<HashMap><database>biostudies-arrayexpress</database><scores/><additional><omics_type>Metabolomics</omics_type><omics_type>Unknown</omics_type><omics_type>Transcriptomics</omics_type><omics_type>Genomics</omics_type><omics_type>Proteomics</omics_type><submitter>Data Submission IFOM - ETS</submitter><instrument_platform>NextSeq 550</instrument_platform><study_type>RNA-seq of coding RNA</study_type><organism>Mus musculus</organism><species>Mus musculus</species><full_dataset_link>https://www.ebi.ac.uk/biostudies/studies/E-MTAB-17005</full_dataset_link><description>Studying the expression profile in lungs of G3 Terc-/- mice, compared to wild-type controls</description><repository>biostudies-arrayexpress</repository><sample_protocol>Library Construction - For each sample, 500 ng of total RNA were used to generate a library of fragments using Stranded mRNA prep ligation kit (Illumina, 20040532). Oligo(dT) magnetic beads purify and capture the mRNA molecules containing polyA tails. The purified mRNA was fragmented and copied into first strand complimentary DNA (cDNA) using reverse transcriptase and random primers. In a second strand cDNA synthesis step, dUTP replaces dTTP to achieve strand specificity. The final steps added adenine (A) and thymine (T) bases to fragment ends and ligate adapters. The resulting products were purified and selectively amplified with 12 cycles of PCR to generate an indexed library of fragments. The library was quantified using Qubit 4.0 fluorimeter, checked on Agilent Bioanalyzer 2100 then loaded on Illumina NextSeq550Dx sequencer for sequencing, following the manufacturer’s instructions.</sample_protocol><sample_protocol>Sample Collection - Library fragments were sequenced using 2x75nt readmode, thus sequencing 75 nucleotides from both ends of each fragment; on average, ~ 50 Million Paired-end fragments were sequenced for each sample. Sequencing results were generated in fastq.gz format.</sample_protocol><sample_protocol>Sequencing - Library fragments were sequenced using 2x75nt readmode, thus sequencing 75 nucleotides from both ends of each fragment; on average, ~ 50 Million Paired-end fragments were sequenced for each sample. Sequencing results were generated in fastq.gz format.</sample_protocol><sample_protocol>Nucleic Acid Extraction - To isolate RNA, 20-30 mg lung tissue was homogenized in TRIzol (Invitrogen, 15596026) with TissueLyser II (Qiagen) and processed with RNeasy Plus Universal Mini Kit (Qiagen, 73404) according to the manufacturer’s specifications. To increase the purity of the RNA extracted, an on‐column RNase-Free DNase Set DNase I (Qiagen, 79256) treatment was performed to remove the residual amounts of DNA. NanoDrop spectrophotometer was used to detect RNA quantity and purity. RNA purity was ascertained via NanoDrop 260/280 and 260/230 ratios. The abundance and integrity of total RNA was assessed using Qubit fluorimeter and Agilent Bioanalyzer 2100 instrument (Agilent Technologies, Palo Alto, CA)</sample_protocol><figure_sub>Organization</figure_sub><figure_sub>MINSEQE Score</figure_sub><figure_sub>Assays and Data</figure_sub><figure_sub>MAGE-TAB Files</figure_sub><pubmed_authors>Data Submission IFOM - ETS</pubmed_authors><pubmed_authors>Fabrizio d'Adda di Fagagna</pubmed_authors><pubmed_authors>Alexandra Mancheno-Ferris</pubmed_authors><pubmed_authors>Francesca Rossiello</pubmed_authors></additional><is_claimable>false</is_claimable><name>The telomeric DNA damage response as a therapeutic target in Idiopathic Pulmonary Fibrosis</name><description>Studying the expression profile in lungs of G3 Terc-/- mice, compared to wild-type controls</description><dates><release>2026-07-10T00:00:00Z</release><modification>2026-07-10T01:01:00.54Z</modification><creation>2026-05-06T10:54:36.705Z</creation></dates><accession>E-MTAB-17005</accession><cross_references><ENA>ERP193072</ENA><Biostudies>E-MTAB-14908</Biostudies><EFO>EFO_0002944</EFO><EFO>EFO_0004170</EFO><EFO>EFO_0005518</EFO><EFO>EFO_0003738</EFO><EFO>EFO_0004184</EFO></cross_references></HashMap>