Project description:Umbilical cord blood-derived mononuclear cells were lineage depleted using a StemSep column and cultured in serum-free liquid suspension culture with cytokines SCF, FL, and Tpo. After four days in culture (d4), cultured cells were split into 2 groups; one subjected to media exchange and one subjected to a mock exchange, and cultured for an additional day. RNA was extracted and analyzed on an oligonucleotide microarray from day 4 cultured cells (d4), day 4-derived sorted lin+ cells (lin+), day 4 cells which were placed in fresh media for 24-hours (d5-E) and day 4 cells which were subjected to a mock media dilution/exchange and left for 24-hours (d5-NE) Total cellular mRNA was collected by lysing cells in 500 μl Trizol Reagent (Invitrogen, Groningen, The Netherlands) for 5 min followed by addition of 100 μl chloroform. After centrifugation at 12,000 g for 15 min, the aqueous phase was collected and mixed with isopropanol to precipitate the mRNA. The mRNA pellet was then obtained by centrifugation at 12,000 g for 10 min, washed in 70% ethanol and re-suspended in sterile water. mRNA concentration was then determined using a mQuant plate reader (Biotek Instruments, Winooski, VT). Subsequent sample preparation and hybridization was conducted as described in the Affymetrix GeneChip Expression Analysis Technical Manual (Affymetrix, Santa Clara, CA). Because of the limited numbers of cells that could be collected from each experiment, the Two-Cycle Target Labeling technique was used which first translates RNA into cDNA using a T7-oligo(dT) polymerase primer. The cDNA was then subjected to in vitro transcription during which biotin labeled nucleotides are incorporated into the resultant cRNA. The cRNA was then fragmented and hybridized to the Affymetrix HU133 chip set. All samples were obtained in triplicate and sent to the Ontario Genomics Innovation Centre (Ottawa Health Research Institute, Ottawa, Canada) for analysis. Keywords: parallel sample

Project description:In this study, we evalauted the transcriptionl profiles of human primordial germ cell-like cell (hPGCLCs) cultured for an extended period on STO feeders in FR10 media for an additional 10 days (D4C10). The hPGCLCs were obtained from two different human embryonic stem cell line (hESCs), UCLA 1 (XX) and UCLA2 (XY) for the RNA sequencing data. For whole genome bisulfite sequencing, we evaluate primed UCLA2 hESCs, directly out of the aggragate hPGCLCs (Day 4= D4) and extended culture hPGCLCs D4C10. Our D4C10 hPGCLCs were compared to prior RNA-sequencing data generated in our laboraty, which revealed that D4C10 hPGCLCs retain germline identy and closely resemble D4 hPGCLCs at the transcriptional level. Our WGBS data revealed that extended culture hPGCLCs at D4C10 have a decrease in CG methlyation, as compared to the starting hESCs and D4 hPGCLCs.

Project description:Tyrosine (Tyr, Y) and phenylalanine (Phe, F) synthesis is shared by the pea aphid and its symbiont Buchnera aphidicola.These aromatic amino acids are essential for the pea aphid growth and development. To characterize the molecular mechanisms, at gene transcriptional level, underlying this symbiotic integrated network pea aphids (Acyrthosyphon pisum, clone LL01) were reared on (i) standard artificial diet (AP3) and (ii) on the same AP3 medium depleted of Tyr (Y) and Phe (F). From each of the two groups, aphids were collected at specific time points and dissected: 12 h (D0), 1 day (D1), 2 days (D2), 3 days (D3), 4 days (D4), 5 days (D5) and 7 days (D7). Total RNA, to be used in gene expression analysis by arrays, was extracted, under the two rearing conditions, from two tissues: gut [from 20 aphids per sample at all 7 time points] and bacteriocytes [from 25 aphids per sample at 4 time points: 3 days (D3), 4 days (D4), 5 days (D5) and 7 days (D7)]. At each time point we included three biological replicates.

Project description:LC-IMS-MS/MS data from a large study of human plasma samples consisting of 40 quality control samples from the NIST Standard Reference Material 1950 and 112 study samples. An internal standard mixture consisting of D4-malonic acid, D4-succinic acid, D5-glycine, D4-citric acid, 13C6-fructose, D5-L-tryptophan, D4-lysine, D7-alanine, D35-stearic acid, D5-benzoic acid, and D15-octanoic acid was added prior to extraction. Each sample was spiked with 50 uL of a solution of the internal standards at 0.166 mg/mL in water. Metabolites and lipids were extracted with concomitant protein precipitation using the Matyash protocol. The metabolite layer was removed and dried in vacuo. Lipid and protein layers were not analyzed. An Agilent 1260 Infinity II high flow liquid chromatography system was used to inject and chromatographically separate samples prior to introduction to the ion mobility spectrometry-mass spectrometry instrument. A steady flowrate of 0.300 mL/min was delivered through a Millipore-Sigma SeQuant Zic-pHILIC column (15 cm length, 2.1 mm inner diameter, packed with 5 um particles). Ion mobility spectrometry-tandem mass spectrometry analysis was performed using an Agilent 6560 Ion Mobility LC/Q-TOF system. Spectra were acquired separately in both positive and negative ionization modes. Fixed collision energies were employed at 10, 20, and 40 eV on alternating frames.

Project description:After isolation, islets were cultured in a serum-exosomes-free culture media for one week. Collected culture media were centrifuged first at 300g for 20 min to pellets cells and then at 10000g for 20 min to discard dead cells and cell debris. Exosomes were then isolated from the supernatant by ultracentrifugation at 110000g for 70 min. Exosomes were collected in a minimal volume of PBS,and added three times the volume of Trizol LS to extract exosomes RNA.

Project description:In this study, we evaluated the 5mC content of single cell human primordial germ cell-like cells (hPGCLCs) generated from a male human embryonic stem cell line (UCLA2, 46XY). tilizing a strand-specific, enzymatic based method of sequencing, we compared the 5mC content of the plus strand relative to the whole chromosome. We evaluated just specified hPGCLCs, at day 4 of differentiation (D4) and then D4 hPGCLCs that were cultured on a feeder layer for additional 10 days (D4C10).

Project description:CUT&Tag seq of HK16ac in TS(trophoblast stem cells), STB-D1(TS cells culture in STB medium for syncytialization one day), STB-D4(TS cells culture in STB medium for syncytialization 4 day), STB-D4 treated with oxamate(TS cells culture in STB medium for syncytialization 4 day and treated with oxamate), STB-D4 treated with oxamate and acetate(TS cells culture in STB medium for syncytialization 4 day and treated with oxamate and acetate). we explored the relationship between glycolysis and syncytializaion.

Project description:Despite the importance of inter-cellular communication networks in regulating stem cell fate decisions, very little is known about the topology, dynamics, or functional significance. Using human blood stem cell cultures as an experimental paradigm, we present a novel bioinformatic approach to integrate genome-scale molecular profiles (transcriptome and secretome) and publicly available databases to reconstruct soluble factor-mediated inter-cellular signalling networks regulating blood stem cell fate decisions. Umbilical cord blood UCB cells were lineage depleted via immuno-magnetic column and placed in serum free media, supplemented with SCF, FL, and TPO. At culture day 4, cells were either subject to Lin- cell re-selection + media exchange (S/E) or not (NS/NE) and cultured for an additional 4 days. At day-8, S/E cell sample was subject to another S/E procedure and cultured for an additional 4 days. At day-0, 4, 8, and 12, cells were separated into Lin- and Lin+ for independent profiling using Affymetrix HU133 v2.0 arrays.

Project description:Intervention1: Biopsy: The biopsy tissue will be processed to obtain the primary cell line. In the next stage of the study, the cultured primary cell line will be subjected to various chemotherapeutic agents in different concentrations and studied using real time cell analyzer for 5 days to obtain IC50 values. Both the primary cells and biopsy sample will be subjected to microarray, qPCR and proteomics. Control Intervention1: Nil: Nil Primary outcome(s): To validate methodology to establish primary tumor cell line from biopsy samples of cancer patients like breast cancer, NSCLC, Head & Neck, Colorectal.Timepoint: Baseline

Project description:The photosynthetic model marine diatom Phaeodactylum tricornutum was cultured with varying nitrogen sources and availability to elicit shifts in the proteome. Cells were grown to mid-exponential phase on ammonium (880 uM), collected by centrifugation and resuspended in N-free media for 2 hrs, and spiked with nitrate (150 uM) for 90 min. Cells were again collected by centrifugation, washed in N-free media, and resuspended in experimental treatments with no nitrogen (N-) and a nitrogen source (300 uM) provided as ammonium, nitrite, or nitrate. Each experimental treatment was sampled after 15 min, 45 min, and 18 hr.