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182. Abstract
The catalytic subunit of cellulose synthase is shown to be associated
with the putative cellulose-synthesizing complex
(rosette terminal complex [TC]) in vascular plants. The catalytic subunit
domain of cotton cellulose synthase was cloned
using a primer based on a rice expressed sequence tag (D41261) from
which a specific primer was constructed to run a
polymerase chain reaction that used a cDNA library from 24 days postanthesis
cotton fibers as a template. The catalytic
region of cotton cellulose synthase was expressed in Escherichia coli,
and polyclonal antisera were produced. Colloidal
gold coupled to goat anti–rabbit secondary antibodies provided a tag
for visualization of the catalytic region of cellulose
synthase during transmission electron microscopy. With a freeze-fracture
replica labeling technique, the antibodies
specifically localized to rosette TCs in the plasma membrane on the
P-fracture face. Antibodies did not specifically label
any structures on the E-fracture face. Significantly, a greater number
of immune probes labeled the rosette TCs (i.e., gold
particles were 20 nm or closer to the edge of the rosette TC) than
did preimmune probes. These experiments confirm the
long-held hypothesis that cellulose synthase is a component of the
rosette TC in vascular plants, proving that the enzyme
complex resides within the structure first described by freeze fracture
in 1980. In addition, this study provides independent
proof that the CelA gene is in fact one of the genes for cellulose
synthase in vascular plants.
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