-
EXPR
ICC WES
Project ID
OEP005036
Project NameICC WES
Experiment TypeGenomic
OEX027276
-
EXPR
Clone library
Project ID
OEP001350
Project NameNewly-designed primers for hadal ecosystem
Experiment TypeMetagenomic
ProtocolPCR amplification of full-length 16S rRNA gene
OEX010862
-
EXPR
Metagenomic
Project ID
OEP001350
Project NameNewly-designed primers for hadal ecosystem
Experiment TypeMetagenomic
ProtocolPCR amplification of multiple 16S rRNA gene hypervariable regions
OEX010861
-
EXPR
Old_RNA-seq
Project ID
OEP004811
Project NameLoss of Setd2 induces systemic inflammation via embryo-derived Kupffer-like cell differentiation to drive malignant transformation
Experiment TypeTranscriptomic
ProtocolFor bulk RNA-seq, total RNA samples were extracted, and ribosomal RNA (rRNA) was removed using the Ribo-Zero rRNA Removal Kit (MRZMB126, Illumina). Subsequently, rRNA-depleted samples were fragmented, then subjected to first and second strand cDNA synthetization. cDNAs were ligated with sequencing adapters according to standard Novaseq 6000 platform (Illumina) manuscripts.
OEX027260
-
EXPR
Old_c-Kit+_scRNA-seq
Project ID
OEP004811
Project NameLoss of Setd2 induces systemic inflammation via embryo-derived Kupffer-like cell differentiation to drive malignant transformation
Experiment TypeTranscriptomic single cell
ProtocolBM cells separated from old WT and Setd2-MDS mice were stained with biotin-c-Kit antibody on ice for 20 minutes, then washed with MojoSort™ Buffer (480017, BioLegend) at 3,000rpm for 5 minutes. Subsequently, samples labelled with biotin-c-Kit antibody were isolated through MACS assay, then the c-Kit+ BM cells were purified with BD FACSAria™ III. After purification, the BD Rhapsody system (BD Biosciences) was used to capture the transcriptomic information of single cells. Then, a limiting dilution approach was performed to randomly sediment and capture the single cell. Beads with oligonucleotide barcodes were then added to reach a saturated state, ensuring that each cell can be paired with one bead. Cells subjected with beads were captured and used for scRNA-seq. Whole transcriptome libraries were constructed following the BD Rhapsody single-cell whole-transcriptome amplification workflow. Single-cell libraries were quantified using a High Sensitivity DNA chip (Agilent) on a Bioanalyzer 2200 and the Qubit High Sensitivity DNA Assay Kit (Thermo Fisher Scientific). The library was sequenced by HiSeq Xten (Illumina) on a 150 bp paired-end run.
OEX027261
-
EXPR
Old_LSK_ATAC_seq
Project ID
OEP004811
Project NameLoss of Setd2 induces systemic inflammation via embryo-derived Kupffer-like cell differentiation to drive malignant transformation
Experiment TypeTranscriptomic
ProtocolA total of 1×105 BM LSKs from WT and KO-MDS mice were sorted, washed in DPBS, and lysed in 50 μL lysis buffer (10 mM Tris-HCl pH 7.4, 10 mM NaCl, 3 mM MgCl2, 0.1% (v/v) Igepal CA-630) for the follow-up process, which was performed by TruePrepTM DNA Library Prep Kit V2 for Illumina (TD501, Vazyme) according to the manufacturer’s instructions. Subsequently, the library fragments were purified by VAHTS DNA clean beads (Vazyme, N411-01) for future sequencing according to standard illumina HiSeq/NextSeq platform manuscripts.
OEX027259
-
EXPR
scRNAseq001
Project ID
OEP004177
Project NameOEP004177
Experiment TypeTranscriptomic single cell
OEX027323
-
EXPR
scRNAseq006
Project ID
OEP004177
Project NameOEP004177
Experiment TypeTranscriptomic single cell
OEX027324
-
EXPR
scRNAseq002
Project ID
OEP004177
Project NameOEP004177
Experiment TypeTranscriptomic single cell
OEX024220
-
EXPR
scRNAseq003
Project ID
OEP004177
Project NameOEP004177
Experiment TypeTranscriptomic single cell
OEX024221