Project description:Amplicon sequencing of ITS and cpDNA regions for molecular phylogenetic analysis of Deutzia (Hydrangeaceae) in Japan

Project description:Amplicon sequencing of ITS and cpDNA regions for molecular phylogenetic analysis of Stellaria (Caryophyllaceae) in Japan.

Project description:Amplicon sequencing of ITS and cpDNA regions for molecular phylogenetic analysis of Clinopodium (Lamiaceae) in western Japan

Project description:Amplicon sequencing of ITS and cpDNA regions for molecular phylogenetic analysis of Hypericum (Hypericaceae) in western Japan

Project description:Amplicon sequencing of ITS and cpDNA regions for molecular phylogenetic analysis of Hydrangea serrata complex (Hydrangeaceae) in western Japan

Project description:Amplicon sequencing of ITS and cpDNA regions for molecular phylogenetic analysis of Japanese fir (Abies) and their closely related species.

Project description:Amplicon-based targeted re-sequencing analysis was performed in the patient-derived gliobastoma cell culture samples. For this purpose, genomic DNA (gDNA) was isolated and DNA libraries were prepared using the TruSeq Custom Amplicon Low Input (Illumina, Inc.) technology. By this, a pool of 375 amplicons was generated for each single sample in order to enrich for the target genes ATRX1, EGFR, IDH1, NF1, PDGFRA, PIK3CG, PIK3R1, PTEN, RB1 and TP53. Sequencing was performed on the Illumina MiSeq® next generation sequencing system (Illumina Inc.) and its 2 x 250 bp paired-end v2 read chemistry. The resulting reads were quality controlled and mapped against the human reference genome (hg19). For all samples, sequence variations of the amplified regions of interest in comparison to the human reference sequence were identified and filtered based on reliability.

Project description:To compare the impact of CRISPR-egineered R175 TP53 mutant variants in HCT116 and H460 cells, mutations at the amino acid position 175 were generated systematically by CRISP/Cas9 editing. Here, genomic amplicon regions covering the TP53 Exons 5 were sequenced via targeted sequencing.

Project description:Immunoprecipitation of the chloroplast splicing factor CAF1 and analysis of bound RNAs with a complete Zea mays cpDNA microarray.

Project description:Genome editing was conducted on a t(3;8) K562 model to investigate the effects of deleting different modules or CTCF binding sites within the MYC super-enhancer. To check mutations after targeting with CRISPR-Cas9 we performed amplicon sequencing using the Illumina PCR-based custom amplicon sequencing method using the TruSeq Custom Amplicon index kit (Illumina). The first PCR was performed using Q5 polymerase (NEB), the second nested PCR with KAPA HiFi HotStart Ready mix (Roche). Samples were sequenced paired-end (2x 250bp) on a MiSeq (Illumina).