Repetitive sequences have been widely used for examining genome and species
relationships by in situ and Southern hybridization. In the present study,
double-stranded DNA sequences, from denatured DNA reannealed to Cot = 1. f
rom Avena strigosa (2n = 2x = 14; A genome; referred to as CotA) and Avena
sativa (2n = 6x = 42; ACD genome; referred to as CotACD) were isolated with
a hydroxyapatite column, and were used for in situ hybridization on hexapl
oid. A. sativa chromosomes. Probe CotACD labelled all chromosomes evenly th
roughout their length at the same intensity. Probe CotA labelled the 28 A a
nd D genome chromosomes strongly and the 14 C genome chromosomes weakly. Th
ree cloned repetitive sequences, pAvKB9 (126 bp), pAvKB26 (223 bp) and pAvK
B32 (721 bp) were characterized in the A, B, C and D Avena genomes and the
genus Arrhenatherum using molecular and cytological methods. Clones pAvKB9
and pAvKB26 were absent from the Avena C genome, while both could identify
the presence of the D genome by Southern hybridization. In situ hybridizati
on to diploid and tetraploid Avena species revealed that the probes showed
a dispersed genomic organization and that they are present on both arms of
all chromosomes. These sequences were excluded from areas where tandem repe
ats, such as rRNA genes and telomeres, are present. These results indicate
the close relationship between A and D genomes and the presence of common D
NA sequences between A and C Avena genomes. All three clones hybridized to
Southern blots containing Arrhenatherum digested genomic DNA, indicating Ar
rhenatherum's close affinity to A, B and D Avena genomes. (C) 2000 Annals o
f Botany Company.