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SRX21375589: GSM7712188: control RV male (CTRL-m_3); Rattus norvegicus; RNA-Seq
1 ILLUMINA (NextSeq 2000) run: 34.2M spots, 2.4G bases, 784.9Mb downloads

External Id: GSM7712188_r1
Submitted by: Soni Pullamsetti, Max Planck Institute
Study: Transcriptional profiling of male and female MCT-induced rats with compensated and decompensated right ventricle
show Abstracthide Abstract
We performed molecular phenotyping of RV remodeling, using transcriptome analysis of RV tissue obtained from MCT-induced rats (of both male and female animals). The clustering approach along with precise hemodynamics assessments identified “early" and "late" subgroups of decompensated state in rat RV. Further molecular characterization of these subgroups identified distinct molecular genes and pathways within different stages of RV remodeling. This study provided a resource to comprehensively compare human RV remodeling with the current animal model of PH (MCT), and led to validation of state-specific biomarkers and potential therapeutic targets for RV dysfunction. Overall design: RNA sequencing was performed for two batches of RV tissues obtained from MCT-induced rats (n=53) which were characterized as compensated RV, decompensated RV, as well as normal RV from control rats. Batch 1 include only male samples as follows: control (n=10), compensated RV (n=7), early decompensated RV (n=3), late decompensated RV (n=6). Second batch includes animals from both sexes as follows: control female RV (n=4), control male RV (n=4), compensated female RV (n=6), compensated male RV (n=5), decompensated female RV (n=3), decompensated male RV (n=5).
Sample: control RV male (CTRL-m_3)
SAMN36996205 • SRS18618705 • All experiments • All runs
Library:
Name: GSM7712188
Instrument: NextSeq 2000
Strategy: RNA-Seq
Source: TRANSCRIPTOMIC
Selection: cDNA
Layout: SINGLE
Construction protocol: MCT tissues from MCT-treated rats were harvested after RHC measurements and snap-frozen. Total RNA from each batch of RV samples were isolated separately using the RNeasy Mini Kit (or miRNeasy Micro Kit, when less sample provided-Qiagen) and snap-frozen. Purification of total RNA was performed as described in the RNeasy handbook, using DNase I digestion (RNase-Free DNase Set, Qiagen). Following the RNA integrity measurement, approximately 2 µg of total RNA were used as starting material for library preparation using the VAHTS Stranded mRNA-seq Library preparation following manufacture's protocol (Vazyme)
Runs: 1 run, 34.2M spots, 2.4G bases, 784.9Mb
Run# of Spots# of BasesSizePublished
SRR2564949034,235,9022.4G784.9Mb2023-09-29

ID:
28813815

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