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Sample GSM3335745 Query DataSets for GSM3335745
Status Public on Aug 17, 2018
Title ZAPKO46_uIFN_2_viral RNA
Sample type SRA
 
Source name Human Immunodeficiency Virus (HIV)
Organism Human immunodeficiency virus
Characteristics cell type: THP-1
genotype: ZAP-KO
ifn treatment: yes
hiv strain: HIV-1 LAI
Treatment protocol 8e6 cells (>500X coverage) were transduced with the PIKAHIV library (MOI of 0.75) and selected in 1ug/mL puromycin for 10-14 days. For each replicate, 8e6 cells were infected with or without overnight IFNα treatment with HIV. Cells and viral supernatants were harvested 3 days post-infection.
Growth protocol THP-1 monocytic cells are grown in RPMI with 10% FBS and Pen/Strep (supplemented to 10mM HEPES, 4.5 g/L D-Glucose, 0.11 g/L Sodium Pyruvate + Glutamax), passaging between 2e5 cells/mL and 1e6 cells/mL.
Extracted molecule total RNA
Extraction protocol Viral RNA was extracted using a QIAamp Viral RNA Mini Kit (Qiagen)
Genomic DNA or reverse-transcribed viral RNA were amplified by a two-step PCR (PCR1: 12 cycles, PCR2: 20 cycles) to amplify 20bp sgRNA sequences in the HIV-CRISPR vector. All Viral RNA was amplified for each sample where appropriate. For Genomic DNA samples a total of 500-fold coverage of the 15,414 sgRNAs were amplified (10^6 cells were estimated to contain 6.6μg gDNA) with a maximum of 2μg gDNA per PCR reaction. For each sample, PCR1 reactions were pooled, cleaned up over a QIAquick PCR purification Kit (2 columns per sample), pooled again and used as template for PCR2. For viral RNA, all PCR1 was amplified in the second round. For gDNA, 5uL of pooled PCR1 was used as input for PCR2 (PCR2 primers include Illumina barcodes and adaptor sequences). Amplicons from PCR2 were pooled, purified by double-sided SPRI (AMPureXP, Beckman Coulter), quantified with a Qubit HS dsDNA assay and pooled for sequencing.
 
Library strategy OTHER
Library source transcriptomic
Library selection other
Instrument model Illumina HiSeq 2500
 
Description viral RNA
Data processing Library strategy: CRISPR screen
Image analysis and base calling were performed using Illumina's Real Time Analysis v1.18 software, followed by generation of fastq files using Illumina's bcl2fastq Conversion Software v1.8.4 (http://support.illumina.com/downloads) /bcl2fastq_conversion_software_184.html).
Reads of low quality were filtered out prior to demultiplexing using FASTX-Toolkit v0.0.13
Reads were trimmed and aligned to the PIKA HIV guide library using Bowtie v1.0.0, allowing 0 mismatches in the guide sequence, followed by tabulation of read counts using R
Genome_build: PIKA HIV sgRNA Library. FASTA is available on series record. More information on the library is also available on bioRxiv:
https://www.biorxiv.org/content/early/2018/07/20/363432
Supplementary_files_format_and_content: tab delimited files with read counts for each guide sequence
 
Submission date Aug 16, 2018
Last update date Aug 17, 2018
Contact name Molly Ohainle
E-mail(s) mohainle@fredhutch.org
Organization name Fred Hutchinson Cancer Research Center
Street address 1100 Fairview Ave N, C2-023
City Seattle
State/province WA
ZIP/Postal code 98109
Country USA
 
Platform ID GPL25457
Series (1)
GSE118631 A Virus-Packageable CRISPR Screen Identifies Host Factors Mediating Interferon Inhibition of HIV
Relations
BioSample SAMN09843422
SRA SRX4559670

Supplementary file Size Download File type/resource
GSM3335745_ZAPKO46_uIFN_2.counts.txt.gz 124.8 Kb (ftp)(http) TXT
SRA Run SelectorHelp
Raw data are available in SRA
Processed data provided as supplementary file

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