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SRX23139545: GSM8008038: A. burtoni, testes, rep3 [smallRNA-seq]; Haplochromis burtoni; ncRNA-Seq
1 ILLUMINA (Illumina NovaSeq 6000) run: 38.3M spots, 1.9G bases, 572.4Mb downloads

External Id: GSM8008038_r1
Submitted by: Department of Biochemistry, University of Cambridge
Study: Dynamic co-evolution of transposable elements and the piRNA pathway in East African cichlid fishes [smallRNA-seq]
show Abstracthide Abstract
East African cichlid fishes have diversified in an explosive fashion, but the (epi)genetic basis of the phenotypic diversity of these fishes remains largely unknown. Although transposable elements (TEs) have been associated with phenotypic variation in cichlids, little is known about their transcriptional activity and epigenetic silencing. Here, we describe dynamic patterns of TE expression in African cichlid gonads and during early development. Orthology inference revealed an expansion of piwil1 genes in Lake Malawi cichlids, likely driven by PiggyBac TEs. The expanded piwil1 copies have signatures of positive selection and retain amino acid residues essential for catalytic activity. Furthermore, the gonads of African cichlids express a Piwi-interacting RNA (piRNA) pathway that target TEs. We define the genomic sites of piRNA production in African cichlids and find divergence in closely related species, in line with fast evolution of piRNA-producing loci. Our findings suggest dynamic co-evolution of TEs and host silencing pathways in the African cichlid radiations. We propose that this co-evolution has contributed to cichlid genomic diversity. Overall design: To profile small RNAs and identify Piwi-interacting RNAs (piRNAs) in the East African cichlid radiations, we have sequenced small RNAs from ovaries and testes of cichlid species representative of the three East African Great Lakes, as well as of Nile Tilapia (Orechromis niloticus) an outgroup to radiating cichlids. We also sequenced muscle, a somatic tissue which is not expected to have prominent piRNA populations.
Sample: A. burtoni, testes, rep3 [smallRNA-seq]
SAMN39313608 • SRS20090586 • All experiments • All runs
Library:
Name: GSM8008038
Instrument: Illumina NovaSeq 6000
Strategy: ncRNA-Seq
Source: TRANSCRIPTOMIC
Selection: size fractionation
Layout: SINGLE
Construction protocol: Tissue pieces were transferred to BeadBug tubes prefilled with 0.5 mm Zirconium beads (Merck, #Z763772) and 500-600 µl of TRIzol (Life Technologies, #15596026) was added to the tubes and mixed vigorously. Afterwards, we conducted the homogenisation using a BeadBug microtube homogeniser (Sigma, #Z764140) at approximately 4oC (in cold room). Each sample was homogenised with five BeadBug runs at maximum speed (4000 rpm) for 60 seconds each. Supernatant was then removed into a clean 1.5 mL tube. Centrifuged the lysates again, this time at maximum speed (approximately 21,000 G) for 5 minutes at 4oC. Transferred supernatant into a clean tube without disturbing the pellet and tissue debris. Mixed supernatant thoroughly 1:1 with 100% ethanol, pipetted the mix into a column provided in the Direct-zol RNA Miniprep Plus kit (Zymo Research, #R2072) and followed manufacturer's instructions, using the recommended in-column DNase I treatment. Samples were processed according to the NEXTFLEX® Small RNA-Seq Kit v4 with UDIs (PerkinElmer, #NOVA-5132-32) with a 1 µg starting input and 12 cycles of PCR. Samples were then pooled in equimolar amounts according to the TapeStation results and sequenced on a Novaseq 6000 system (PE50 on one lane of an SP Flowcell).
Runs: 1 run, 38.3M spots, 1.9G bases, 572.4Mb
Run# of Spots# of BasesSizePublished
SRR2746798438,275,8041.9G572.4Mb2024-04-01

ID:
31262557

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