Abstract
In the publication "Genome-wide deposition of 6-methyladenine in human DNA reduces the viability of HEK293 cells and directly influences gene expression" bacterial DNA-adenine N6-Methyltransferases were expressed in human HEK293 cells. Cell proliferation and gene expression were investigated. Gene expression was investigated by RNA-seq.RNA-seq data were obtained from stable HEK293 cell lines, containing the bacterial N6-MTase CcrM (wildtype or catalytically inactive D39A mutant). Expression of CcrM was controlled by the doxycycline (dox)-inducible TRE3G promoter. RNA-seq experiments were performed with cells before ('no dox') or after 10 days ('10d dox') of dox treatment. Total RNA was isolated from ~10^6 cells using the RNeasy® Mini Kit (Qiagen), and quantified via NanoDrop1000. For each library, 1 µg RNA was taken as input material. Since total RNA is mostly constituted of rRNA (≥ 80%), poly-adenylated mRNA was first enriched using the NEBNext® Poly(A) mRNA Magnetic Isolation Module (NEB). Afterwards, RNA-seq libraries were generated using the NEBNext® Ultra™ II Directional RNA Library Prep Kit for Illumina® (NEB), in combination with NEBNext® Multiplex Oligos for Illumina® (Index Primers Set 1) (NEB), thus resulting in strand-specific RNA libraries (opposite sense strand). For quality assessment of the RNA-seq libraries, fragment size distributions and concentrations were determined by Labchip® GX Touch (Perkin Elmer). Finally, 300 ng of each RNA library was submitted to Novogene Corporation Inc. U.K. for Next-Generation-Sequencing (Illumina Novaseq 6000 system, paired-end, 2 x 150bp-mode). Sequencing data were received in FASTQ format (~2 x 20 million reads/sample), and all subsequent data processing steps were performed on the European Galaxy Platform (Afgan et al., 2016).
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