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Sample 4

Identifiers
BioSample: SAMEA104557120; SRA: ERS2168404
Organism
Anopheles coluzzii
cellular organisms; Eukaryota; Opisthokonta; Metazoa; Eumetazoa; Bilateria; Protostomia; Ecdysozoa; Panarthropoda; Arthropoda; Mandibulata; Pancrustacea; Hexapoda; Insecta; Dicondylia; Pterygota; Neoptera; Endopterygota; Diptera; Nematocera; Culicomorpha; Culicoidea; Culicidae; Anophelinae; Anopheles; Cellia; Pyretophorus; gambiae species complex
Attributes
tissuewhole organism
sample nameE-MTAB-6443:Sample 4
sexfemale
strainM
ENA first public2018-06-28
ENA last update2018-01-31
ENA-CHECKLISTERC000011
External IdSAMEA104557120
INSDC center aliasIP
INSDC center nameInstitut Pasteur
INSDC first public2018-06-28T17:03:06Z
INSDC last update2018-01-31T14:16:54Z
INSDC statuspublic
Submitter IdE-MTAB-6443:Sample 4
broker nameArrayExpress
replicate2
Description

Protocols: 12 mosquitoes per pool, in each of two biological replicate pools, were collected 3 d after infection by oral feeding with ONNV and homogenized in TriReagent (Sigma). The A. coluzzii Ngousso strain was originally initiated with mosquitoes collected in Cameroon in January 2006, and belongs to the M molecular and Forest chromosomal forms (Harris et al., 2010). Mosquitoes were reared under standard conditions at 26°C and 80% relative humidity, with a 12 h light/dark cycle as previously described (Mitri et al., 2015). Mosquitoes were infected on an infectious bloodmeal containing physiologically natural viral titers O'Nyong-Nyong strain SG650. 10ug of RNA (>200nt fraction) was used to prepare directional libraries using the TruSeq SmallRNA sample prep kit, set A and B (Illumina). Chemical fragmentation of polyA RNA was made with Ambion reagent (AM8740), followed by purification on RNeasy columns (Qiagen, #74204). Phosphatase and PNK treatments were performed and followed by purification on RNeasy columns (Qiagen, #74204). The fragmented RNA was ligated with 3'- and 5'- TruSeq adapters, as described in the original protocol. Synthesis of cDNA was performed by reverse transcription. The cDNA product was then specifically amplified by 11 cycles of PCR and products purified on Agencourt AMPure XP beads (Beckman Coulter Genomics, # A63881).

BioProject
PRJEB24724 Anopheles coluzzii RNAseq
Retrieve all samples from this project

Submission
EBI; 2018-07-03
Accession:
SAMEA104557120
ID:
9554443

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