Project description:Purpose: To elucidate the molecular basis governing lung metastasis in ESCC cells, we established two subpopulations of ESCC cells with enhanced pulmonary metastatic potential, namely K30LM3 and K450LM2 respectively. Then, transcriptional profiling of highly metastatic cells (K30LM3 and K450LM2) and their parental cells (K30 and K450) were performed to characterize differentially expressed genes (DEG). Methods: When parental and highly metastatic cells grew to approximately 80% confluence, these cells were washed twice using pre-chilled PBS. Total RNAs were harvested using Trizol reagents (Thermo Fisher Scientific). Poly(A) mRNA was isolated and enriched using NEBNext Poly(A) mRNA Magnetic Isolation Module. The mRNA was then recovered for library generation with NEBNext ® Ultra™ Directional RNA Library Prep Kit for Illumina (NEB, E7420S) following the manufacturer’s instructions. The cDNA libraries were sequenced at WuXiNextCODE (China). FastQC was used to examine the quality of raw reads. Read alignment was conducted using STAR (v2.5.1b), and R package edgeR (v3.8.5) was used to determine relative transcript abundances and differentially expressed genes (DEGs) between sample pairs. Results: Generally, 1502 genes (FDR<0.05, Fold Change>2) between K30 and K30LM3 cells and 650 genes (FDR<0.05, Fold Change>2) between K450 and K450LM2 cells were detected. Among thses DEGs, 52 genes were co-upregulated while 32 genes were co-downregulated in K30LM3/K450LM2 cells. GSEA showed that these commonly-changed genes were significantly enriched in epithelial-mesenchymal transition (EMT), cell adhesion, and anoikis process. Conclusions: In vivo selection approach enriched highly metastatic subpopulations with acquired essential molecular traits.

Project description:Purpose: to find the potential down-stream target gene of circFAM120A Methods: mRNA profiles of decidualized human endometrial stromal cells (hESCs) after down-regulated FAM120A and control using siRNA were generated by NGS and compared by bioinformatics analysis Results: we sequenced 26414 mRNAs in hESCs between the si-NC and si-circFAM120A groups and identified 242 differentially expressed mRNAs, between which 161 were downregulated and 81 were up-regulated in si-circFAM120A group Conclusions: Our study represents the detailed analysis of decidualized hESCs transcriptomes between si-NC and si-circFAM120A groups.

Project description:Purpose: To elucidate how ACAT2 influenced the expression profile in STAD cells, ACAT2 expression was reduced using one shRNA in STAD HGC-27 cells. Then, transcriptional profiling of cells with ACAT2 knockdown (shACAT2) and the control cells (shNC) was performed to characterize differentially expressed genes (DEG).Methods: When shNC and shACAT2 cells grew to approximately 80% confluence, these cells were washed twice using pre-chilled PBS. Total RNAs were harvested using Trizol reagents (Thermo Fisher Scientific). Poly(A) mRNA was isolated and enriched using NEBNext Poly(A) mRNA Magnetic Isolation Module. The mRNA was then recovered for library generation with NEBNext ® Ultra™ Directional RNA Library Prep Kit for Illumina (NEB, E7420S) following the manufacturer’s instructions. The cDNA libraries were sequenced at WuXiNextCODE (China). FastQC was used to examine the quality of raw reads. Read alignment was conducted using STAR (v2.5.1b), and R package edgeR (v3.8.5) was used to determine relative transcript abundances and differentially expressed genes (DEGs) between sample pairs. Results: Generally, 241 genes were increased and 117 genes decreased in HGC-27 shACAT2 cells, compared with shNC cells (FDR<0.05, Fold Change>2). GO analysis showed that these changed genes were significantly enriched in signal pathways related to cancer. Conclusions: Reduced ACAT2 expression alters multiple cancer-related signal pathways.

Project description:Gene expression profiling of endometrial stromal cells (ESCs) after transfection with si-NC or si-ASPM.

Project description:In order to screen the target genes regulated by lncMGPF,we transfected the siRNA to knock down lncMGPF gene (si-lncMGPF) and negative control siRNA (si-NC), induced cells to differentiate for 2 days.

Project description:Transcriptome variation of SiHa cells transfected with si-CNN3 or si-NC were detected by RNA-seq.

Project description:RNA-seq was used to analyze the differential expression of mRNAs between si-LINC00882 and si-NC-LINC00882 231 cells.

Project description:RNA-seq was used to analyze the differential expression of mRNAs between si-THAP7-AS1 and si-NC 231 cells.

Project description:Purpose: RNA-Seq was used to detect the dwonstream genes after CircRREB1 knockdow. Method: Three chondrocyte total RNA profiles of Si-NC samples and Si-CircRREB1 samples were analyzed.

Project description:Purpose: RNA-Seq was used to detect the dwonstream genes after FASN knockdow. Method: Three chondrocyte total RNA profiles of Si-NC samples and Si-FASN samples were analyzed.