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Satellite DNA in Paphiopedilum subgenus Parvisepalum as revealed by high-throughput sequencing and fluorescent in situ hybridization

Author: A Chochai
A Ebihara
Andrew R. Leitch
AV Cox
AV Cox
B Koukalova
Barbara Gravendeel
BC Stöver
ELL Sonnhammer
F Ronquist
FJ Ruiz-Ruano
GA Torres
H Akaike
H Weiss-Schneeweiss
Ilia J. Leitch
J Doležel
J Felsenstein
J Ištvánek
J Macas
J Macas
J Macas
JA Nylander
JD Thompson
JH de Jong
Jing Wei Yap
JJ Clarkson
JL Bennetzen
JS Hawkins
JS Heslop-Harrison
K Emadzade
K Karasawa
K Karasawa
K Karasawa
K Karasawa
K Karasawa
K Karasawa
K Karasawa
K Karasawa
K Karasawa
K Skalická
KY Lim
LJ Kelly
LJ Kelly
M Kearse
Marinus J. M. Smulders
MC Chung
Michael F. Fay
N Ohmido
Oriane Hidalgo
P Cribb
P Novák
P Novák
P Trávníček
R Begum
RR Choudhury
S Altschul
S Dodsworth
S Heckmann
S Kubis
S Mehrotra
S Taketa
Shairul Izan
Steven Dodsworth
T Lan
T Schmidt
T Wicker
TJ White
U Pich
WL Gerlach
WL Gerlach
Y Sun
YI Lee
Yi-Ching Lee
YK Lim
YK Lim
Yung-I Lee
YY Guo
Z Yang
Publication venue: 'Springer Science and Business Media LLC'
Publication date: 24/11/2017
Field of study

Background: Satellite DNA is a rapidly diverging, largely repetitive DNA component of many eukaryotic genomes. Here we analyse the evolutionary dynamics of a satellite DNA repeat in the genomes of a group of Asian subtropical lady slipper orchids (Paphiopedilum subgenus Parvisepalum and representative species in the other subgenera/sections across the genus). A new satellite repeat in Paphiopedilum subgenus Parvisepalum, SatA, was identified and characterized using the RepeatExplorer pipeline in HiSeq Illumina reads from P. armeniacum (2n = 26). Reconstructed monomers were used to design a satellite-specific fluorescent in situ hybridization (FISH) probe. The data were also analysed within a phylogenetic framework built using the internal transcribed spacer (ITS) sequences of 45S nuclear ribosomal DNA. Results: SatA comprises c. 14.5% of the P. armeniacum genome and is specific to subgenus Parvisepalum. It is composed of four primary monomers that range from 230 to 359 bp and contains multiple inverted repeat regions with hairpin loop motifs. A new karyotype of P. vietnamense (2n = 28) is presented and shows that the chromosome number in subgenus Parvisepalum is not conserved at 2n = 26, as previously reported. The physical locations of SatA sequences were visualised on the chromosomes of all seven Paphiopedilum species of subgenus Parvisepalum (2n = 26–28), together with the 5S and 45S rDNA loci using FISH. The SatA repeats were predominantly localisedin the centromeric, peri-centromeric and sub-telocentric chromosome regions, but the exact distribution pattern was species-specific. Conclusions: We conclude that the newly discovered, highly abundant and rapidly evolving satellite sequence SatA is specific to Paphiopedilum subgenus Parvisepalum. SatA and rDNA chromosomal distributions are characteristic of species, and comparisons between species reveal that the distribution patterns generate a strong phylogenetic signal. We also conclude that the ancestral chromosome number of subgenus Parvisepalum and indeed of all Paphiopedilum could be either 2n = 26 or 28, if P. vietnamense is sister to all species in the subgenus as suggested by the ITS data

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