA1 determined by real-time PCR were consistent with the results of gene microarray analysis. Conclusions: The results of microarray analysis of gene expression profiles showed that there are a large number of differentially expressed genes in pancreatic cancer tissue samples comparing Mongolian and Han population. These genes are closely related to the cell proliferation, differentiation, invasion, metastasis and multi-drug resistance in pancreatic cancer. They are also involved in the regulation of multiple important signaling pathways in organisms.

Screening differentially expressed genes of pancreatic cancer between Mongolian and Han people using bioinformatics technology

10.21203/rs.2.11118/v5 ◽

2020 ◽

Author(s):

Jiasheng Xu ◽

Kaili Liao ◽

ZHONGHUA FU ◽

ZHENFANG XIONG

Keyword(s):

Gene Expression ◽

Pancreatic Cancer ◽

Gene Ontology ◽

Microarray Analysis ◽

Cancer Tissue ◽

Tissue Samples ◽

Abstract Objective: To screen and analyze differentially expressed genes in pancreatic carcinoma tissues taken from Mongolian and Han patients by Affymetrix Genechip. Methods: Pancreatic ductal cell carcinoma tissues were collected from the Mongolian and Han patients undergoing resection in the Second Affiliated Hospital of Nanchang University from March 2015 to May 2018 and the total RNA was extracted. Differentially expressed genes were selected from the total RNA qualified by Nanodrop 2000 and Agilent 2100 using Affymetrix and a cartogram was drawn; The gene ontology (GO) analysis and Pathway analysis were used for the collection and analysis of biological information of these differentially expressed genes. Finally, some differentially expressed genes were verified by real-time PCR. Results: Through the microarray analysis of gene expression, 970 differentially expressed genes were detected by comparing pancreatic cancer tissue samples between Mongolian and Han patients. A total of 257 genes were significantly up-regulated in pancreatic cancer tissue samples in Mongolian patients; while a total of 713 genes were down-regulated. In the Gene Ontology database, 815 differentially expressed genes were identified with clear GO classification, and CPB1 gene showed the highest increase in expression level (multiple difference: 31.76). The pathway analysis detected 28 signaling pathways that included these differentially expressed genes, involving a total of 178 genes. Among these pathways, the enrichment of differentially expressed genes in the FAK signaling pathway was the strongest and COL11A1 gene showed the highest multiple difference (multiple difference: 5.02). The expression of differentially expressed genes CPB1, COL11A1、ITGA4、BIRC3、PAK4、CPA1、CLPS、PIK3CG and HLA-DPA1 determined by real-time PCR were consistent with the results of gene microarray analysis. Conclusions: The results of microarray analysis of gene expression profiles showed that there are a large number of differentially expressed genes in pancreatic cancer tissue samples comparing Mongolian and Han population. These genes are closely related to the cell proliferation, differentiation, invasion, metastasis and multi-drug resistance in pancreatic cancer. They are also involved in the regulation of multiple important signaling pathways in organisms.

Screening differentially expressed genes of pancreatic cancer between Mongolian and Han people using bioinformatics technology

10.21203/rs.2.11118/v3 ◽

2019 ◽

Author(s):

Jiasheng Xu ◽

Kaili Liao ◽

ZHONGHUA FU ◽

ZHENFANG XIONG

Keyword(s):

Gene Expression ◽

Pancreatic Cancer ◽

Gene Ontology ◽

Microarray Analysis ◽

Cancer Tissue ◽

Tissue Samples ◽

Abstract Objective: To screen and analyze differentially expressed genes in pancreatic carcinoma tissues taken from Mongolian and Han patients by Affymetrix Genechip. Methods: Pancreatic ductal cell carcinoma tissues were collected from the Mongolian and Han patients undergoing resection in the Second Affiliated Hospital of Nanchang University from March 2015 to May 2018 and the total RNA was extracted. Differentially expressed genes were selected from the total RNA qualified by Nanodrop 2000 and Agilent 2100 using Affymetrix and a cartogram was drawn; The gene ontology (GO) analysis and Pathway analysis were used for the collection and analysis of biological information of these differentially expressed genes. Finally, some differentially expressed genes were verified by real-time PCR. Results: Through the microarray analysis of gene expression, 970 differentially expressed genes were detected by comparing pancreatic cancer tissue samples between Mongolian and Han patients. A total of 257 genes were significantly up-regulated in pancreatic cancer tissue samples in Mongolian patients; while a total of 713 genes were down-regulated. In the Gene Ontology database, 815 differentially expressed genes were identified with clear GO classification, and CPB1 gene showed the highest increase in expression level (multiple difference: 31.76). The pathway analysis detected 28 signaling pathways that included these differentially expressed genes, involving a total of 178 genes. Among these pathways, the enrichment of differentially expressed genes in the FAK signaling pathway was the strongest and COL11A1 gene showed the highest multiple difference (multiple difference: 5.02). The expression of differentially expressed genes CPB1, COL11A1、ITGA4、BIRC3、PAK4、CPA1、CLPS、PIK3CG and HLA-DPA1 determined by real-time PCR were consistent with the results of gene microarray analysis. Conclusions: The results of microarray analysis of gene expression profiles showed that there are a large number of differentially expressed genes in pancreatic cancer tissue samples comparing Mongolian and Han population. These genes are closely related to the cell proliferation, differentiation, invasion, metastasis and multi-drug resistance in pancreatic cancer. They are also involved in the regulation of multiple important signaling pathways in organisms.

Screening differentially expressed genes of pancreatic cancer between Mongolian and Han people using bioinformatics technology

10.21203/rs.2.11118/v1 ◽

2019 ◽

Author(s):

Jiasheng Xu ◽

Kaili Liao ◽

ZHONGHUA FU ◽

ZHENFANG XIONG

Keyword(s):

Gene Expression ◽

Pancreatic Cancer ◽

Gene Ontology ◽

Pathway Analysis ◽

Cancer Tissue ◽

Tissue Samples ◽

Abstract Objective To screen and analyze differentially expressed genes in pancreatic carcinoma tissues taken from Mongolian and Han patients by Affymetrix Genechip. Methods: Pancreatic ductal cell carcinoma tissues were collected from the Mongolian and Han patients undergoing resection in the Second Affiliated Hospital of Nanchang University during March 2015 to May 2018 and the total RNA was extracted. Differentially expressed genes were selected from the total RNA qualified by Nanodrop 2000 and Agilent 2100 using Affymetrix and a cartogram was drawn; The gene ontology (GO) analysis and Pathway analysis were used for the collection and analysis of biological information of these differentially expressed genes. Finally, some differentially expressed genes were verified by real-time PCR. Results Through the microarray analysis of gene expression, 970 differentially expressed genes were detected by comparing pancreatic cancer tissue samples between Mongolian and Han patients. A total of 257 genes were significantly up-regulated in pancreatic cancer tissue samples in Mongolian patients;while a total of 713 genes were down-regulated. In the Gene Ontology database, 815 differentially expressed genes were identified with clear GO classification, and CPB1 gene had the highest multiple of differential expression (difference multiple: 31.76). The Pathway analysis detected 28 signaling pathways that included these differentially expressed genes, involving a total of 178 genes. Among these pathways, the enrichment of differentially expressed genes in the FAK signaling pathway was the highest and COL11A1 gene had the highest multiple difference (multiple difference: 5.02). The expressions of differentially expressed genes CPB1, COL11A1、ITGA4、BIRC3、PAK4、CPA1、CLPS、PIK3CG and HLA-DPA1 determined by real-time PCR were consistent with the results of gene chip analysis. Conclusions The results of microarray analysis of gene expression profiles showed that there are a large number of differentially expressed genes in pancreatic cancer tissue samples compared between Mongolian and Han populations. These genes are closely related to the proliferation, differentiation, invasion and metastasis and multi-drug resistance of pancreatic cancer and are involved in the regulation of multiple important signaling pathways in organisms.

Digital Gene Expression Profiling Analysis of Aged Mice under Moxibustion Treatment

Evidence-based Complementary and Alternative Medicine ◽

10.1155/2018/4767328 ◽

2018 ◽

Vol 2018 ◽

pp. 1-10 ◽

Cited By ~ 3

Author(s):

Nan Liu ◽

Yunyao Jiang ◽

Min Xing ◽

Baixiao Zhao ◽

Jincai Hou ◽

...

Keyword(s):

Gene Expression ◽

Gene Ontology ◽

Gene Expression Profiling ◽

Pathway Analysis ◽

Expression Profiling ◽

Digital Gene Expression ◽

Aged Mice ◽

Digital Gene Expression Profiling

Aging is closely connected with death, progressive physiological decline, and increased risk of diseases, such as cancer, arteriosclerosis, heart disease, hypertension, and neurodegenerative diseases. It is reported that moxibustion can treat more than 300 kinds of diseases including aging related problems and can improve immune function and physiological functions. The digital gene expression profiling of aged mice with or without moxibustion treatment was investigated and the mechanisms of moxibustion in aged mice were speculated by gene ontology and pathway analysis in the study. Almost 145 million raw reads were obtained by digital gene expression analysis and about 140 million (96.55%) were clean reads. Five differentially expressed genes with an adjusted P value < 0.05 and |log⁡2(fold change)| > 1 were identified between the control and moxibustion groups. They were Gm6563, Gm8116, Rps26-ps1, Nat8f4, and Igkv3-12. Gene ontology analysis was carried out by the GOseq R package and functional annotations of the differentially expressed genes related to translation, mRNA export from nucleus, mRNA transport, nuclear body, acetyltransferase activity, and so on. Kyoto Encyclopedia of Genes and Genomes database was used for pathway analysis and ribosome was the most significantly enriched pathway term.

Selenium Regulates Gene Expression for Glucosinolate and Carotenoid Biosynthesis in Arabidopsis

Journal of the American Society for Horticultural Science ◽

10.21273/jashs.136.1.23 ◽

2011 ◽

Vol 136 (1) ◽

pp. 23-34 ◽

Cited By ~ 22

Author(s):

Carl E. Sams ◽

Dilip R. Panthee ◽

Craig S. Charron ◽

Dean A. Kopsell ◽

Joshua S. Yuan

Keyword(s):

Gene Expression ◽

Plant Species ◽

Chlorophyll Biosynthesis ◽

Plant Secondary Metabolites ◽

Carotenoid Biosynthesis ◽

Biosynthesis Pathway ◽

Tissue Samples ◽

Expression Of Genes

Glucosinolates (GSs) and carotenoids are important plant secondary metabolites present in several plant species, including arabidopsis (Arabidopsis thaliana). Although genotypic and environmental regulation of GSs and carotenoid compounds has been reported, few studies present data on their regulation at the molecular level. Therefore, the objective of this study was to explore differential expression of genes associated with GSs and carotenoids in arabidopsis in response to selenium fertilization, shown previously to impact accumulations of both classes of metabolites in Brassica species. Arabidopsis was grown under 0.0 or 10.0 μM Na2SeO4 in hydroponic culture. Shoot and root tissue samples were collected before anthesis to measure GSs and carotenoid compounds and conduct gene expression analysis. Gene expression was determined using arabidopsis oligonucleotide chips containing more than 31,000 genes. There were 1274 differentially expressed genes in response to selenium (Se), of which 516 genes were upregulated. Ontology analysis partitioned differentially expressed genes into 20 classes. Biosynthesis pathway analysis using AraCyc revealed that four GSs, one carotenoid, and one chlorophyll biosynthesis pathways were invoked by the differentially expressed genes. Involvement of the same gene in more than one biosynthesis pathway indicated that the same enzyme may be involved in multiple GS biosynthesis pathways. The decrease in carotenoid biosynthesis under Se treatment occurred through the downregulation of phytoene synthase at the beginning of the carotenoid biosynthesis pathway. These findings may be useful to modify the GS and carotenoid levels in arabidopsis and may lead to modification in agriculturally important plant species.

Gene Expression Profiling of Reticulocytes in Patients with Hereditary Spherocytosis after Depleting Globin Gene Transcripts

Blood ◽

10.1182/blood.v128.22.1255.1255 ◽

2016 ◽

Vol 128 (22) ◽

pp. 1255-1255

Author(s):

Reena Das ◽

Aggarwal Anu ◽

Manu Jamwal ◽

Prashant Sharma ◽

Man Updesh Singh Sachdeva ◽

...

Keyword(s):

Gene Expression ◽

Microarray Analysis ◽

Hereditary Spherocytosis ◽

Transcriptome Profile ◽

Total Rna ◽

Before And After ◽

Carnitine Metabolism ◽

Global Transcriptome

Abstract Introduction Global transcriptome analysis of circulating reticulocytes using microarrays is challenging due to the high abundance of globin transcripts. In order to accurately measure the transcriptome in reticulocytes, we planned to study the reticulocytes transcriptome profile before and after globin depletion. Patients with Hereditary Spherocytosis (HS) were recruited because of high reticulocytosis and also there was no global trancriptome profile available for the disease to the best of our knowledge. Methods Reticulocytes were purified by passing EDTA anticoagulated red cell suspensions through a column of microcrystalline cellulose and α-cellulose mixture. The extraction of total RNA was done fresh prior to microarray analysis using TRIzol reagent (Invitrogen) and RNeasy columns as per manufacturer's instruction. The globin transcripts were depleted with starting quantity of 3 µg of total RNA.using GLOBINclearTMHuman kit (Ambion, Austin, TX). RNA quality were assessed before and after depletion using Agilent Technologies 2100 Bioanalyzer in each sample used for the study. The Agilent Low Input Quick Amp Labelling kit was used to generate cRNA with a sample input of 200 ng total RNA in single-color microarray analysis (SurePrint G3 Human Gene Expression v3 8x60K Microarray, G4858A- 072363). cRNA was hybridized for 17 hours at 65˚C. After thorough washing, the results were extracted with Feature Extraction Project software and analysed using GeneSpring v13.0. For this study, differentially expressed genes were identified according to the criteria: t-test unpaired p (Corr) cut-off = 0.05 and fold-change cut-off of 2.0. These differentially expressed genes were imported in PANTHER (Protein Analysis Through Evolutionary Relationships) classification system to classify the genes. Results Transcriptome profiling of reticulocyte RNA from HS patients revealed 5318 annotated transcripts and 2744 lnc-RNA/uncharacterized transcripts to be differentially regulated before globin depletion. After globin depletion increase (8196 annotated transcripts and 4292 lnc-RNA) in the number of differentially regulated genes were observed. An increase of 54% and 56% was seen in annotated transcripts and noncoding transcripts respectively after globin depletion. This increased coverage may be attributed to the removal of the globin transcript. Gene Ontology analysis for molecular function, biological process, cellular component and protein class did not reveal any difference in the percentage of the category, though the number of transcripts was more after depletion. There were approximately 7% more pathways in the globin transcript depleted samples. Namely, 2-arachidonoylglycerol biosynthesis, biotin biosynthesis, carnitine metabolism, cobalamin biosynthesis, coenzyme a linked carnitine metabolism, cysteine biosynthesis, flavin biosynthesis, phenylalanine biosynthesis, sulfate assimilation, tyrosine biosynthesis pathways, etc. were elucidated only after globin depletion. Conclusions The globin transcript reduction followed by microarray analysis represents a robust methodology for studying pathophysiology of hematologic diseases which are not related to globin chain disorders. Furthermore we describe the global transcriptome profile of HS for the first time. Globin transcript depletion elucidates the better number of the transcripts and eventually the pathways which may have been earlier masked under the abundance of globin mRNAs. Pathway analysis and validation experiments are required to explain the role of these differentially expressed genes in the pathophysiology of HS. Disclosures No relevant conflicts of interest to declare.

Investigation of Aberrantly Methylated Differentially Expressed Genes in Pancreatic Cancer by Integrated Bioinformatics Analysis

10.21203/rs.3.rs-132250/v1 ◽

2021 ◽

Author(s):

Cailin xue ◽

Peng gao ◽

Xudong zhang ◽

Xiaohan cui ◽

Lei jin ◽

...

Keyword(s):

Gene Expression ◽

Pancreatic Cancer ◽

Signaling Pathways ◽

Dna Sequences ◽

Receptor Interaction ◽

Biological Processes ◽

Ppi Network ◽

Hub Genes

Abstract Background: Abnormal methylation of DNA sequences plays an important role in the development and progression of pancreatic cancer (PC). The purpose of this study was to identify abnormal methylation genes and related signaling pathways in PC by comprehensive bioinformatic analysis of three datasets in the Gene Expression Omnibus (GEO). Methods: Datasets of gene expression microarrays (GSE91035, GSE15471) and gene methylation microarrays (GSE37480) were downloaded from the GEO database. Aberrantly methylated-differentially expressed genes (DEGs) were analysis by GEO2R software. GO and KEGG enrichment analyses of selected genes were performed using DAVID database. A protein–protein interaction (PPI) network was constructed by STRING and visualized in Cytoscape. Core module analysis was performed by Mcode in Cytoscape. Hub genes were obtained by CytoHubba app. in Cytoscape software. Results: A total of 267 hypomethylation-high expression genes, which were enriched in biological processes of cell adhesion, biological adhesion and regulation of signaling were obtained. KEGG pathway enrichment showed ECM-receptor interaction, Focal adhesion and PI3K-Akt signaling pathway. The top 5 hub genes of PPI network were EZH2, CCNA2, CDC20, KIF11, UBE2C. As for hypermethylation-low expression genes, 202 genes were identified, which were enriched in biological processes of cellular amino acid biosynthesis process and positive regulation of PI3K activity, etc. The pathways enriched were the pancreatic secretion and biosynthesis of amino acids pathways, etc. The five significant hub genes were DLG3, GPT2, PLCB1, CXCL12 and GNG7. In addition, five genes, including CCNA2, KIF11, UBE2C, PLCB1 and GNG7, significantly associated with patient's prognosis were also identified. Conclusion: Novel genes with abnormal expression were identified, which will help us further understand the molecular mechanism and related signaling pathways of PC, and these aberrant genes could possibly serve as biomarkers for precise diagnosis and treatment of PC.

AKT1 (E17K) Mutation in Pancreatic Cancer

Technology in Cancer Research & Treatment ◽

10.1177/153303460800700509 ◽

2008 ◽

Vol 7 (5) ◽

pp. 407-408 ◽

Cited By ~ 12

Author(s):

Azim Mohamedali ◽

Nicholas C. Lea ◽

Roger M. Feakins ◽

Kavita Raj ◽

Ghulam J. Mufti ◽

...

Keyword(s):

Pancreatic Cancer ◽

Cell Line ◽

Somatic Mutation ◽

Cancer Progression ◽

Pleckstrin Homology Domain ◽

Cancer Tissue ◽

Tissue Samples ◽

Pancreatic Cell ◽

Ras Mutation

The prevalence of a novel somatic mutation (E17K) in the pleckstrin homology domain of AKT1 was investigated in pancreatic cancer using a quantitative pyrosequencing assay. This mutation was un-detectable in pancreatic cancer tissue samples (n=65) and pancreatic cell line (n=10) DNA suggesting that pancreatic cancer progression is mainly dependent on the K-Ras mutation.

Identification of key biomarkers for thyroid cancer by integrative gene expression profiles

Experimental Biology and Medicine ◽

10.1177/15353702211008809 ◽

2021 ◽

pp. 153537022110088

Author(s):

Jinyi Tian ◽

Yizhou Bai ◽

Anyang Liu ◽

Bin Luo

Keyword(s):

Gene Expression ◽

Thyroid Cancer ◽

Molecular Mechanisms ◽

Expression Profiles ◽

Thyroid Tissue ◽

Gene Signature ◽

Gene Expression Omnibus ◽

Tissue Samples

Thyroid cancer is a frequently diagnosed malignancy and the incidence has been increased rapidly in recent years. Despite the favorable prognosis of most thyroid cancer patients, advanced patients with metastasis and recurrence still have poor prognosis. Therefore, the molecular mechanisms of progression and targeted biomarkers were investigated for developing effective targets for treating thyroid cancer. Eight chip datasets from the gene expression omnibus database were selected and the inSilicoDb and inSilicoMerging R/Bioconductor packages were used to integrate and normalize them across platforms. After merging the eight gene expression omnibus datasets, we obtained one dataset that contained the expression profiles of 319 samples (188 tumor samples plus 131 normal thyroid tissue samples). After screening, we identified 594 significantly differentially expressed genes (277 up-regulated genes plus 317 down-regulated genes) between the tumor and normal tissue samples. The differentially expressed genes exhibited enrichment in multiple signaling pathways, such as p53 signaling. By building a protein–protein interaction network and module analysis, we confirmed seven hub genes, and they were all differentially expressed at all the clinical stages of thyroid cancer. A diagnostic seven-gene signature was established using a logistic regression model with the area under the receiver operating characteristic curve (AUC) of 0.967. Seven robust candidate biomarkers predictive of thyroid cancer were identified, and the obtained seven-gene signature may serve as a useful marker for thyroid cancer diagnosis and prognosis.