Diverse mechanisms of pectic polysaccharide degradation distinguished in fruit cell walls in vivo
dc.contributor.advisor
Fry, Stephen
en
dc.contributor.advisor
Halliday, Karen
en
dc.contributor.author
Othman, Babul Airianah
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dc.date.accessioned
2013-09-25T13:43:25Z
dc.date.available
2013-09-25T13:43:25Z
dc.date.issued
2012-11-30
dc.description.abstract
Cell wall loosening and degradation are important processes in major stages of plant
development including fruit ripening. Three main mechanisms have been proposed to
contribute towards cell wall polysaccharide degradation in vivo: enzymic hydrolysis
by endopolygalacturonase (EPG), enzymic elimination by pectate lyase (PL), and
non-enzymic scission by hydroxyl radicals (•OH). However, little idea as to which of
these three mechanisms predominates in homogalacturonan degradation especially
during fruit ripening. This study presents an attempt to discover the respective
contribution of those three mechanisms of attack. The strategy used to achieve the
objective of this study was to identify and measure homogalacturonan molecules that
exhibit symptoms of each mechanism of attack.
A method that was developed in this study is a fluorescent labelling method
mainly to study the •OH attack on pectic polysaccharides. This labelling method is
based on the ability of 2-aminoacridone (2-AMAC) to reductively aminate oxo
groups of sugar moieties followed by exhaustive digestion with Driselase. In a model
in-vitro experiment, the developed novel fluorescent labelling method, when applied
to homogalacturonan, that had been attacked by •OH (Fenton reagent), produced at
least three fluorescent ‘fingerprint’ compounds, separable by high-voltage paper
electrophoresis (HVPE) based on their charge/mass properties at pH 6.5 and also by
high pressure liquid chromatography (HPLC) on a C18 column with a fluorescence
detector at λem= 520 nm. These fingerprint compounds include: a monomer, 1A*; a
dimer, 2A*; and an unidentified compound, X*. In-vivo application with alcoholinsoluble
residue (AIR) of seven species of fruit (pear, mango, banana, apple,
avocado, strawberry and strawberry tree fruit) at three stages of softening produced
at least two fluorescent fingerprint compounds: a monomer, 1AF and a dimer, 2AF.
XF, an interesting compound found in a few samples in in-vivo experiments, showed
electrophoretic mobility similar to X*; however, the retention time of this compound
on HPLC did not agree with that of X*. 2AF was suggested to be exclusive evidence
for •OH attack in vivo while 1AF was suggested to be a useful evidence not only to
reveal •OH attack but also to reveal EPG and PL attack on pectic polysaccharides
during fruit softening.
HVPE and HPLC results showed an increasing pattern of 2AF in mango,
banana, avocado and strawberry tree fruit, which indicated progressive •OH attack on
pectic polysaccharides during the softening process. There was no clear evidence of
2AF at any stage of softening in apple and strawberry, which may suggest that fruit
softening in apple and strawberry was not associated with •OH attack. On the other
hand, HVPE analysis of 1AF showed and increasing pattern in pear, mango, banana,
avocado and strawberry tree fruit, which may indicate EPG, PL and/or •OH attack
during fruit softening. Production of these fluorescent fingerprint compounds
provides good evidence for •OH attack on pectic polysaccharides, and has the
potential to give useful information for EPG and PL attack in vivo.
en
dc.identifier.uri
http://hdl.handle.net/1842/7878
dc.language.iso
en
dc.publisher
The University of Edinburgh
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dc.subject
pectic polysaccharides
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dc.subject
cell walls
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dc.subject
hydroxyl radicals
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dc.subject
endopolygalacturonase
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dc.subject
pectate lyase
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dc.title
Diverse mechanisms of pectic polysaccharide degradation distinguished in fruit cell walls in vivo
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dc.type
Thesis or Dissertation
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dc.type.qualificationlevel
Doctoral
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dc.type.qualificationname
PhD Doctor of Philosophy
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