Maize
Genetics Cooperation Newsletter vol 86 2012
PIRACICABA,
SP, BRAZIL
ESALQ,
Universidade de S�o Paulo
Amplification of heterochromatic
knob size in callus culture by unequal sister chromatid exchange
Gardingo,
JR; Santos-Serejo, JA; Aguiar-Perecin, MLR
Tissue culture and in vitro plant regeneration systems
have provided alternative means for mass proliferation of several plant
species. Several reports have given evidence that successful plant regeneration
from maize embryo-derived callus cultures is genotype dependent (see Fluminhan
and Aguiar-Perecin, 1998). In addition, tissue and cell culture systems have
been useful for studies on the effect of stress on chromosome stability.
Chromosome breakage associated with heterochromatin regions has been observed
in plant species, as for instance the occurrence of breakpoints on chromosome
arms containing heterochromatic knobs detected by meiotic studies of
regenerated maize plants (Lee and Phillips, Genome 29:122-128, 1987). In a
previous study, we found altered chromosomes in embryo-derived callus cultures
from sister lines obtained from a Brazilian flint variety. These materials were
homozygous for knobs at the long arm of chromosomes 6 (K6L2; K6L3) 7 (K7L) and
8 (K8L), and the short arm of chromosomes 7 (K7S) and 9 (K9S); in one of these lines,
K9S was not present. Chromosome changes were detected by C-banding technique
applied to callus cells. Chromosome 7 was the most affected, and this was
interpreted as a consequence of the presence of knobs on both arms of this
chromosome (Fluminhan et al., Ann. Bot. 78:73-81, 1996). The presence of an
altered chromosome 7 with a normal long arm and a duplication
on the short arm (displaying two knobs), was explained by the occurrence of a
breakage event at K7S followed by cycles of breakage-fusion-bridge (BFB).
Interestingly, this abnormal chromosome was stable for several months in vitro,
giving evidence that healing at the chromosome broken ends had occurred. In
fact, it was further demonstrated the presence of telomeric sequences on the
termini of this chromosome (unpublished). Other type of change observed in the
chromosome 7 was the occurrence of amplification of the knob located on the
long arm.
The origin of this amplification was investigated in
further experiments, by the cytogenetic analysis of R1 progenies
resulting from regenerated plants derived from a callus culture designed 12F,
obtained from line 13342/5. Figure 1 shows C-banded mitotic prophases of
regenerated plants, respectively homozygous for the normal K7L (Figure 1A) and
heterozygous for the presence of the amplified K7L (Figure 2B). Fourteen heterozygous
plants were selfed and in the progeny, 19 amplified K7L homozygotes, 58
heterozygotes and 39 normal K7L homozygotes were recovered. The plants homozygous
for the K7L amplification survived. So, we interpreted that the amplification
of K7L would not have been derived from a BFB event as it was the case of the
change mentioned above involving the terminal knob at the short arm of
chromosome 7. The knob on the long arm is not terminal and a breakage followed
by BFB cycles would cause deletion of a significant distal region of the arm. In
a further experiment using 2-4 month-old callus cultures derived from sister
lines designated 13342/1, 13342/5, 132331 and their hybrids (references on the
lines in Fluminhan and Aguiar-Perecin, Ann. Bot. 82:569-576, 1998), we observed
metaphase cells with one of the homologues of chromosome 7 displaying an
asymmetric C-band corresponding to K7L (Figure 1C). This gave evidence that
unequal sister chromatid exchange at the knob site occurred in culture, and
would modify the knob size without disrupting gene linkage in the chromatids
involved. The frequency of this event was very low: it was detected in three
cells of two lines and one hybrid in an experiment in which 5223 C-banded
metaphases were analyzed and 2.35% presented alterations (knob amplification or
reduction) on the long arm of chromosome 7. These results are interesting not
only in the context of effects of tissue culture on heterochromatin, but also
as evidence of one of the mechanisms that must have occurred during the
evolution of maize races. For example, in a classical analysis of maize races,
McClintock, Kato and Blumenschein (Chromosome Constitution of Races of Maize,
Chapingo, M�xico, 1981) characterized several genotypes by their knob position
and sizes. This size polymorphism might have originated from unequal crossing–over
involving germ cells.
Callus culture techniques and C-band preparations were
carried out as previous described (Fluminhan et al., Ann. Bot. 78:73-81, 1996).
Figure
captions
Figure
1. C-banded mitotic prophases of plants regenerated from a two-year-old callus
culture designated 12F (A, B) and C-banded mitotic metaphase of a 2-month-old
callus culture derived from hybrid 13342/5 x 13342/1 (C). Note the normal size
of K7L in both homologues in A and a K7L amplification in B. The small arrow in
C points to chromosome 7 showing an asymmetric band on the long arm and the
large arrow indicates normal chromosome 7. Scale bar = 10�m.
Please
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