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SRX12727601: GSM5645923: AAV9_Lysate_TechRep2; Adeno-associated virus 9; RNA-Seq
1 ILLUMINA (Illumina NovaSeq 6000) run: 42.6M spots, 6.4G bases, 1.7Gb downloads

External Id: GSM5645923_r1
Submitted by: Dougherty, Genetics, Washington University in St. Louis
Study: Extensive sex differences in depression-linked variants functionally assayed in mouse brain [Hippocampus]
show Abstracthide Abstract
Here, we selected >1000 variants from over 30 depression-associated loci using brain epigenomic data, and functionally assayed them using in vivo functional assays in the mouse brain to examine sex-by-genotype interactions. We identify extensive sex-by-allele effects in mature hippocampus, suggesting genetic risk and thus disease mechanisms may be distinct between the sexes. Unbiased informatics approaches indicated a role for nuclear hormone receptors, which was supported by . Further, comparative analysis of allelic function in the neonatal mouse brain, during a key between developmental neonates during the masculinizing testosterone surge, and in the adult hippocampus—a region of interest in depression pathology—but not at 10 days old, a older hormonally quiescent developmental stage juveniles. Our study provides novel insights into depression genetics as influenced by age, biological sex, and cell type, and provides a framework for in vivo parallel assays at a scale not previously shown possible to functionally define interactions between sex and disease variation. Overall design: n=5 replicates each of AAV9-transduced adult mouse brain tissues: male total hippocampus, female total hippocampus, male Vglut1+ translating-ribosome affinity purification immunoprecipitated RNA fraction, female Vglut1+ translating-ribosome affinity purification immunoprecipitated RNA fraction. Additional grant information: 571009 - Joseph Dougherty - Simons Foundation
Sample: AAV9_Lysate_TechRep2
SAMN22512613 • SRS10692096 • All experiments • All runs
Library:
Name: GSM5645923
Instrument: Illumina NovaSeq 6000
Strategy: RNA-Seq
Source: GENOMIC
Selection: cDNA
Layout: SINGLE
Construction protocol: Hippocampus dissected away from rest of brain, homogenized with power drill in glass pestle with RNAse inhibitors and translation inhibitor cycloheximide, spun 2,000g, supernatant mixed with 10% NPC and 10% DHPC 20min on ice, 20,000g spin, part of supernatant added to trizol for "input" (total hippocampal) RNA and remainder used for immunoprecipitation of GFP+ ribosomes (i.e. TRAP). See methods in paper for full details. Reporter-specific cDNA synthesis using a reverse-complementary primer, followed by PCR, digestion, adapter ligation, and index PCR. DNA from plasmid was prepared simultaneously, starting with the first PCR step. Each step was followed by a cleanup using size-selection beads (brands Ampure XP and Magbind).
Runs: 1 run, 42.6M spots, 6.4G bases, 1.7Gb
Run# of Spots# of BasesSizePublished
SRR1652498542,555,5516.4G1.7Gb2023-02-10

ID:
17328513

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