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Sample GSM498722 Query DataSets for GSM498722
Status Public on Jan 20, 2010
Title CMV delta2b in Arabidopsis thaliana (col), replicate
Sample type SRA
 
Source name leaves of wt Arabidopsis thaliana infected with CMVf-Δ2b
Organisms Arabidopsis thaliana; Cucumber mosaic virus (strain FNY)
Characteristics a.thaliana genotype: wild type (col)
a.thaliana tissue: leaves
cmv genotype/variation: CMVf-Δ2b
cmv strain: FNY
collected time: 14 days after inoculation
Extracted molecule total RNA
Extraction protocol Small RNAs of 18- to 28-nt extracted by Trizol from the systemically infected leaves 14 days after inoculation with CMVf-Δ2b were purified from 15% denatured polyacrylamide gel. Purified small RNAs were directly ligated to the 3′-linker used for miRNA cloning (Integrated DNA Technology) by T4 RNA ligase 2Tr (New England Biolabs). The ligation products were purified and ligated to the 5′ Solexa linker (GUU CAG AGU UCU ACA GUC CGA CGA UC) by T4 RNA ligase I (New England Biolabs). The final ligation products were reverse transcribed using a primer targeting the 3′-linker (CTGTAGGCACCATCAAT OR CACTCGGGCACCAAGGA ) and the cDNA pool was amplified by PCR and sent for sequencing by the Solexa technology (Illumina). Duplicate libraries were constructed from two independent RNA samples from WT, rdr1, and rdr1 rdr2 rdr6 plants and sequenced by the Solexa platform in Illumina, Inc, and the University of California–Riverside Core Facility, respectively.
 
Library strategy OTHER
Library source viral RNA
Library selection cDNA
Instrument model Illumina Genome Analyzer
 
Description total small RNAs in systemically infected leaves of A. thaliana
barcode: ATC
Data processing All sequences containing perfect match 5' barcode (ATC/CGT/TAC) and at least 6 sucessive perfect-matched nucleotides of the 3' linker ( CTGTAGGCACCATCAAT / CACTCGGGCACCAAGGA) were kept for later analysis. The barcode and linker sequences were computationally removed by in-house perl script. All trimmed sequences in length of 17~30nt were aligned with CMV genome and the perfect matched reads were used for all further analysis.
 
Submission date Jan 20, 2010
Last update date May 15, 2019
Contact name Qingfa Wu
E-mail(s) qingfawu@ucr.edu
Phone 1-951-827-2340
Organization name UC Riverside
Lab Shou-Wei Ding
Street address 900 University Ave
City Riverside
State/province CA
ZIP/Postal code 92507
Country USA
 
Platform ID GPL9951
Series (1)
GSE19965 Virus-derived siRNAs in Arabidopsis thaliana
Relations
SRA SRX015845
BioSample SAMN00007554

Data table header descriptions
SEQUENCE filtered, unique sequence reads
COUNT absolute counts

Data table
SEQUENCE COUNT
TGAAGCTGCCAGCATGATCTA 95110
GTTCAATAAAGCTGTGGGAAG 71196
TGAAGCTGCCAGCATGATCTGG 46134
TTGTCGCTAAGATTCGA 35845
AGTGCTGGTCGTAACCGTCGA 17960
TTCCACAGCTTTCTTGAACTT 17566
TCGCTTGGTGCAGGTCGGGAAC 16433
AGTTACTAATTCATGATCTGGC 15349
CGTTAGCAGCTGGTCGTCCAA 14534
TCGCTTGGTGCAGGTCGGGAA 14050
TGAAAGTGACTACATCGGGGT 13056
GAGGGGCCGGACTGAAATAGC 12796
AGTTGATACAGTAGACATCTG 12002
TTTGTCGCTAAGATTCGA 11106
TACAAGCGAATGAGTCATTCA 10618
TCCCAAATGTAGACAAAGCA 10471
TTTGGATTGAAGGGAGCTCTT 10418
TTCCACAGCTTTCTTGAACTG 10194
GGGTGGTTAATAGTTGGACGA 9755
CGTGTGGGTGACAGTCCGTAA 8966

Total number of rows: 1972779

Table truncated, full table size 47717 Kbytes.




Supplementary data files not provided
SRA Run SelectorHelp
Processed data included within Sample table
Raw data are available in SRA

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